Analytical Profiles of Substances Volume 8 Edited by
Klaus Florey The Squibb Institute for Medical Research New Brunswi...
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Analytical Profiles of Substances Volume 8 Edited by
Klaus Florey The Squibb Institute for Medical Research New Brunswick, New Jersey
Contributing Editors
Norman W. Atwater Lester Chafetz Rafik Bishara Boen T. Kho Glenn A. Brewer, Jr. Hans-Georg Leemann Bruce C. Rudy Compiled under the auspices of the Pharmaceutical Analysis and Control Section Academy of Pharmaceutical Sciences
Academic Press New York San Francisco London 1979 A Subsidiary of Harcourt Brace Jovanovich. Publishers
EDITORIAL BOARD Norman W. Atwater Rafik Bishara Jerome I. Bodin Glenn A. Brewer, Jr. Lester Chafetz Edward M. Cohen Klaus Florey Salvatore A. Fusari
Derek W. Houghton Erik H. Jensen Boen T. Kho Hans-Georg Leemann Arthur F. Michaelis Gerald J. Papariello Bruce C. Rudy Bernard Z. Senkowski
Academic Press Rapid Manuscript Reproduction
COPYRIGHT @ 1979, BY ACADEMIC PRESS, INC. ALL RIGHTS RESERVED. NO PART OF THIS PUBLICATION MAY BE REPRODUCED OR TRANSMITTED IN ANY FORM OR BY ANY MEANS, ELECTRONIC OR MECHANICAL, INCLUDING PHOTOCOPY, RECORDING, OR A N Y INFORMATION STORAGE AND RETRIEVAL SYSTEM, WITHOUT PERMISSION IN WRITING FROM THE PUBLISHER.
ACADEMIC PRESS, INC.
11 1 Fifth Avenue, New York, New York 10003
United Kingdom Edition published by ACADEMIC PRESS, INC. (LONDON) LTD.
24/28 Oval Road, London NW1 7DX
ISBN 0-12-260808-9
PRINTED IN THE UNITED STATES OF AMERICA
79 80 81 82
9 8 7 6 5 4 3 2 1
AFFILIATIONS OF EDITORS, CONTRIBUTORS, AND REVIEWERS H . Y. Aboul-Enein, Riyadh University, Riyadh, Saudi Arabia A . A . Al-Badr, Riyadh University, Riyadh, Saudi Arabia T. Alexander, Food and Drug Administration, Washington, D.C. N. W. Atwater, E. R. Squibb and Sons, Princeton, New Jersey S . A . Benezra, Burroughs Wellcome Company, Research Triangle Park, North Carolina R. Bishara, Eli Lilly and Company, Indianapolis, Indiana J. I . Bodin, Carter Wallace, Inc., Cranbury, New Jersey G . A . Brewer, The Squibb Institute for Medical Research, New Brunswick, New Jersey L. Chafetz, Warner-Lambert Research Institute, Morris Plains, New Jersey Z. L. Chang, Abbott Laboratories, North Chicago, Illinois A. P . K. Cheung, SRI International, Menlo Park, California E. M . Cohen, Merck Sharp & Dohme, West Point, Pennsylvania R . D . Daley, Ayerst Laboratories, Rouses Point, New York E. Debesis, Hoffmann-LaRoche, Inc., Nutley, New Jersey K . Florey, The Squibb Institute for Medical Research, New Brunswick, New Jersey K . Furnkranz, Food and Drug Administration, Washington, D.C. S. A . Fusari, Parke-Davis, Inc., Detroit, Michigan D. A . Giron-Forest, Sandoz Limited, Basel, Switzerland P . E. Crubb, Sterling- Winthrop Research Institute, Rensselaer, New York W. F. Heyes, The Squibb Institute for Medical Research, Moreton, Wirral, England D . W . Houghton, G . D. Searle and Company Ltd., High Wycombe, Bucks, England E. Jensen, The Upjohn Company, Kalamazoo, Michigan B. T. Kho, Ayerst Laboratories, Rouses Point, New York J . Kirschbaum, T h e Squibb Institute for Medical R e s e a r c h , N e w Brunswick, New Jersey vii
viii
AFFILIATIONS OF EDITORS, CONTRIBUTORS, AND REVIEWERS
W . L . Koch, Eli Lilly and Company, Indianapolis, Indiana H. G. Leemann, Sandoz Limited, Basel, Switzerland P . Lim, SRI International, Menlo Park, California H. B. Long, Eli Lilly and Company, Indianapolis, Indiana J. W . McRae, Burroughs Wellcome Company, Research Triangle Park, North Carolina A. F. Michaelis, KV Pharmaceutical Company, St. Louis, Missouri N. G. Nash, Ayerst Laboratories, Rouses Point, New York C. E. Orzech, Ayerst Laboratories, Rouses Point, New York G. Pupariello, Wyeth Laboratories, Philadelphia, Pennsylvania L . 0. Pont, SRI International, Menlo Park, California B. Rudy, Burroughs Wellcome Company, Greenville, North Carolina W . D . SchBnleber, Sandoz Limited, Basel, Switzerland G. Schwartzman, United States Pharmacopeia, Rockville, Maryland G. Selzer, Food and Drug Administration, Washington, D.C. B. Senkowski, Alcon Laboratories, Fort Worth, Texas E. R . Townley, Schering Plough Corporation, Bloomfield, New Jersey L . Wuyland, Food and Drug Administration, Washington, D.C. C-H. Yung, Burroughs Wellcome Company, Research Triangle Park, North Carolina
PREFACE Although the official compendia list tests and limits for drug substances related to identity, purity, and strength, they normally do not provide other physical or chemical data, nor do they list methods of synthesis or pathways of physical or biological degradation and metabolism. For drug substances important enough to be accorded monographs in the official compendia, such supplemental information should also be made readily available. To this end the Pharmaceutical Analysis and Control Section, Academy of Pharmaceutical Sciences, has undertaken a cooperative venture to compile and publish Analytical Profiles of Drug Substances in a series of volumes of which this is the seventh. The concept of analytical profiles is taking hold not only for compendia1 drugs but, increasingly, in the industrial research laboratories. Analytical profiles are being prepared and periodically updated to provide physicochemical and analytical information of new drug substances during the consecutive stages of research and development. Hopefully, then, in the not too distant future, the publication of an analytical profile will require a minimum of effort whenever a new drug substance is selected for compendial status. The cooperative spirit of our contributors has made this venture possible. All those who have found the profiles useful are requested to contribute a monograph of their own. The editors stand ready to receive such contributions. Thanks to the dedicated efforts of Dr. Morton E. Goldberg, a long cherished dream has come to fruition with the publication of Pharmacological and Biochemical Properties of Drug Substances, M. E. Goldberg, editor, published by APhA Academy of Pharmaceutical Sciences. This new series supplements the comprehensive description of the physical, chemical, and analytical characteristics of drug substances covered in Analytical Profiles of Drug Substances with the equally important description of pharmacological and biochemical properties. ix
X
PREFACE
Drug substances appearing in the new series will be cross-referenced in the cumulative index. The goal to cover all drug substances with comprehensive monographs is still a distant one. It is up to our perseverance to make it a reality. Klaus Florey
Analytical Profiles of Drug Substances, 8
ASPIRIN Klaus Florey I . Introduction 1 . 1 Foreword 1.2 History 2. Description 2. I Name, Formula, Molecular Weight 2.2 Appearance, Color, Odor 3. Synthesis 4. Physical Properties 4.1 Spectra 4.11 Infrared 4.12 Ultraviolet 4.13 Fluorescence-Phosphorescence 4.14 Raman 4.15 Nuclear Magnetic Resonance 4.16 Mass 4.2 Solid Properties 4.2 I Melting Range 4.22 Differential Thermal Analysis 4.23 Thermogravimetric Analysis 4.24 Crystal Properties 4.3 Solution Properties 4.3 I Solubility 4.32 Dissociation Constant (pKa) 4.33 Partition Coefficients 4.34 Dielectric Constant, Dipole Moment 4.35 Radiation Absorption 5. Methods of Analysis 5.1 Historical Synopsis 5.2 Identity and Color Tests 5.3 Quantitative Analysis 5.31 Elemental 5.32 Colorimetric 5.33 Ultraviolet 5.34 Infrared 5.35 Fluorescence-Phosphorescence 5.36 Titrimetric-Electrochemical 5.37 Miscellaneous (NMR) 5.4 Chromatographic Methods 5.41 Paper 5.42 Thin-Layer 5.43 Column I
Copyright @ 1979 by Academic Press, inc. All rights of reproduction in any form reserved. ISBN 0-12-260808-9
2
KLAUS FLOREY 5.44 High Pressure Liquid 5.45 Gas-Liquid 5.5 Electrophoretic Methods 5.6 Determination of Impurities 5.61 Salicylic Acid 5.62 Acetic Acid 5.63 Acetylsalicylic Anhydride and Acetylsalicylsalicylic Acid 6. Stability-Degradation 7. Pharmacokinetics-Drug Metabolism Products 8. Bioavailability-Dissolution 9. Determination in Biological Fluids and Tissues 10. Determination in Pharmaceutical Preparations 1 1 . Acknowledgments 12. References
ASPIRIN
3
Introduction 1.1 Foreword The writing of an analytical profile of aspirin, this drug of drugs, poses two major dilemmas. The first is in the name itself. There are many countries where Aspirin is still a tradename of the German firm Bayer AG, and Acetylsalicylic Acid is used as the generic. Yet, I decided to use the former because it is the U . S . P . and B.P., the better known worldwide and the more elegant name. Aspirin has now been available for close to 80 years, and its usefulness and popularity are undiminished. Consequently, the literature is voluminous and also undiminished. A complete coverage would be beyond the scope of an analytical profile. I have endeavored to cover the newer literature as comprehensibly as possible and have included only those older references which I found of historical interest. To all those who have labored in the vineyard of aspirin and who go unreferenced in this profile, I tender my sincere apologies. 1.
1.2
Bistor d u m e n t e d facts of the discovery of aspirin are quickly told. It was synthesized-by the German chemist Felix Hoffmann (1868-1946) in the laboratories of Farbenfabriken Bayer, Elberfeld, Germany in 1897 (Fig. 1). The compound was tested pharmacologically by H. Dreser' and clinically among others by Wohlgemuth and Witthauer3 who documented the antirheumatic, antipyretic and analgesic properties free of the undesirable side effects of salicylic acid. Apparently, there was some initial reluctance at Bayer to market the new compound since it was thought that the field was already crowded with new drugs. But opposition faded when the new drug got the support of Carl Duisberg, then the general manager of Bayer. Duisberg, of course, was the great chemist and industrialist who built Bayer into the chemical giant of world renown. After the inspired trade name Aspirin, a contraction of acetyl and "spirssure" (salicylic acid), was coined in the offices of Bayer - Euspirin was also considered and fortunately discarded4 -it was marketed in tablet form in 1899 and conquered the world.
KLAUS FLOREY
44
-. .. .
&...
. ,.,... . .
.
..
.
'
,
.
..I .
F i g u r e 1.
L a b o r a t o r y notebook e n t r y of F e l i x Hoffmann, d e s c r i b i n g h i s f i r s t p r e p a r a t i o n of a s p i r i n . The i n i t i a l s CD o n t h e p a g e are t h o s e of C a r l D u i s b e r g . ( C o u r t e s y of Bayer A . G . , L e v e r k u s e n , Germany)
ASPIRIN
5
What motivated Hoffmann to undertake this momentous synthesis? Legend has it that he wanted to help his father who was suffering from rheumatism and who was no longer able to tolerate sodium salicylate, then widely used in rheumatic and arthritic diseases. Salicylic acid occurs naturally in several plants. The analgesic and antipyretic properties of willow bark were already known in antiquity to Hippocrates and the blossoms of spiraea ulmaria (meadow sweet) were used in the middle ages. Salicylic acid was crystallized from willow bark extracts in the early years of the last century, and Kolbe, in 1859, was able to synthesize it from sodium phenolate and carbon dioxide. His student von Heyden worked out a commercially feasible process and started a factory to produce salicylic acid which made possible its widespread use in rheumatic diseases. However, its bad taste, stomach irritation and other side effects were a strong incentive to search for derivatives which retained its efficacy without its disadvantages. Acetylation of the hydroxyl group was one of the logical modifications. Acetylated salicylic acid had already been described three times in the literature (see Section 3 ) . Von Heyden and possibly also Merck, Darmstadt,are reputed to have experimented with aspirin without being able to produce the pure drug. At the time when Felix Hoffmann prepared pure aspirin successfully in the Bayer laboratories, one of his colleagues was Arthur Eichengrun, who had been hired by Carl Duisberg in 1896, while Hoffmann had been hired in 1894. Eichengrun,as an old man, had to undergo the horrors of the infamous Nazi concentration camp in Theresienstadt which he survived. In 1949, Eichengrun published his memoirs relating to the invention of aspirin5 which was then a half-century old. He claimed that it was he who told Hoffmann to prepare acetylsalicylic acid. Acetylation certainly was on Eichengrh's mind, since he had also experimented successfully with the acetylation of cellulose about the same time. He went cn to fame as the inventor and developer of rayon and safety film. Eichengrcn also claimed that anothercolleague of Bayer, the pharmacologist Dreser, opposed clinical trials. However, the memory of the 82 year-old Eichengrun must have been faulty when he
KLAUS FLOREY
6
wrote these rather bitter reminiscences concerning Hoffmann's, Dreser's and his own role in the discovery of aspirin because, in 1913, Eichengrun wrote a chapter on "The Pharmaceutical Research Laboratory" in the book History and Development of Farbenfabriken Bayer, V o r m . Friedr. Bayer & Co., Elber?eld by F. Fischer, 1913'+, where he laid no paternity claim to aspirin and described Dreser's role correctly. The pertinent passage (p. 412) translates as follows: "Acetylsalicylic acid, prepared by Felix rested unnoticed for 1+ years Hoffmann among thepreparations rejected by the pharmacological laboratory until in 1898,during unrelated investigations, Dreser's attention was again drawn to it. On account of the observation that the acetyl compound was increasing cardiac activity in contrast to salicylic acid itself, he recommended a clinical trial of the product . . . . I '
........
Felix Hoffmann did not publish his version of the discovery, nor did he obtain a German patent, since the synthesis had been previously described. Farbenfabriken Bayer did obtain a U.S. Patent6 in 1900 which named him as the inventor. Chemical Abstracts reveal no subsequent publications by him, nor is there any record that he was publiclyhonored for his contribution. However, in 1899, he was appointed director of the pharmaceutical research and marketing division of Bayer. He retired in 19287. In many ways, the story of the discovery of aspirin is typical for the way in which new drugs are invented and developed in pharmaceutical research laboratories, where many individuals have to make a contribution and where it is often difficult to fathom completely what thought processes, suggestions and interactions lead to a successful new drug. Description 2.1 Name, Formula, Molecular Weight Aspirin is acetylsalicylic acid, also salicylic acid acetate and 2-(acetyloxy)-benzoic acid (50-78-2). The last name is currently popular in Chemical Abstracts. 2.
ASPIRIN
‘gH8’4
M.W.
180.16
Appearance, Color, Odor Aspirin is a white, crystalline powder. It is odorless but might have a faint odor of acetic acid. 2.2
S nthesis h synthesis of aspirin is credited to Gerhardt* in 1853. Gerhardt was investigating
3.
mixed organic acid anhydrides and, among others, reacted acetylchloride with sodium salicylate. He obtained a solid product, undoubtedly impure acetylsalicylic acid,which immediately and without further characterization he hydrolyzed with aqueous sodium carbonate to salicylic and acetic acids. Next it was prepared by reaction of salicylic acid with acetylchloride by H. von Gilmg in 1859, who described a crystalline product. In 1869, K.Krautlo had a student, A . Prinzhorn, prepare acetylsalicylic acid by the methods of Gerhardt and von Gilm and obtained an identical product by both methods with a reported melting point of 118.5O. Kraut also correctly observed that the product is not an acid anhydride as assumed by Gerhardt but rather a phenolic ester. Felix Hoffmann6 used acetic anhydride for its preparation. CH 3,COC1
(gooH +
OH
or
CH CO 3 \ CH3CO” or CH2=C0
catalyst
KLAUS FLOREY
8
Essentially, all methods of synthesis are variations of the reaction of acetylchloride, acetic anhydride or ketenell with salicylic acid using a variety of catalysts such as pyridine12 or sulfuric acid13 and reaction conditions (c.f. 14). The preparation of aspirin labeled with a 14C-labeled acetyl group has also been reported.15 Efforts to improve the commercial processes continue to the present day. 4.
Physical Properties 4.1 Spectra 4.11 Infrared The assignment of the KBr infrared spectrum (Figure 2) of aspirin (U.S.P. reference standard #0675-F-4) is summarized in Table 1.16 It agrees essentially with a spectrum published previ~usly?~A reflection spectrum has also been presented.
*
TABLE 1 Infrared Spectrum Interpretation Wavelength (c m-') 2300-2500 1760 1690 1490 1220 1 1190 760
Assignment carboxyl OH vinyl ester C=O aromatic acid C=O aromatic C=C stretch =C-0 (acid and ester) ortho subst. phenyl C-H bending
4.12
Ultraviolet Aspirin in 0.1N sulfuric acidlg and in dilute1trichloroacetic acid20 exhibits maxima at 229 nm (El 484) and 276 nm (E 65.5) .1 In chloroform a maximum was found at 2 7 nm (El 68).21 Fluorescence - Phosphorescence The native fluorescence of aspirin, in contrast to salicylic acid, is a weak one and has been studied only recently.22 Excitation wavelength maximum is at 280 nm and emission maximum is at 335 nm. Maxima for salicylic acid are at 308 and 450 nm respectively. 4.13
id
rd
aE
KLAUS FLOREY
10
The phosphorescence emission maximum was found at 410 nm.23 4.14
Raman. Raman spectra are described and discussed in the following references: 24, 25 4.15
Nuclear Magnetic Resonance The 60 and 100 MHz proton macrnetic resonance spectra of aspirin have been published as part of a n a l y t i ~ a l ~and ~-~ biochemical ~ studie~.~O?~l The 100 MHz pmr spectrum of a deuter ochloroform solution containing tetramethylsilane as an internal reference was obtained on a Varian Associates XL-100-15 spectrometer equipped with a Nicolet pulsed Fourier accessory. 3 2 (Figure 3 ) The rms error for the experimental and calculated spectra shown in Figure 4 is 0.2. The proton assignment is shown below. 6 J = 8.05Hz H1 12.04 3?4 = 1.34Hz J H* 2.34(3H) 3?5 J3,6 = 0.3Hz H3 7.13 J = 7.80Hz H4 7.61 4?5 = 1.74Hz J H5 7.33 4?6 = 7.96Hz J H6 8.11 5?6
.
The differences in the pmr spectrum previously reported in aqueous media30 are attributed to the solvent used. The proton-proton couplings of the aryl protons are virtually identical, however. The fully decoupled I3C-NMR spectrum of aspirin in CD30D (200 mg/ml) is shown in Figure 5. The spectrum was obtained on a Varian XL-100-15 NMR spectrometer equipped with a Transform Technology TT-100 FT data system. The data represent the transformation of a 400 pulse FID obtained using 4096 data points with a 15 second delay time between accumulations.33 Peaks a-i (Figure 5) arise from the nine carbons of aspirin. The seven peak multiplet centered at 6=49.0 ppm
12.0
11.0
10.0
9.o
8 .O
7.0
6.0
5.0
4 .O
3.0
2.0
I.o
PPM
Figure 3.
100 MHz PMR Spectrum of Aspirin.
Instrument:
Varian XL-100-15
0.o
- -
c
=z
12
d
k
-4
a
-4
2 rCI
0 Id
)-I
a,
u
+J
a p:
v)
E
a
Id
a, 4J
I
rl
u
u
Id
rl
Id
c
a a
a,
Id
4J
2
rl
m
-4
a,
w
m
k 3
kl
.rl
13
6,
5
.-
KLAUSFLOREY
14
arises from the solvent. Assignment of each of the peaks can be made on the basis of their chemical shifts and the coupling information summarized in Peak a is the sole peak in the aliphatic Table 2 . region of the spectrum and is, therefore, assigned to methyl carbon (C-9). As expected, the fully coupled spectrum exhibits four peaks in this region - - - and f can with a 'JCH of 130 + 2 hz. Peaks b,d,e be assigned to the Four singly protonated aromatic carbons Each is strongly coupled to one proton ~ '65 ~ + 2 hz. Weak long range coupwith a i J of - - - and f can be ling can also be observed. Peak b,d,e assigned to carbons 3,5,6 and 4, respectivery by comparison of their chemical shifts to values predicted on the basis of substituent effects observed in model systems. Peaks c,g,h and i must arise from non-protonated carbons since they do not exhibit appreciable splitting in the fully coupled spectrum. Chemical shift predictions based on substituent effects enable assignment of peaks c and 2 to the C-1 and C-2 aromatic ring carbons, respectively. The remaining peaks h and i must arise from the carbonyl carbons. Comparrson 07 their respective chemical shifts to those of model compounds suggest their assignment to the carboxyl (C-7) and a-cetoxy carbonyls (C-81, respectively. This assignment is confirmed by the observation of a long range coupling of peak i to the three protons of the methyl group. TABLE 2 l3C-NMR Data for Aspirin Assignment Jcab Multiplicityb Peak G(ppm)a Carbon # 21.6 124.6 124.9 126.9 132.6 134.7 151.9 167.4 171.2
9 3 1 5 6 4 2 7 8
a) ppm from TMS external via the relationship 6 (CD30D)=49.0 ppm. b) obtained from the fully coupled spectrum.
ASPIRIN
c) none observed. m) weakly coupled multiplets due to long range effects. 4.16
Mass The low resolution mass
spectrum was obtained on an AEI MS-902 double-focussing mass spectrometer equipped with a frequency-modulated analog tape recorder at a source temperature of looo C. above ambient (approximately 1300 C.). 32 By adjusting the sample flow and the electron multiplier gain, the maximum sensitivity was obtained without clipping the most intense peak. The recorded analog spectrum was processed on a PDP-11.34 Except for differences in the intensity of the molecular ion (M’), the intensities shown in Figure 6 are virtually identical to the previously published spectrum.35 Differences could be ascribed to instrument design, source temperatures or even source design. The assignment of a number of fragment ions of the mass spectrum is shown in Figure 7. Figure 7.
120
+H 138
m* 104 3 m/z 138 -H20
92
‘HCO -m/z
m/z 120
m/z 64 63
The metastable ion at m/z 104.3 supports the loss of the elements of water from the m/z 138 rearrangement ion.
KLAUS FLOREY
16
5292 R S P I R I N 03-RUG-78
MF16761
100 30
90 >IH
cn
Z W IZ H
W
>
H
l-
a
-I W rY
80
25
70
W : Z
0 H
I-
a
kl H
60
20
Z
0 H
50
_I
15 a I-
40
cj
I-
30
10
I-
Z W
0
20
5
10
a: W
a
0
I N T E N S I T Y SUM = 4 0 1 4 0
Figure 6.
BRSE PERK X = 3 3 . 0 7
Mass Spectrum of Aspirin. Instrument: AEI MS 902
ASPIRIN
17
The mass spectrum of aspirin has been used as an aid in the rapid identification of toxic materials isolated from urine, blood or gastric aspirates of drug abuse patients.36r37 4.2
Solid Properties 4.21 Melting Range The melting point of aspirin is nothing very definitive having variously been given between 118-144°38 and a good deal of work has been done to get the best methods for compendia1 Early commercial preparation melted around 135°.44 The European P h a r m a ~ o p e i agives ~~ a melting point of 141° to 144O as determined by the instantaneous method. For further discussion, see Polymorphism (Section 4.242)
.
4.22
Differential Thermal Analysis When aspirin (USP reference standard) was heated at a rate of 15O/min. in air, a single endotherm was observed with a T onset=1340 and T peak = 139°.46 DTA and TGA patterns of aspirin have also been previously studied4&nd used for forensic drug identification.48 4.23
Thermogravimetric Analysis When aspirin (USP reference standard) was heated at 20°/min. and a N2 flow of 20 cc/min.,no weight loss was observed at less than 1300. 4.24
Crystal Properties 4.241 Single Crystal X-Ray Diffraction The crystal structure of aspirin was determined by Wheatley.49 The monoclinic crystals have a space group of P21/C. The dimension of the unit cell are: a=11.446A; b=6.596A; c=11.388 A; ~ = 9 5 033'; n=4. 4.242
Powder X-Ray Diffraction The powder x-ray diffraction pattern of aspirin is presented in Table 3 and Figure 8. 5 0 4.243
Polymorphism Tn 1968, Tawashi5' claimed that aspirin exists in several polymorphic forms.
a,
0
aJ
8k
2
W
.
PI
4
4 0
W
aJ
k
ASPIRIN
19
TABLE 3
P o w d e r X-Ray D i f f r a c t i o n P a t t e r n o f A s p i r i n (U.S.P. Reference S t a n d a r d )
20 (Deg . I 7.80 14.09 15.63 16.78 18.19 20.63 20.95 21.53 22.56 23.20 25.00 27.05
D
(b)
11.3 6.25 5.68 5.28 4.88 4.30 4.22 4.12 3.93 3.83 3.55 3.30
R e l at i v e
Intensity 0.539 0.033 1,000 0.087 0.038 0.079 0.035 0.030 0.268 0.210 0.033 0.427
20 (Deg . I 27.56 28.85 29.62 30.26 31.54 32.57 33.85 34.50 36.04 36.55 37.45 39.37
R el ati v e . .
3.23 3.08 3.02 2.96 2.84 2.74 2.67 2.60 2.50 2.46 2.40 2.29
Intensity 0.054 0.068 0.040 0.039 0.120 0.110 0.051 0.037 0.049 0.048 0.034 0.038
This started a f l u r r y of a c t i v i t y . DeBis~chop~~ claimed t o have o b t a i n e d t h r e e d i f f e r e n t c r y s t a l forms b u t s t r e s s e d t h a t t h e o n l y s t a b l e one i s t h e monoclinic one m e l t i n g a t 142O C . However, t h e c l a i m f o r t r u e polymorphism of a s p i r i n w a s u e s t i o n e d o r ref u t e d i n several l a b ~ r a t o r i e s ~ ~and - ~ c%a n be b e s t summarized i n t h e words o f G . Schwartzman:57 " I t i s g e n e r a l l y a c c e p t e d t h a t t r u e polymorphism r e s u l t s i n d i s t i n c t o p t i c a l and s p e c t r a l p r o p e r t i e s . The data p r e s e n t e d a r e e n t i r e l y n e g a t i v e i n t h e s e r e s p e c t s . The e v i d e n c e accumulated a g r e e s w i t h t h e f i n d i n g s o f P f e i f f e r 5 5 and q u e s t i o n s t h e f o r m a t i o n of a s p i r i n polymorphs. W e believe t h a t the d i f f e r e n t crystal habits w e r e c a u s e d by t h e s o l v e n t s used f o r c r y s t a l l i z a t i o n . The d i s s i m i l a r m e l t i n g p o i n t s a r e probabl y due t o t h e poor t r a n s f e r of h e a t caused by the larger crystal s i z e o r t o possible crystal d e f e c t s . I'
4.244
Optical Constants A s p i r i n h a s been d e s c r i b 8=95O ed a s m o n o c l i n i c , a:b:c = 1.7322:1:1.7322, 8=1.6424 4.25'. I n d i c e s f o r 576 p p a r e : d=1.5042;
KLAUS FLOREY
20
and 2=1.6554; 2V=15' 46'. The optical plane is normal to (010) and lies in obtuse angle f3.58 Very similar constants are presented in reference 41. Polarized Crystal Absorption Spectrum The polarized absorption spectrum of a single crystal of aspirin was measured which indicated that aspirin may be spectroscopically treated as perturbed benzoic acid.59 4.245
Calorimetry The heat of combustion at constant volume was determined as 859.3 kcal/Mol.60 Aspirin tablets make good samples for use in oxygen bomb calorimetry.61 4.25
4.3
Solution Properties 4.31 S ~ l u b i l i t v ~ ~ ' ~ ~
g/ml Water at 25' 0.0033 Water at 37O 0.01 Water at 100' 0.03 0.2 - 0.4 Ethanol Chloroform 0.025 - 0.06 Carbon tetrachloride 0.0004 0.1 - 0.2 Ether Abs. ether sparingly soluble Benzene 0.0033 Petroleum ether insoluble The solubility in polyethylene glycol 400 and in aqueous solution of other polyethylene glycols has been described.65-66 The effect of selected surfactants above and below the critical micelle concentration (CMC) on aspirin solubility6 was studied. Dissociation Constant (pKa) In 1913, Springer and determined the dissociation in-aqueous solution at various temperatures. At 25O they determined the (pKa 3.55). The dissociation constant as 2.8 x Merck Index62 gives a value of 3.27 x (pKa 3.49) at 25O. When the apparent pKa was de4.32
ASPIRIN
21
termined in DMF, using quaternary butyl ammonium hydroxide as the titrant, the pKa observed depended on the solvent of crystallization. From ethanol (m.p. 140-142O) , a value of 8.99; from hexane (m.p. 121-124O), a value of 9.19 was obtained. The latter higher value was ascribed to internal hydrogen bonding of the carbonyl to the hydroxy group.69 This apparent pKa should not be confused with the true pKa of 3.5 (see above). Partition Coefficients When aspirin was partitioned between buffers pH 1-7 and octyl alcoho1,partition coefficients ranging from k=17.7 (pH 1) to k=0.025 (pH 7) were obtained.70 Earlier, coefficients of 0.32 in to1uene:water and 1.81 in ch1oroform:water were determined.71 4.33
4.34
Dielectric Constant, Dipole Moment
Dielectric constant: fb 2.35 5 to 7
Dipole Moment: 2.09
-
Ref. 72 73 74
5.65 calc.; 4.36 observed 0.93 (acc. to 75 Onsager by immersion)
Radiation Absorption The absorption coerricient of a collimated beam of 6oCo z-radiation was determined for aspirin. See reference 76 for details. 4.35
Methods of Analysis 5.1 Historical Synopsis As the following pages of this section will show, there is hardly a new method of analysis which is not immediately tried for the determination of aspirin as such, or in formulations and biological fluids. The analysis of aspirin is intricately interwoven with that of salicylic acid, its precursor and degradation product. From the very first,residual salicylic acid was determinedby the convenient reaction with ferric salts --typical for phenols -- which give a violet complex with salicylic acid. In spite of the plethora of methods, the 5.
22
KLAUS FLOREY
compendia1 approach to determine purity and strength of aspirin has been very conservative. A monograph for aspirin was introduced into U.S.P. not earlier than Volume X (1926) and has not been changed in its essentials for the last fifty years; Aside from such niceties as ash, carbonizable substances, chloride, sulfate and heavy metals, the mainstays then (U.S.P. X, 1926) and now (U.S.P. XIX, 1975) are: a) identification by a color test with ferric chloride after heating, saponification to salicylic acid, identified as a white precipitate and an odor test (ethyl acetate), b) residual salicylates as determined by a color matching test with ferric ammonium sulfate with a 0.1% limit and c) an assay involving saponification to salicylic and acetic acids and back titration of excess alkali with a purity specification of 99.5 to 100.5%. The European P h a r m a c ~ p e i auses ~ ~ essentially the same analytical methods as U.S.P. In contrast to aspirin itself, the U.S.P. monograph for aspirin tablets has undergone considerable changes. For some reason, U.S.P. does not use the ferric salt test for free salicylic acid, as does the British Pharmacopeia of 1973. Apparently, certain excipients such as citric and tartaric acid interfere with this reaction.77 Already in 1913, a double titration method was developed78 which was made an official method in 1926.79 This method was used as the assay method when the aspirin tablets monograph was introduced into U.S.P. XI1 in 1942. For identification, the same two tests as for aspirin itself were prescribed then (U.S.P. XII) and now (U.S.P. XIX) ; however, due to the pioneering work of Higuchi, Banes, Smith and Levine in the ' ~ O ' S ,a ~ ~ test for non-aspirin salicylates was introduced using a siliceous earth column for separation from excipients and aspirin, and spectrophotometric finish at 306 nm. A limit of 0.3% is specified. The same column method with different eluting solvents and a spectrophotometric finish at 280 nm is used for the assay with limits of 95 tb 105 percent. 5.2 Identity and Color Tests Aspirin can be identified by the following name tests:
ASPIRIN
23
Test Color Ref. Trinder's reagent Purple after hydrolysis 63 McNally's test Red 63 Mandelin's reagent Green with blue 81 (Ammonium vanadate ) tint; changes to red-violet Feigl Saponif. to salicylic 82 acid. Reaction with KOH at 130°: Violet fluorescence Kulberg Saponif. to salicylic 83 acid. Addition of FeC13 in HC1: red-violet coloration Vitali Morin Orange to red 84 Kofler Microscopic Identifi85 cation
For identification by infrared, see Section 4.11. Identification in combination products by mass spectrometry has been described.86 5.3
Quantitative Analysis 5.31 Elemental The percent of carbon, hydrogen and oxygen is as follows:62 % (theoretical) 60.00 c9 4.48 H8 35.53 O4 5.32
Colorimetric The use of basic organic dyes for ion pair extraction-photometric determination has been described.87 After ammonia treatment,,an orange-red color with CuSoq and H202 (Deniges) can be quantitated.88 A water insoluble violet complex ( X max. 620 nm) with 2-picoline-Cu(II) has also been reported.89 5.33
Ultraviolet The maximum at 277 nm has been used to determine aspirin in tablets after chromatography (see Section 5.43). It also has been used to determine aspirin in mixtures with other drugs (cf. 21). For simultaneous determination of
KLAUS FLOREY
24
aspirin and salicylic acid, see Section 5.61. 5.34
Infrared The infrared spectrum has been used to determine aspirin in combination products. Accuracy of 1-2% has been claimed (cf. 90,911. For aspirin, the absorption maximum at 1765 cm-1 has been used.92 Fluorescence - Phosphorescence Although fluorescence of aspirin, as contrasted to that of salicylic acid, is weak (see Section 4.13), it has been used for the determination in tablets.2 2 Phosphorimetry (see Section 4.13) has been described as useful in the determination of aspirin in blood serum and plasma.23 Since the phosphorescence of salicylic acid at the maximum of 410 nm is about 500 times weaker, it does not interfere. 5.35
Titrimetric - Electrochemical Although theoretically aspirin could be titrated directly with alkali, this tends to give inaccurate results due to its instability in alkali and, therefore, the compendia1 methods back titrate after saponification (cf. 7 9 ) . However, non-aqueous titration is possible and desirable, particularly for determination in combination products. Sodium methoxide in benzene-methanol is used as the titrant and methylisobutyl ketone as the solvent. The end point is determined potentiometrically.93 Alternately, tetrabutyl ammonium hydroxide and DMF as titration solvent have also been used.94,95 Titration in ethylene diamine has also been described.96 Potentiometric measurements of ion-pair association and selective acid stren th in ethylene diamine and water has been reported.7 7 Potentiometric titration in aqueous medium has also been described9* as has colorimetric.99 5.36
The direct current and alternating current polarographic response of aspirin in an a aprotic organic solvent system (acetonitrile - 0.1M tetrabut 1 ammonium perchlorate) has been studied.Y0 The following values were obtained: 1. dc half-wave potential: E%= -1.64 2. ac fundamental harmonic peak potential: Ep = -1.76
ASPIRIN
25
3. ac second harmonic minimum potential: E min = 1.87 n values calculated from the three modes are: 0.44; 0.45 and 0.40. Approximate detection limits (moles/liter) for the three modes are: 5 x 10-5; 1 x 10-4; 1 x 10-4. On a rotating disk electrode, aspirin was reduced to the aldehyde.lo1 5.37
Miscellaneous (NMR) Nuclear magnetic resonance spectrometry has been used to quantitate aspirin in a combination product with a coefficient of variation of 1.1.1°2 For quantitation, the shift at 2.3 ppm representing the ester methyl group was used. 5.4
Chromatographic Methods 5.41 Paper Paper chromatographic systems have been tabulated in Table 4 . TABLE 4 Solvent systems: Pet-ether, Methanol, Benzene and Water (25:20:20:0.05) Iso-propyl alcohol, Water, Ammonia (15:85: 10) Methanol, Water, Ammonia (10:90:10) Butanol, 25% Ammonia (4:1) 0.75% Nitric Acid *RfA
=
aspirin; RfS
=
RfA* RfS* -
Detection
Ref.
0.05
-
FeC13
103
-
-
FeC13
104
-
-
FeC13
104
0.45 0.8
0.6
U.V. 105 Fluorimetry 106
salicylic acid.
Cellulose anion-exchange paper chromatography with 5 % acetic acid-n-propanol (5:l) gave good separation,detected by U.V. light, of aspirin ( R f . 0.07) from salicylic acid ( R f . 0.51) . l o 7
KLAUS FLOREY
26
5.42
Thin Layer TLC has been used to identifv and quantify aspirin in pharmaceutical preparations and body fluids. Data have been summarized in Table 5. Readout by d e n s i t o m e t e r ~ ~and ~ ~ TLC , ~ ~separation ~ as student experimentsllO have also been described. 5.43
Column mentioned in the historical synopsis (Section 5.1) , Levine perfected the compendia1 partition column procedure in which aspirin in chloroform is first trapped in an immobile phase of sodium bicarbonate on a column of siliceous earth (celite) then eluted with a solution of acetic acid in chloroform and measured spectrophotometrically. This has been also used for separation in combination products.80 For the determination of salicylic acid in presence of aspirin by this method, see Section 5.61. Ion exchange columns filled with strongly or weakly basic anion exchange resin in the acetate or chloride cycle have also been used for se aration of aspirin ,724 This has also in combination products. 2 2 I been adapted for a student experiment.125 A Sephadex-G25 column has been used for the separation of aspirin from salicylic acid. As
5.44
High Pressure Liquid This newest of chromatographic techniques has already been used quite-extensively for the determination of aspirin in pharmaceutical products. Separation on columns filled with anionexchange resin127 or cation-exchange resin with and without counter ions128r129were investigated in detail. Silica surface columns have also been used130 as have been reverse phase (octadecyl) ones!31-134 U . V . detection was used throughout. 5.45
Gas-liquid Determination of aspirin by qaschromato raphy was first reported by Hoffkan and Mitchellq35 in 1963 who separated it from other tablet ingredients by direct chromatography on tetrafluoroethylene polymer coated with Dow-Corning silicone, using a flame ionization detector and an integrator. A glass-bead column, coated with carbowax and isophthalic acid has also been used.136 Most other investigators made the methyl- or trimethylsilyl-derivative prior to chromatography. A s
TABLE 5 Thin Layer Chromatography of Aspirin Support Silica Silica Gel G Silica Po1yamide Polyamide Polyamide Polyamide Silica Gel G Polyamide
Silica Gel G
Solvent System MeOH-HOAc-Et2O-CgH6 (1:18: 60/120) Et20-AcOEt (1:4) C6H6-HOAC-MeOH-CHC13Pet-ether CH3C13-C6H6-90% HC02H (5:l:O.l) iso-PrOH-H20-90% HC02H' (1:5: 6: 01) CH3C13-90% HC03H (20:0.1) Cyclohexane-CHC13-HOAc (4:5:1) Cyclohexane-CHC13-HOAc (50:40:10) CHC13-Cyclohexane-HOAcDioxane (40:60:1:10) CHC13-Cyclohexane-HOAc (40:60:1) EtOH-IsoProOH-XyleneCHC13 (12.5:12.5:25:50)
Rf.Asp.
Rf.Sa1.
QJo.9
-
0.26
'
-
Detection
W
Ref.
-
111 112
0.42
0.44
w
113
0.44
0.24
W
114
0.32
0.08
w
114
0.47
0.24
W
114
0.61
0.41
w
114
0.36
-
K4(Fe(CNa))3
115
0.48
0.14
W
116
0.37
0.12
w
116
Iodine
117
0.04
-
TABLE 5 (continued) Support
Solvent System
Rf.Asp.
Rf.Sa1.
Detection
Ref.
NH4 Vanadate NH4 Vanadate
118 118
CHC13-(CH3)2C0 (9:1) MeOH NH3(100:1.5)
0.075 0.75
-
Silica Gel GF
EtOAc-t-PrOH-NH3 (40:30:3)
0.25
S i l i c a Gel GF
E ~ O H - H O A C - H ~ O(60:30:10) CgHg
0.92 0.10
-
-
-
Silica
-
Silica Gel GF Silica Gel 6 0
C6Hg-Dioxane-HOAc ( 6 0 : 20: 2)
-
W W
w
119 119 119
Fluorimetry
120
ASPIRIN
29
meth lating agents, diazomethane in ether alcohollY7 or tetrahydrofurane, 3 8 methanol with boron t r i f l ~ o r i d e land ~ ~ methyl iodide with potassium carbonate140 were used. For trimethylsilylation hexamethyl disilazane,141-143N-0-bis(trimethy1silyl) acetamide and other trimethylsilyl BSTFA145-146and MSTFA147 have been tried. It was noted that derivatization with BSTFA or MSTFA resulted in slight hydrolysis of aspirin.147 Electrophoretic Methods Aspirin can be separated from salicylic Separation acid by ionophoresis at a pH of 4-5.14* of aspirin in combination products has been achieved with paper strip electrophoresis, ysinq4$uffers at pH 2-8 and a 200 V. applied potential. Aspirin was separated from metabolites by paper electrophoresis in a phthalate buffer of pH 3.2 and an ionic strength of 0.0125-0.0500.150 5.5
Determination of Impurities 5.61 Salicylic Acid As has alreadv been pointed out, the determination of salicylic acid is intricately‘ interwoven with that of aspirin itself. There is the convenient color reaction with ferric chloride which was already used by Dreserl to determine free salicylic acid in his own urine after the ingestion of aspirin. However, this reaction is not too specific and considerable work has gone in the development of interference free methods. 5.6
My task has been made easy since there is an excellent review by C.A. Kelly151 on the determination of salicylic acid in aspirin and aspirin products. A more recent review has been compiled by S.L. Ali.152
I , therefore, have restricted my tabulation of methods to those references which discuss determination of salicylic acid in biological specimens, which were not covered by Kelly, to important references which have been published since the Kelly review and references which are pertinent to other sections of this profile. References for the determination of salicylic acid: 1. Colorimetric (iron complex): 77,78,153,154 (Folin-Ciocalteu reagent): 218,219
KLAUS FLOREY
30
Nonaqueous titration: 104 Iodometric: 131 Spectrophotometric: 20, 156-158 Fluorometric: 22,159,160 Infrared: 92 Column: 57,137,138,103 PC (for Rf values and solvent systems see Section 5.41): 106,107 9. TLC (for Rf values and solvent systems see Section 5.42): 114,116,119 10. VPC: 106,107,140,141,144,145,146,147 11. HPLC: 152,164 12. Automated: 165-167 2. 3. 4. 5. 6. 7. 8.
5.62
Acetic Acid It is easily forgotten that aspirin degrades to acetic as well as salicylic acid. And, indeed, any smell aspirin might have is due to acetic acid. However, the volatility of acetic acid does not make the determination of acetic acid a reliable tool to measure stability or degradation. A.N. Smith in 192016* devised a method to determine acetic acid in aspirin by bubbling dry air through a thin layer of powdered aspirin, trapping the acetic acid in water and backtitrating it with alkali. Gas chr~matographyl~~ has also been used. 5.63
Acetylsalicylic Anhydride and Acetylsalicylsalicylic Acid In addition to salicylic and acetic acids, very small quantities of acetylsalicylanhydride (0.0012 to 0.024%) and acetylsalicylsalicylic acid (0.03 to 0.1%) have been found in aspirin preparations. The former has been determined by gas chromatography, TLC1 and spectro hotometry , the latter by gas chromatography. tT4 A controversy is still ongoing (cf. 152) whether the occasionally observed hypersensitivity against aspirinis caused by these two impurities and whether the basis of the adverse reaction is immunological. Stability - Deqradation That aspirin is sensitive to moisture is wellknown and most of us at one time or another have observed the growth of salicylic acid whiskers on aspirin tablets left f o r too long in a humid bath6.
ASPIRIN
31
room wall cabinet. The hydrolysis of aspirin to salicylic acid was already of concern to the pharmacologist, Dreser' (see Section 1.21, who in 1899 prepared what nowadays one would call a preformulation profile. He tested the hydrolysis of aspirin in acid and alkaline solutions and,by perusing textbooks of Ostwald and Nernst to devise the proper equations, determined hydrolysis constants of 3.3 x at "body temperature" in acid medium and 2.5 x at room temperature in alkaline medium. He also observed that aspirin was easily split in weakly alkaline medium which had consequences for the metabolism (see Section 7 ) . One could say that he established the first profile for the pH dependence of hydrolysis of aspirin. Of course, the definition of pH was unknown at the time. The next systematic study of the hydrolysis of aspirin in water, albeit at 1000 C., was undertaken by Rath172 who determined a hydrolysis constant of about 0.17 depending on experimental conditions. Much work has been done since, and it is quite evident that this seemingly simple hydrolysis to acetic and salicylic acids is both complex and controversial. I am fortunate that I can refer the reader to the excellent and detailed review by Clark A . KellylS1 already mentioned in Section 5.61. The most complete and thorough kinetic studies of the factors involved in the hydro1 sis of aspirin are undoubtedly those by Edwards 73, which were further elaborated by Garrett.174 Stability and decomposition kinetics of aspirin both as a solid and in solution continue to be studied. The topochemical decomposition pattern of aspirin tablets has been explored.175 The degradation of aspirin in the presence of sodium carbonate and hi h humidity was studied by x-ray diffraction. l q 6 The activation energy of decomposition by water vapor in the solid state was found to be 30 kcal/mo1.177 The effect of common tablet excipients on aspirin in aqueous suspension was also studied.178 An exhaustive study of the stability of aspirin in polyethylene glycols (substituted, unsubstituted and esterified), as well as other polyhydric alcohols, was undertaken by Whithworth and collaborator^!^^-^^^
32
KLAUS FLOREY
It was found that decomposition is in part due to transesterification and that substitution increases stability. The effect of gamma radiation on aspirin has been described.lE4 The pH stability profile of aspirin according to Edwards has been made the subject of a student experiment.lE5 Pharmacokinetics - Drug Metabolic Products When Dreser' investigated the pharmacological properties of aspirin in 1897 (see Section 1.21, he postulated that, based on the easy hydrolysis of aspirin in weakly alkaline medium, aspirin also should be converted to salicylic acid in vivo. And, indeed, he found that only 22 minutes Z t a n gestion of aspirin, his own urine gave a positive reaction for salicylic acid with ferric chloride. After 12 hours, he could no longer detect salicylic acid in his urine. He found no evidence for aspirin itself in urine, nor did he find a combination of aspirin with glycine analogous to the formation of hippuric acid already known at the time. He had evidence for formation of another nitrogen containing derivative. This early investigation should give food for thought to those who believe that pro-drugs and pharmacokinetics are recent discoveries.
7.
In 1911, NeuberglE6 detected small amounts of gentisic acid (2,5-dihydroxybenzoic acid) in the urine of dogs dosed with aspirin. The metabolism of aspirin is intertwined with that of salicylic acid, but I was unable to ascertain who first reported the metabolic formation of salicyluric acid, the major metabolite of both salicylic acid and aspirin, specifically after administration of aspirin. Reviews by PuetterlE7 and by Levy,188-190taken together present a comprehensive picture of the pharmacokinetics and metabolism of aspirin. Once absorbed, aspirin is rapidly converted to salicylic acid. After i.v. administration, the half life of aspirin in the human organism was found to be only 15 minuteslgl by Rowland and Riegelman who also estimated that only 2 0 % of the -in vivo hydrolysis takes place in blood.192 Apparently, all tissues investigated possess
ASPIRIN
33
esterases which can split aspirin; however, most of it seems to be hydrolyzed in the liver.187 While the major pathway of hydrolysis leads to free acetic acid, it is noteworthy that a significant portion of the acetic acid is not set free but used for transacetylation of certain factors which pla a role in the inhibition of platelet aggregation1J 3 only shown by aspirin but not by salicylic acid. The kinetics of this important pathway still need exploration.187 Aspirin serum esterase activity is species dependent.Ig4 In man it is sex linked since it was found to be higher in men than women.lg5 It also seems to be age dependent.lg6 Once aspirin is hydrolyzed to salicylic acid, it follows the metabolic pathway of the latter. The metabolic products of salicylic acid are presented in Figure 9 . Over the last decade, the pharmacokinetics of salicylates in the healthy and diseased organism have been explored in great detail by Levy.188 Salicylic acid (11) is eliminated by five parallel and competing pathways (Fig. 9 ) leading to renal excretion. These are: excretion unchanged (II), conjugation with glycine to form salicyluric acid (111) -- the major pathway -conjugation of the carboxyl or phenolic hydroxyl group to form glucuronides IV and V and hydroxylation to gentisic acid (VI) To a minor degree, salicyluric acid can be further conjugated with glucuronic and sulfuric acids.187 The major metabolic pathways (salicyluric and salicyl phenol glucuronide) are easily saturated in the usual dosage range for treatment of inflammation.lg7 For the clinical implications of these non-linear pharmacokinetic characteristics, I refer to the reviews by Levy.188'190
.
To properly treat bovine "sufferers of headaches" (inflammation) the pharmacokinetics of aspirin in cattle have also been explored.1g8 Bioavailability - Dissolution In the last two decades, the concept of bioavailability has gained prominence and-with it dissolution as a possible in vitro model for drug absorption. In 1960, S w i n t o s k y d BlytheIg9 8.
I I
0
W Ocn U
E o' u
/ I
8
8u o'
I
E
X
0
0
rcl
ASPIRIN
35
compared the relative availability of aspirin from entexic coated and compressed tablets by measuring the excretion of salicylate. About the same time, Levy200,201started to compare dissolution and absorption rates of different commercial aspirin tablets, found good correlation and proposed that the U.S.P. tablet disintegration test be replaced by a dissolution test; a suggestion which as of this writing has not been heeded. These studies were extended and further perfected by Gibaldi.163 Many other papers on this subject have appeared. Particularly,the influence of the crystal habitat (see Section 4.243) on absorption has been studied (cf. 202). Significant intraindividua1,but not i n t e r i n d i v i d u a 1 , v a r i a t i o n s in blood plasma aspirin levels were found in young male subjects after administration of aspirin as tablets or solutions. The plasma level curves obtained for tablets were more variable than those obtained for solutions.203 Levy204 found that using urinary excretion measurements for evaluation of aspirin dosage forms,with different absorption rates in man, requires that such measurements be made during the first hour after drug administration. The use of a pHstat for testing dissolution of various aspirin dosage forms has been described.205 Determination in Biological Fluids and Tissues All the advances in pharmacokinetics and drug metabolism described in Sections 7 and 8 would not have been possible without the availability of the proper analytical methods. The following is a tabulation of publications in this field, most of which have already been discussed in Section 5. It should be mentioned that a few publications talk about aspirin blood levels, but really mean salicylate levels. The following tabulation covers only those papers where aspirin was differentiated from other salicylates by chromatography or other means. It seems that the "workhorse" for serum salicylate levels is still the colorimetric (ferricnitrate) method of Brodie, Udenfriend and C ~ b u r n ' ~ ~ published in 1944, or modifications thereof. Simplified versions (cf. 206) may lead to erroneous results under certain conditions.207 The method is also applicable for urinary metabolites after proper hydrolysis (cf. 2 0 8 ) . For other methods restricted to salicylic acid, see Section 5.61. The first gas chromatographic separation of aspirin 9.
KLAUS FLOREY
36
and salicylic acid in plasma was described by Rowland and Riegelman, 4 1 who presented a brief review of earlier methods. Methods for aspirin: Colorimetric (with differential extraction):218,219 Spectrophotometric (differential): 20, 209 Fluorometric (as salicylic acid): 160, 210 Phosphorimetric: 23 VPC: 137,141,143,145,146 PC: 106,107,119 TLC: 118,211 Mass Spectrometric: 37 Radioisotopic: 212-214 Determination in Pharmaceutical Preparations The following tabulation of references highlights those methods (see Section 5 ) useful in pharmaceutical analysis. 10.
1.
Determination in tablets: Differential U.V.: 157,158 Automation: 166 22 Fluorometric : 121 Column : TLC : 120 GC : 136,139,144
2.
Determination in buffered tablets: Fluorometric: 159 161,162 Column :
3.
Determination in combination products: a. General Identity tests: 83,86,103,104,105, 112 b. Aspirin, caffeine, acetophenetidine (and more components) w: 21,215 IR: 91-93 NMR: 102 Electrophoresis: 149 110 ,111 TLC : Column: 80 Ion-exchange column: 123 HPLC : 127,130,131 135 ,142 VPC : Pot. titration: 216
ASPIRIN
11.
37
c.
Aspirin, acetaminophen, caffeine: Nonaqueous titration: 94,217 Potentiometric: 102
d.
Aspirin-barbiturate combinations: Nonaqueous titration: 93
e.
Cough-cold mixtures: HPLC: 132
Acknowledgments
I would like to express my gratitude to the Archives of Bayer AG, Leverkusen, Germany for historical information, to G. Levy, School of Pharmacy, S.U.N.Y., Buffalo for a critical review of the section on pharmacokinetics, to A . I. Cohen, M. Porubcan and B. Toeplitz for providing spectral information and interpretations, and to M. Bruno for her expert secretarial assistance.
KLAUS FLOREY
38
12.
References
H. Dreser, Pflug. Arch. Gen. Physiol., 76, 306 (1899). 2. J. Wohlgemuth, Ther. Mh., 13, 276 (1899). 3. K. Witthauer, Ther. Mh., 13,330 (1899). 4. Bayer A.G. Grchives 5. A. Eichengrun, Pharmazie, 4, 582 (1949). 6. F. Hoffmann, U.S. Patent c44077 of February 27, 1900. 7. Neue Deutsche Biographien, p. 415. 8. C. Gerhardt, Annalen der Chemie, 67, 149(1853). 9. H. von Gilm, Annalen, 112, 181 (1859). 1 5 0 3 (1869). 10. K. Kraut, Annalen, 11. D.A. Nightingale, U.S. Patent 1,604,472; C.A. 21, 157 (1927). 12. BayerT Co., DRP 386679 (1924); Beilstein 111, p . 41. 21, 23 13. Fernandez, Torres, An.Soc. espaz., (1923); Beilstein 111, p. 41. 14. Norwich Pharmacal.Co., Brit. Pat. 893,967 (1962); C.A. 57, 3572f (1962). J.P. Hummel, W.D. Paul and 15. J.W. Clappiso: J. I. Routh, J. Am. Pharm. ASSOC., 40, 532 (1951). 16. B. Toeplitz, The Squibb Institute for Medical Research, Personal Communication. 17. O.R. Sammul, W.L. Brannon and A.L. Hayden, J. Assoc. Offic. Agr. Chemists, 47, 918 (1964). - 91861p 18. S.G. Il'yasov, V.L. Dragun, C.A.82, (1975). 19. Isolation and Identification of Drugs, E.C.G. Clarke, Editor, The Pharmaceutical Press, London (1969). 6, 275 20. A. Garner, J.K. Sugden, Anal. Lett. (1973). 21. M. Jones and R.L. Thatcher, Anal. Chem., 23, 957 (1951). 22. C.I. Miles and G.H. Schenk, Anal. Chem., 42, 656 (1970). 23. J.D. Winefordner and H.W. Latz, Anal. Chem., 35, 1517 (1963). 74, 24. L. Kahovec and K.W.F. Kohlrausch, Monotsh. 333 (1943); C.A. 38, 51475 (1944). 25. G.V.L.N. Murty andT.R. Seshadri, Proc.Indian Acad. Sci., 19A, 17 (1944); C.A. 38, 6197-8 (1944). 1.
ASPIRIN
26. 27. 28. 29. 30. 31. 32. 33. 34.
35. 36. 37. 38. 39. 40. 41. 42. 43. 44. 45. 46. 47. 48. 49. 50.
39
E.G. Brame, Encycl. Ind. Chem. Anal., 2, 707 (1966). G.A. Olah, P.W. Westerman, J. Org. Chem., 2 1307 (1974). B.L. Shapiro, L.E. Mohrmann, J. Phys. Chem. Ref. Data, 6 919 (1977). K.N. Scott,-J. Magn. Resonance, 5, 55 (1972). B.D. Sykes, W.E. Hull, Ann. N.Y. Acad. Sci., 226, 60 (1973); C.A. 80, 74282s (1974). A.J. Marcus, S.E. Lasker, Haernostasis, 2, 92 (1973); C.A. 82, 8 0 3 6 0 ~(1975). A.I. Cohen, The Squibb Institute for Medical Research, Personal Communication. M. Porubcan, The Squibb Institute for Medical Research, Personal Communication. P.J. Black, A.I. Cohen, presented at the 20th Annual Conference on Mass Spectrometry and Allied Topics, Dallas, Texas, June 4-9, 1972. H.M. Fales, G.W.A. Milne, N.C. Law, Arch. Mass Spectral Data, 2, 628 (1971). N.C. Law, V. Aandahl; H.M. Fales, G.W.A. Milne, Clin. Chim. Acta, 32, 221 (1971). W. Boerner, S. Abbzt, J.C. Eidson, C.E. C.E. Becker, H.T. Horio, K. Loeffler, Clin. Chim. Acta, 49, 445 (1973). L. Kofler, Pharm. Zentralhalle, 89, 223 (1950); C.A. 45, 1301a (1951). G.D. =a1 and C.R. Szalkowski, J. Am. Pharm. ASSOC., 22, 36 (1933). T.S. Carswell, J. Am. Pharm. ASSOC., 16,306 (1927). J.L. Hayman, L.R. Wagener and E.F. Holden, J. Am. Pharm. ASSOC., 14, 388 (1925). H.W. Johnson and C.W. Ballard, Pharm. J., 157, 88 (1946). M. deBisschop, J. Pharm. Belg., 25, 330 (1970). Beilstein X, p. 67 (1927). Europeian Pharmacopeia I, 236 (1969). T. Prusik, The Squibb Institute for Medical Research, Personal Communication. W.W. Wendlandt, J. Hoiberg, Anal. Chim. Acta, 29, 539 (1963). K W . Wendlandt, L.W. Collins, Anal. Chim. Acta, 71, 411 (1974). P.J. Wheatley, J. Chem. S O C . Suppl., 1964,6039. Q. Ochs, The Squibb Institute for Medical Research, Personal Communication.
40
51. 52. 53. 54. 55. 56. 57. 58. 59. 60. 61. 62. 63. 64. 65. 66. 67. 68. 69. 70. 71. 72. 73. 74.
KLAUSFLOREY
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41
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358,
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w.
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J.V. Swintosky and R.H. Blythe, Drug Standards, 28, 5 (1960). 200. G. Levy, J.Pharm. Sci., 50, 3.88 (1961). 201. G . Levy, J.R. Leonards anhJ.A. Procknal, J. Pharm. Sci., 54, 1719 (1965). 202. A.G. Mitchell, B.L. Milaire, D.J. Saville, R.V. Griffiths, J. Pharm. Pharmacol., 23,. 534 (1971). 203. K. Frislid, E.M. Haram, R. Norberg, S. Oie, Pharm. Acta Helv., 48, 610 (1973). 204. G. Levy and A. Yacobi, J. Clin. Pharmacol., 15, 525 (1975). 205. S. Goto, J. Nakashima, M. Tsuruta, H. Sato, T. Nakayama, Yakuzaigaku, 34, 160 (1974); C.A. 83, 152268~(1975). 206. W.C. gller, Am. J. Clin. Path., 17, 22 (1947). 207. L.J. Fenton, M.E. Beresford, W.J. Keenan, Pediatrics, 59, 55 (1977). 208. G. Levy and T A . Procknal, J. Pharm. Sci., 57, 1330 (1968). 209. J.I. Routh, N.A. Shane, E. Arrendondo, W.D. Paul, Clin. Chem., 13, 734 (1967). 210. S.L. Kanter, W.R. Horbalz J. Pharm. Sci., 60, 1898 (1971). 211. Z.I. El-Darawy, Z;M. Mobarak, Forensic Sci., -4 , 171 (1974). 212. E.M. Burnham, W.D. Paul and J.I. Routh, Proc. Iowa Acad. Sci., 63, 403 (1956); C.A. 50, 21671.1 (1956). 213. W.R. Borst, J.E. Christian and T.S. Miya, J. Pharm. Sci., 45, 511 (1956). 214. H.G. Mandel, N.M.Cambosos, P.K. Smith, J. Pharmacol. Exptl. Therap., 112, 495 (1954). 215. A.W. Clayton and R.E. Thiers, J. Pharm. Sci., 55, 404 (1966). 216. S.L. Lin and M.I. Blake, Anal. Chem., 38, 549 (1966). 217. S.P. Agarwal, M.I. Blake, Can. J. Pharm. Sci., 7, 123 (1972). 218. E.J.H. Smith, J. Pharm. Pharmacol., 3, 409 (1951). 219. I.A. Muni, J.L. Leeling, R.J. Helms, N. Johnson, Jr., J.J. Bare and B.M. Phillips, J. Pharm. Sci., 67, 289 (1978). The literature has been covered systematically through Chemical Abstracts,Volume 88 (1978), with a few stray references beyond.
-
-
Analytical Profiles of Drug Substances, 8
BROMOCRIPTINE METHANESULPHONATE Danielle A . Giron-Forest and W . Dieter Schonleber
3. 4.
5.
6. 7.
8.
Introduction 1 . 1 History I .2 Name, Formula, Molecular Weight 1.3 Appearance, Color, Odor Ph ysicochemical Properties 2. I Elemental Analysis 2.2 Spectra 2.21 Infrared 2.22 Ultraviolet 2.23 Fluorescence 2.24 Proton Nuclear Magnetic Resonance 2.25 Carbon-13 Nuclear Magnetic Resonance 2.26 Mass 2.3 Crystal Properties 2.3 I Melting Characteristics 2.32 Polymorphism 2.33 X-Ray Diffraction 2.34 Differential Scanning Calorimetry 2.35 Thermogravimetry 2.4 Solubility 2.5 Dissociation Constant 2.6 Partition Coefficients 2.7 Optical Rotation Synthesis Stability and Degradation Processes 4.1 InBulk 4 . 2 In Solution 4.3 In the Dosage Form Biopharmaceutics 5. I Pharmacokinetics 5.2 Metabolism Toxicology Analytical Methods 7. I Application of General Tests 7.2 Titration 7.3 Spectroscopic Methods 7.31 Infrared 7.32 Ultraviolet 7.33 Colorimetry 7.34 Nuclear Magnetic Resonance 7 . 4 Chromatography 7.41 Paper 7.42 Thin-Layer 7.43 Gas-Liquid 7.44 High Performance Liquid 7.5 Differential Scanning Calorimetry 7.6 Phase Solubility 7.7 Analysis of the Dosage Form 7.8 Determination in Body Fluids and Tissues References All 41
Copyright @ 1979 by Academic Press, Inc. rights of reproduction in any form reserved. ISBN 0 12-260808-9
DANIELLE A. GIRON-FOREST AND W. DIETER SCHONLEBER
48
1.
Introduction 1.1 History
The most valuable pharmacological p r o p e r t i e s of the pept i d e type e r g o t a l c a l o i d s induced a v a r i e t y of attempts of chemical d e r i v a t i s a t i o n of t h e p a r e n t compounds ( 1 , 2 + lit. quoted t h e r e i n ) . I n one of these the bromination of a-ergoc r y p t i n e l e d t o a product of h i g h l y i n t e r e s t i n g pharmacology, namely bromocriptine. I t became known t o suppress p r o l a c t i n e s e c r e t i o n , and i t i s t h e r e f o r e a u s e f u l t o o l i n t h e treatment of p r o l a c t i n e dependent d i s o r d e r s , such a s g a l a c t o r r h e a a s s o c i a t e d with hyperprolactinemia and postpartum, a s w e l l as c e r t a i n kinds of s t e r i l i t y ( 3 - 9 ) . I n more e l e v a t e d doses, t h e drug i s a p o t e n t antiparkinsonicum. I n a d d i t i o n , t h e r e i s r e c e n t evidence of bromocriptine playing an important r o l e i n the trace heavy metals balance of t h e b r a i n ( 1 0 ) .
1.2
Name, Formula, Molecular Weight
Bromocriptine mesilate i s 2-bromo-a-ergocryptine methanesulphonate o r 2-bromo-12'-hydroxy-2'-(l-methylethyl)-5'-(2methylpropyl-5'a-ergotaman-3',6',18-trione methanesulphonate o r Bromocriptinum ( I N N ) . I t i s the a c t i v e i n g r e d i e n t i n ParlodelB dosage forms.
CH3
/..
x CH3S03H
BROMOCRIPTINE METHANESULPHONATE
49
Chemical A b s t r a c t s R e g i s t r y Numbers : 25614-03-3 (26409-15-4) ( 4783 0- 26- 2 )
Average Molecular Weights : base :
654.61
mesilate:
750.71
Average Formulas : base :
C
mesilate: C
H
32 4 0
BrN 0 5 5
H BrN 0 S 33 44 5 8
1 . 3 . Appearance, Colour, Odour Grey tinged white o r l i g h t yellow, f i n e l y c r y s t a l l i n e powder, odourless o r of weak, c h a r a c t e r i s t i c odour. 2.
Physicochemical P r o p e r t i e s 2.1
Elemental Analysis
The elemental a n a l y s i s of bromocriptine mesilate y i e l d e d t h e following r e s u l t s (11): element
calculated
%
52.8 5.9 10.6 9.3 17.0 4.3
C
H Br N 0 S
2.2
%
found 53.2 6.0 10.5 9.2 16.8 4.4
Spectra
2.21 I n f r a r e d
The i n f r a r e d spectrum of bromocriptine m e s i l a t e i n a KBr p e l l e t i s given i n f i g . 1. I t was recorded on a Perkin
Elmer 257 i n f r a r e d spectrophotometer. The main c h a r a c t e r i s t i c bands are t h e following
:
%Absorption
a,
m
cr ffl
rl .d
P
BROMOCRIPTINE METHANESULPHONATE wave number ( c m 3200 1728
-
2900
1642, 1672 1560
-1
)
51
assignment C-H-stretching v i b r a t i o n s C=O-stretching o f 5-membered r i n g lactam ( c y c l o l ) C=O-stretching o f 6-membered r i n g l a c t a m (amide I ) amide-11 band and C=C- st r e t c h i n g
The s p e c t r u m of t h e b a s e h a s been r e p o r t e d by P.A. S t a d l e r and co-workers (11). 2.22 U l t r a v i o l e t The u l t r a v i o l e t spectrum o f b r o m o c r i p t i n e mesilate was r e c o r d e d on a P h i l i p s 1700 uv s p e c t r o p h o t o m e t e r i n 0 . 1 M met h a n o l i c methanesulphonic a c i d s o l u t i o n . I t i s g i v e n i n f i g . 2. A maximum o c c u r s a t a b o u t 308 nm w i t h a l o g molar absorpt i v i t y o f 4.0. I n 1:l dichloromethane/methanol s o l u t i o n t h e a b s o r p t i o n maximum was r e p o r t e d as 306 nm l o g = 3.988 (11). 2.23 F l u o r e s c e n c e Bromocriptine m e s i l a t e e x h i b i t s fluorescence l i k e the o t h e r l y s e r g i c and i s o l y s e r g i c a c i d type a l c a l o i d s . I n 2 p e r c e n t e t h a n o l i c t a r t a r i c a c i d s o l u t i o n , t h e e m i s s i o n maximum a p p e a r s a t 402 m ( e x c i t a t i o n a t 325 nm) See f i g . 3 .
.
2 . 2 4 P r o t o n Nuclear Magnetic Resonance The PMR spectrum of b r o m o c r i p t i n e mesilate i n d e u t e r a t e d d i m e t h y l s u l p h o x i d e a s o b t a i n e d on a Bruker HX-90 NMR s p e c t r o meter i s p r e s e n t e d i n f i g . 4. TMS s e r v e d a s i n t e r n a l s t a n d a r d . The c h a r a c t e r i s t i c s of t h e spectrum a r e g i v e n i n the f o l l o w i n g t a b l e (see a l s o 1 2 , 1 3 and lit. q u o t e d t h e r e i n ) :
Chemical S h i f t downf i e l d (ppm)
PMR-spectrum and Assignment Intensity Multiplicity Assignment
11.85
1 H
Singlet
indole-Ng
10.45
1 H
Singlet
NH -
9.55
1 H
Singlet
CONH-
7.3
4H
I
7
-
and
(18-19)
OH
DANIELLE A. GIRON-FOREST AND
52
230
Figure 2.
270
310
350
w. DIETER SCHONLEBER
390
nm
Ultraviolet Spectrum of Bromocriptine Mesilate in 0.1 M Methanolic Methanesulphonic Acid. CA = 0.05 mg/ml, C = 0.012 m g / m l . B Instrument: Philips SP 1700
53
BRLOMI3CRIPTINE METHANESULPHONATE
nm
Figure 3.
Fluorescence Spectrum of Bromocriptine Mesilate in 2 % Ethanolic Tartaric Acid. C = 65,ug/ml. Instrument: Perkin Elmer MPF-3
Figure 4.
PMR Spectrum of Bromocriptine Mesilate in (CD ) SO, 3 2 Instrument: Bruker HX-90 E
55
BROMOCRIPTINE METHANESULPHONATE
1H
6.47 4.3
-
4.5 3.2
3
2.37
2.1
16 H
- 4.2
-
2*1 1.5
1
Singlet
{
3 H 8-9 H
{
Triplet singlet Multiplet
H-C
-
9
H-C
- 5' 6-CH ((2-17) -3 g-C C-!; ;H-C4; 8' 11' H-C5 ; F-C * H-C 7 ' 8 CH C0CK2CH3 ; H20 3 (recryst. solvent)
Singlet
CH -SO H
Singlet
CH COCH CH
Multiplet
-3
3
-3 2 3 5'-C€12 ; 5'-Cg ; 2 ' - C g
H-Cg,
0.75-1.15
12 H
Multiplet
2'CH
-3
;
; g-C 1 0 '
-
5'-CH -3
and
CH3COCH CH
2 -3
2.25 Carbon-13 Magnetic Resonance Spectrum The spectrum o f b r o m o c r i p t i n e m e s i l a t e h a s been r e c o r d e d i n d i m e t h y l s u l p h o x i d e u s i n g a Bruker HX-90 NMR s p e c t r o p h o t o meter ( f i g . 5 ) . The a s s i g n m e n t o f t h e i n d i v i d u a l s i g n a l s i s g i v e n i n f i g . 6. 2.26
Mass Spectrum
The low r e s o l u t i o n e l e c t r o n impact mass s p e c t r a l p a t t e r n of bromocriptine m e s i l a t e ( f i g . 7 ) corresponds q u i t e n i c e l y t o t h o s e o f t h e o t h e r non- and d i h y d r o g e n a t e d e r g o t a l c a l o i d s ( 1 2 , 1 3 and lit. quoted h e r e i n ) . The m o l e c u l a r peak M of t h e b a s e shows up a t 653 and 655, r e s p e c t i v e l y , r e f l e c t i n g t h e n a t u r a l abundance o f t h e bromine i s o t o p e s , and M - 1 8 a t 635/637 mass u n i t s . A s i n t h e p a r e n t compounds t h e n e x t s m a l l e r f r a g m e n t a p p e a r s a t M-228, i n d i c a t i c g a s u b s t a n t i a l loss of t h e p e p t i d e s e c t i o n c o n s t i t u e n t s w i t h t h e t e n t a t i v e fragment s t r u c t u r e F1. From t h i s s p e c i e s t h e i s o p r o p y l group s p l i t s o f f e a s i l y t o y i e l d t h e l i n e p a i r a t 382/384 m a s s u n i t s . L o s s o f t h e e n t i r e p e p t i d e moiety l e a d s t o t h e f o r m a t i o n o f 2-bromo-lysergamide F2 a t 345/347 m.u., t h e mass s p e c t r a l b e h a v i o u r of which c o r r e s p o n d s t o t h a t o f t h e bromine-free compound. Thus, i t g i v e s r i s e t o peak p a i r s a t 300/302 and 299/301, r e s p e c t i v e l y , presumably by l o s s of formamide o r by t h e r u p t u r e of t h e t e t r a - h y d r o - p y r i d i n e r i n g ,
6000
4003
2000
3000
2000
>m
'%a
rm
xa
I tm
I
-
4ca
I
t T
Figure 5 .
y1
T
lb
T
lbo
L
T
13-C-NMR Spectrum of Bromocriptine Mesilate in (CD ) SO, 3 2 Instrument: Bruker HX-90 E
I 0
57
100 90 80
I
1
I
I
'O
70
I__
60 50 YO
30
20 10
36
I
582
635 653
'25
f
1 " " " " ' 1 " " " ' " l ' " ' ' " " " " " ' ' ~
100
Figure 7 .
200
300
900
500
Low Resolution Electron Impact Mass Spectrum of Bromocriptine Mesilate Instrument: CEC 21-llOB; Energy 70 eV, Ion Source 0 Temperature 160 - 200 C
600
M/Z
700
BROMOCRIPTINE METHANESULPHONATE
59
a decay mode t h a t w a s proposed e a r l i e r (14,15) for l y s e r g i c a c i d d e r i v a t i v e s . Peak d o u b l e t s a t 285/287 and 274/276 m.u. i n d i c a t e fragments of i l l i c i t s t r u c t u r e s t i l l c o n t a i n i n g bromine.
425/427 m.u. The p e p t i d e moiety i t s e l f (308 rn.u.1 obviously does n o t appear i n t h e spectrum, whereas i t s fragmentation p a t t e r n with peaks a t m/e 195 (F3), 167 (F3-CO), 155 - 153 (F4), 125 (FS), 86 (F6), and base peak 70 (F7) mass u n i t s , i s c l e a r l y understood (14,15) The m e s i l a t e shows a s i g n a l a t m/e 96.
-
1
I 195 m.u.
F3
F4 1 5 4 m.u
DANIELLE A. GIRON-FOREST AND W. DIETER SCHONLEBER
60
D ' q0
H
F5
125 m.u.
2.3
F7 86 m.u.
70 m.u.
Crystal Properties
2.31 M e l t i n g C h a r a c t e r i s t i c s Bromocriptine m e s i l a t e decomposes between 180 and 200 O C , t h u s a m e l t i n g p o i n t o r m e l t i n g r a n g e c a n n o t be g i v e n . 2.32 Polymorphism I n v e s t i g a t i o n s f o r t h e o c c u r r e n c e o f polymorphism have been u n d e r t a k e n by i r s p e c t r o s c o p y , d i f f e r e n t i a l s c a n n i n g c a l o r i m e t r y and x-ray powder d i f f r a c t i o n ( G u i n i e r - d e W o l f f ) . N o polymorphism h a s been observed so f a r . An amorphous form may be p r e p a r e d a r t i f i c i a l l y by r a p i d e v a p o r a t i o n o f a methanolic s o l u t i o n of t h e drug substance. 2.33 X-Ray D i f f r a c t i o n X-ray s t r u c t u r a l a n a l y s i s o f b r o m o c r i p t i n e , c r y s t a l l i z e d a s t h e b a s e from dichloromethane/diethylether, h a s been carr i e d o u t on a CAD 4 - d i f f r a c t o m e t e r w i t h CuKa-radiation ( 1 6 ) . 3371 r e f l e x i o n s were w i t h i n s i n @/A<0.62 8-l. Assessment o f t h e s t r u c t u r e was a c h i e v e d by computation t o a r e f i n e m e n t o f R = 0.033 f o r t h e a b s o l u t e c o n f i g u r a t i o n . The c r y s t a l d a t a w e r e : Space g r o u p P 2 a = 10.681, 1' b = 13.454, c = 11.049, @ = 9 9 - 7 5 " , Z = 2. I n f i g . 8 t h e r e s u l t a n t conformation of bromocriptine base i s depicted. 2.34 D i f f e r e n t i a l Scanning C a l o r i m e t r y The DSC thermogram o f b r o m o c r i p t i n e m e s i l a t e , o b t a i n e d w i t h a P e r k i n E l m e r DSC-2 i n s t r u m e n t a t a h e a t i n g r a t e o f 20 'C/min. and i n a n i t r o g e n atmosphere, i s shown i n f i g . 9.
2a
Figure 8.
Conformation of Broaocriptine Base established on the Basis of the X-ray Structural Analysis.
0
=
Nitrogen,
=
Hydrogen
0
= oxygen,
0
= Carbon,
DANIELLE A. GIRON-FOREST AND W. DIETER SCHONLEBER
62
TG
\ T
40
60
Figure 9.
80
100
120
140
160
180
200
Differential Scanning Calorimetry and. Thermogravimetry Curves of Bromocriptine Mesilate, each at a heating rate of 200C/min. and a Nitrogen Flow of 15 ml/min. Instruments: Perkin Elmer DSC-2 Perkin Elmer TGS-1
OC
BROMOCRIF'TINE METHANESULPHONATE
63
The m e l t i n g endotherm i s f o l l o w e d immediately by a s t r o n g exothermic d e g r a d a t i o n . S i n c e b r o m o c r i p t i n e mesilate decomposes under m e l t i n g , the t r a n s i t i o n t e m p e r a t u r e i s s t r o n g l y dependent on the h e a t i n g r a t e . A b r o a d b u t weak endotherm between 40 and 100 "C i n d i c a t e s t h e v o l a t i l i z a t i o n o f s o r b e d r e c r y s t a l l i z a t i o n s o l v e n t ( u s u a l l y butanone-2, see s e c t i o n 3 ) . 2.35 Thermogravimetry The thermogram o f b r o m o c r i p t i n e m e s i l a t e , c a r r i e d o u t on a P e r k i n E l m e r TGS-1 thermobalance, i s g i v e n i n f i g . 9. The sample t e m p e r a t u r e w a s r a i s e d a t a r a t e o f 20"C/minute m a i n t a i n i n g a n i t r o g e n atmosphere. A c o n s i d e r a b l e loss o f weight, a t t r i b u t e d t o a loss of sorbed s o l v e n t ( s . above), i s observed below 130 'C. Sample decomposition o b v i o u s l y s t a r t s a f t e r melting. 2.4.
Solubility
The s o l u b i l i t y of b r o m o c r i p t i n e mesilate w a s d e t e r m i n e d i n a v a r i e t y of s o l v e n t s e q u i l i b r a t e d by v i b r a t i o n d u r i n g 2 4 h o u r s a t 25 OC. They are a s f o l l o w s : Solvent
S o l u b i l i t y i n mg/g
water m e t h a no 1 ethanol 2-propanol a c e t o n i tr i l e acetone ethyl acetate chloroform benzene hexane
0.8
910 23.0 1.2 1.6 0.2 0.2 0.45
<0.1 <<0.1
S o l u b i l i t y i n g/100 m l 0.08 72 1.8 0.1 0.12 0.015 0.015 0.06 <0.02
<<0.01
A t 22 ?r 2 OC b r o m o c r i p t i n e m e s i l a t e d i s s o l v e s r e a d i l y ( > 2 % ) i n p r o p y l e n e g l y c o l , 50 % e t h a n o l , 95 % e t h a n o l and n - o c t a n o l , whereas i t i s p o o r l y s o l u b l e (<0.1 % ) i n s i m u l a t e d g a s t r i c and i n t e s t i n a l f l u i d s a t 37 ? 2 "C.
2.5
Dissociation Constant
Due t o t h e low s o l u b i l i t y o f b r o m o c r i p t i n e m e s i l a t e i n w a t e r , t h e pK v a l u e had t o be determined i n methyl c e l l o a s o l v e / w a t e r 8: 2 (w/w) T i t r a t i o n a t ambient t e m p e r a t u r e y i e l d 0.05 f o r a 0.0078 M s o l u t i o n . e d p K a a s 4.90
*
.
DANIELLE A . GIRON-FOREST AND
64
2.6
w. DIETER SCHONLEBER
P a r ti t i o n C o e f f i c i e n t s
The p a r t i t i o n c o e f f i c i e n t s of b r o m o c r i p t i n e mesilate between water of pH 1 . 2 and n - o c t a n o l o n t h e o n e hand, and water of pH 7.5 and n - o c t a n o l o n t h e o t h e r , h a v e b e e n determined a t 37.0 ? 0 . 5 "C.
water p H 1 . 2 / n - o c t a n o l water pH 7.5/n-octanol
1 : 90 1 : 235
Optical R o t a t i o n
2.7
T h e o r e t i c a l l y , w i t h 6 c h i r a l c e n t e r s w i t h i n the m o l e c u l e ( a t 6 , 9 , 2 ' , 5 ' , 11' and 1 2 ' p o s i t i o n s ) 64 d i a s t e r e o m e r i c forms are p o s s i b l e . However, b r o m o c r i p t i n e i s s t e r i c a l l y w e l l d e f i n e d a t a l l o f t h e s e p o s i t i o n s , a s it i s d e r i v e d from the n a t u r a l l y occurring a-ergocryptine. The s p e c i f i c o p t i c a l r o t a t i o n of b r o m o c r i p t i n e mesilate i n d i f f e r e n t s o l v e n t s i s g i v e n below f o r 20° C corrected f o r l o s s on d r y i n g . A P e r k i n E l m e r p o l a r i m e t e r 241 w a s u s e d , the a c t u a l c o n c e n t r a t i o n b e i n g 1 0 mg/ml. wavelength (nm) solvent
589
578
546
436
365
s p e c i f i c o p t i c a l r o t a t i o n i n degrees dichloromethane/ methanol 1:l ethanol d i m e t h y l formamide
101.0 100.6 127.4
107.5 107.0 135.2
130.1 129.6 162.0
327.8 328.7 388 .O
F o r t h e s p e c i f i c r o t a t i o n of 2-bromo-a-ergocryptine bases see (11). 3.
329.4 331.3 392.7 and - i n i n e
Synthesis
B r o m o c r i p t i n e b a s e i s manufactured by b r o m i n a t i o n of a - e r g o c r y p t i n e w i t h N-bromosuccinimide i n d i o x a n e s o l u t i o n . The mesilate i s t h e n formed by a d d i t i o n of methanesulphonic a c i d . The s a l t i s r e c r y s t a l l i z e d from butanone-2 ( s . f i g . 1 0 ) (2,3111)
-
BROMOCRIPTINE METHANESULPHONATE
a-Ergocryptine Base
N-Bromo-succinimide
Bromocriptine Base
Methanesulphonic Acid
*
Bromocriptine Methanesulphonate
Figure 10.
Route of Synthesis
65
DANIELLE A. GIRON-FOREST AND W. DIETER SCHONLEBER
66
4.
S t a b i l i t y and Degradation Processes
P o s s i b l e degradation pathways of e r g o t a l c a l o i d s a t t h e example of ergotamine t a r t r a t e have been c l e a r l y summarized by H. Bethke e t a l . ( 1 7 ) and B. Kreilgaard (13). A s a nonhydrogenated e r g o t a l c a l o i d , bromocriptine i s r e l a t i v e l y s e n s i t i v e t o autoxidation both i n s o l i d and i n d i s solved states, b u t degradation products have not y e t been e l u c i d a t e d . S i m i l a r i t y t o t h e o x i d a t i v e transformation of t h e p a r e n t compounds i s t o be s t r o n g l y a n t i c i p a t e d ( 1 2 ) .
I n hydroxyl-containing s o l v e n t s , nonhydrogenated e r g o t p e p t i d e a l c a l o i d s a r e r e a d i l y epimerized a t C-8 t o an e q u i l i b r a t e d mixture of the l y s e r g i c and i s o - l y s e r g i c a c i d series , c a l l e d t h e -ine/-inine forms (-ine = 88, - i n i n e = 8 a ) ( 1 2 , 1 8 and lit. quoted t h e r e i n ) . The h y d r o l y s i s of t h e l y s e r g i c a c i d amide bond i s of minor importance f o r t h e beginning degradat i o n , b u t , of course, p r e v a l e n t under more d r a s t i c h y d r o l y s i s conditions. Under t h e same conditions, b u t a t e l e v a t e d temperatures, t h e C-2I-center i s very l i k e l y t o be i n v e r t e d ( a c i - i n v e r s i o n ) y i e l d i n g a more a c i d i c isomeric compound.
-
The light-induced a d d i t i o n of water t o t h e 9,lO-double bond of bromocriptine y i e l d i n g t h e so-called lumi-products, i s of high p r o b a b i l i t y ( 1 2 , 1 8 ) . They have, however, n o t y e t been i s o l a t e d o r c h a r a c t e r i z e d . The corresponding l0a-methoxylumi-derivative could be prepared by t h e photo-catalyzed a d d i t i o n of methanol (19) under s l i g h t l y a c i d i c conditions. 4.1
i n Bulk
Although bromocriptine m e s i l a t e i s s e n s i t i v e t o h e a t and l i g h t , i t i s s t a b l e f o r up t o 3 y e a r s a t ambient temperat u r e ( 2 0 ) when s t o r e d i n s e a l e d polyethylene bags contained i n twist-off amber g l a s s b o t t l e s . I n warm and t r o p i c a l climat e (30 "C/75 p e r c e n t r e l a t i v e humidity) and under i d e n t i c a l package c o n d i t i o n s , it i s s t a b l e f o r 1 y e a r , however o n l y f o r 3 months a t 50 "C. I f not properly p r o t e c t e d , bromocriptine adsorbs up t o 6 p e r c e n t by weight of water i n t r o p i c a l climate.
BROMOCRIPTINE METHANESULPHONATE
4.2
67
i n Solution
Bromocriptine follows t h e behaviour sketched above and i s t h u s r a t h e r l a b i l e i n aqueous o r aqueous/alcoholic s o l u t i o n s , p a r t i c u l a r l y i n t h e presence of a c i d , y i e l d i n g mainly t h e e q u i l i b r a t e d mixture with i t s 8-epimer (1) and t o a smaller e x t e n t , i t s h y d r o l y s i s products 2-bromo-lysergamide and 2-bromo-lysergic a c i d and t h e i r 8a-isomers, r e s p e c t i v e l y . 4.3
i n t h e Dosage Form
Bromocriptine m e s i l a t e i s marketed a s ParlodelB c a p s u l e s ( 1 0 mg f o r t h e treatment of Parkinson's d i s e a s e ) and t a b l e t s ( 2 . 5 mg a s l a c t a t i o n s u p p r e s s o r ) . Both forms have proved s t a b l e a t l e a s t f o r 4 y e a r s when s t o r e d a t ambient temperature i n amber g l a s s b o t t l e s ( 2 2 ) . 5.
Biopharmaceutical Aspects (23) 5.1.
Pharmacokinetics
The d i s p o s i t i o n of bromocriptine has been s t u d i e d i n s e v e r a l animal s p e c i e s and man following s i n g l e o r a l and intravenous a d m i n i s t r a t i o n of t h e drug l a b e l l e d with e i t h e r t r i t i u m o r carbon-14. The e n t e r a l absorption of bromocriptine from an aqueous s o l u t i o n amounts t o 30 - 40 8 as determined from t h e sum of t h e cumulative b i l i a r y and u r i n a r y e x c r e t i o n of r a d i o a c t i v i t y ( p a r e n t drug + m e t a b o l i t e s ) i n b i l e d u c t cannulated animals. The blood l e v e l s following o r a l and intravenous doses a r e very low i n a l l animal s p e c i e s . This, most l i k e l y , i s due t o t h e marked a f f i n i t y of t h e drug f o r v a r i o u s t i s s u e s and t h e r a p i d h e p a t i c e x t r a c t i o n of t h e absorbed f r a c t i o n . The main r o u t e of e x c r e t i o n i s t h e b i l e . L e s s than 5 % of t h e dose a r e recovered i n t h e u r i n e of i n t a c t animals a f t e r o r a l o r i n t r a venous a d m i n i s t r a t i o n . I n man, t h e e x t e n t of e n t e r a l absorption i s estimated t o be a t l e a s t of t h e same order of magnitude than determined f o r animals. Absorption i s r a p i d with an approximate r a t e c o n s t a n t of 1 . 4 h-' ( t '/2 = 30 min)
.
DANIELLE A. GIRON-FOREST AND W. DIETER SCHONLEBER
68
Peak plasma l e v e l s are reached about 1 . 5 h a f t e r o r a l i n g e s t i o n , t h e maximum c o n c e n t r a t i o n s being i n t h e o r d e r of 2 - 3 ng equivalents/ml ( p a r e n t drug + m e t a b o l i t e s ) f o r an o r a l 1 mg dose. The e l i m i n a t i o n from t h e plasma i s b i p h a s i c and proceeds with mean h a l f - l i v e s of 6 h (a-phase) and 50 h (6-phase). S i m i l a r e l i m i n a t i o n h a l f - l i v e s are obtained from t h e u r i n a r y e x c r e t i o n . The cumulative r e n a l e x c r e t i o n i s p r a c t i c a l l y t h e same a f t e r o r a l and intravenous a d m i n i s t r a t i o n 7 % of t h e r a d i o a c t i v i t y dosed. The main and amounts t o 6 p o r t i o n of t h e dose, e i t h e r o r a l or intravenous, i s e l i m i n a t e d by t h e b i l i a r y r o u t e i n t o t h e faeces. The k i n e t i c s of bromoc r i p t i n e has been demonstrated t o be l i n e a r i n t h e o r a l dose range from 2.5 t o 7 . 5 mg.
-
P a r e n t drug i s bound t o bovine and human plasma p r o t e i n s t o an e x t e n t of 89 - 96 % ( i n v i t r o c o n c e n t r a t i o n range 0.2 80 pg/ml) and e x e r t s a pronounced a f f i n i t y to v a r i o u s t i s s u e s . 5.2
Metabolism
Bromocriptine i s r a p i d l y and completely metabolised i n animals and man. The major components of t h e u r i n a r y metabol i t e s have been i d e n t i f i e d as 2-bromo-lysergic a c i d and 2-bromo-isolysergic a c i d . Apart from t h e h y d r o l y t i c cleavage of t h e amine bond and t h e isomerization a t p o s i t i o n 8 of t h e l y s e r g i c a c i d moiety, a t h i r d p r i n c i p a l biotransformation pathway cons i s t s i n t h e o x i d a t i v e a t t a c k of t h e molecule a t t h e p r o l i n e fragment of t h e peptide p a r t , predominantly a t p o s i t i o n 8 ' , giving r i s e t o t h e formation of a number of hydroxylated and f u r t h e r oxidized d e r i v a t i v e s of bromocriptine, and i n a d d i t i o n of conjugated d e r i v a t i v e s t h e r e o f . 6.
Toxicology
The a c u t e t o x i c i t y of bromocriptine mesilate h a s been determined i n t h e mouse a s 230 and 2620 mg/kg i . v . and P.o., r e s p e c t i v e l y . I n t h e r a b b i t , t h e corresponding values w e r e 1 2 and >lo00 mg/kg ( 2 ) . Thus, bromocriptine proved less t o x i c than t h e nonhydrogenated e r g o t a l c a l o i d s by one o r d e r of magnitude, resembling t h e behaviour of t h e dihydrogenated derivatives. Chronic t o x i c i t y s t u d i e s were c a r r i e d o u t with r a t s , dogs, and rhesus monkeys ( 2 ) . I n n e a r l y a l l c a s e s , the p r i n c i p a l e f f e c t produced w a s ischemia of some p a r t of t h e body. The well-known e m e t i c e f f e c t of e r g o t a l c a l o i d s i n dogs w a s p a r t i c u l a r l y pronounced with bromocriptine, even with o r a l doses of a s low a s 0 . 1 mg/kg.
BROMOCRIPTINE METHANESULPHONATE
7.
69
A n a l y t i c a l Methods 7.1
Application of General T e s t s
Compared with t h e u n s u b s t i t u t e d e r g o t a l c a l o i d s (1,181 t h e i n t r o d u c t i o n of bromine i n t o t h e 2-position of t h e indole nucleus diminishes t h e r e a c t i v i t y of t h e molecule i n r e s p e c t t o general a l c a l o i d t e s t s . Nevertheless, they s t i l l remain applicable. 1. KeLlgrLs-tgsL. Bromocriptine m e s i l a t e i s d i s s o l v e d i n g l a c i a l a c e t i c a c i d t o which have been added t r a c e s of f e r r i c c h l o r i d e . A f t e r c a r e f u l l y l a y e r i n g with concentrated s u l f u r i c a c i d , a green colour i s produced a t t h e i n t e r f a c e . U s u a l l y an i n t e n s e b l u e - v i o l e t colour occurs with 2-H-substituted compounds. 2 . I a n grk's gegcLion, ( 2 4 ) Bromocriptine m e s i l a t e i s dissolved i n methanol. After a d d i t i o n of van U r k ' s r e a g e n t and vigorous shaking a blue colour develops slowly, which i s s u b s t a n t i a l l y weaker than with 2-H-ergot a l c a l o i d s .
3. Meyeg's t e z t L Bromocriptine m e s i l a t e i s d i s s o l v e d i n methanol/water 3:lO. After a d d i t i o n of one drop of d i l u t e d hydrochloric a c i d and one drop of Meyer's reagent (mercuric potassium iodide) and s h a k b g , a white p r e c i p i t a t e i s produced. 7.2
Titration
Bromocriptine m e s i l a t e may be assayed i n g l a c i a l a c e t i c a c i d / a c e t i c anhydride 1 : 7 by t i t r a t i o n with 0 . 1 N p e r c h l o r i c a c i d . The endpoint may be determined p o t e n t i o m e t r i c a l l y using a glass/calomel e l e c t r o d e system. The methanesulphonic a c i d c o n t e n t of bromocriptine m e s i l a t e i s u s u a l l y determined by t i t r a t i o n with 0 . 1 N methanolic potassium hydroxide. The endpoint may be d e t e c t e d p o t e n t i o m e t r i c a l l y using a glass/calomel e l e c t r o d e system. Residual N-bromosuccinimide from t h e manufacturing process may be i d e n t i f i e d and/or q u a n t i f i e d by making use of i t s o x i d a t i o n p o t e n t i a l by t i t r a t i o n of l i b e r a t e d i o d i n e a f t e r a d d i t i o n of potassium iodide i n a c e t i c a c i d ( 2 5 ) .
70
DANIELLE A. GIRON-FOREST AND W. DIETER SCHONLEBER
7.3
Spectroscopic Methods
7.31 Infrared I n f r a r e d spectroscopy i s u t i l i z e d f o r i d e n t i f i c a t i o n purposes during t h e a n a l y s i s of t h e drug substance. (see 2 . 2 1 ) 7.32 U l t r a v i o l e t Spectrophotometric a n a l y s i s of bromocriptine m e s i l a t e i s c a r r i e d o u t d i r e c t l y using t h e uv maximum a t about 305 run i n methanolic methanesulphonic a c i d . However, t h e method i s n o t very s p e c i f i c . I t was p r e f e r r e d t o f i r s t s e p a r a t e t h e i m p u r i t i e s from bromocriptine by t h i n l a y e r chromatography and then t o i s o l a t e t h e substance by e l u t i o n from t h e s i l i c a g e l of t h e p l a t e with methanol. The i n t a c t a c t i v e i n g r e d i e n t i s measured i n 0.01 M methanolic methanesulphonic a c i d ( 2 6 ) .
7 . 3 3 Colorimetry I n moderately a c i d i c s o l u t i o n s bromocriptine m e s i l a t e r e a d i l y forms i o n p a i r s with a n i o n i c dyes such a s p i c r i c a c i d , bromothymol blue, methyl orange, which a r e e x t r a c t a b l e with an organic s o l v e n t . A procedure has been developed both f o r d i r e c t assay and f o r assay following chromatographic separat i o n from t h e i m p u r i t i e s . Therein bromocriptine m e s i l a t e i s allowed t o r e a c t with bromothymol blue a t pH 2.5. The r e s u l t i n g i o n p a i r i s then e x t r a c t e d with benzene and i t s concent r a t i o n determined a t 410 nm ( 2 5 ) . 7.34 Proton Magnetic Resonance PMR spectroscopy may be used f o r i d e n t i f i c a t i o n of t h e drug substance. ( s e e 2 . 2 4 )
7.4
Chromatography
7 . 4 1 Paper Paper chromatography was applied formerly t o t h e d e t e r mination of bromocriptine. conditions: system 1: s t a t i o n a r y phase: 25 % formamide mobile phase : carbon t e t r a c h l o r i d e / d i e t h y l e t h e r 1:l
BROMOCRIPTINE METHANESULPHONATE
71
system 2 : s t a t i o n a r y phase: 10 % dimethylphthalate mobile phase : dimethylformamide/ 0 . 5 N hydrochloric a c i d 15:85 The drug substance i s v i s u a l i z e d by r e a c t i o n with i o d i n e vapour
.
Rf values of bromocriptine and precursor system 1
system 2
0.88
0.09
0.70
0.31
Bromocriptine a- ergocr yp t i n e (precursor) 7 . 4 2 Thin Layer
The r e l a t i v e i n s t a b i l i t y of bromocriptine makes it very d i f f i c u l t t o avoid a r t i f a c t formation i n t e s t s o l u t i o n s o r during s p o t t i n g on t h e p l a t e . Therefore, bromocriptine mesil a t e , u s u a l l y d i s s o l v e d i n chloroform/methanol 1:1, has t o be s p o t t e d on t h e p l a t e very r a p i d l y and with t h e exclusion of l i g h t . The s e p a r a t i o n being terminated, t h e mobile phase i s removed by means of high vacuum f o r 30 minutes. A g r e a t number of t l c systems have been i n v e s t i g a t e d f o r t h e s e p a r a t i o n of by-products, degradation products, metabol i t e s , and e x c i p i e n t s . Also a v a r i e t y of spraying r e a g e n t s have been t e s t e d ( s e e t a b l e ) . The most advantageous one w a s Dragendorff's r e a g e n t with consecutive spraying by 30 % hydrogen peroxide. methods: s t a t i o n a r y phase: s i l i c a g e l 60 F254, Merck t l c p l a t e s , no.5715 mobile phase 1
:
(27)
dichloromethane/dioxane/96 p e r c e n t ethanol/conc.ammonia (v/v/v/v)
180:15:5:0.1
mobile phase 2
:
chloroform/methanol/formic a c i d 7 8 :20 : 2 (v/v/v)
mobile phase 3
:
chloroform/96 p e r c e n t ethanol/conc. ammonia 192:8:0.35 (v/v/v)
I n the procedure with mobile phase 1 and 2 , t h e visual i z a t i o n i s accomplished by screening under uv l i g h t (254 and 366 nm) and i n a d d i t i o n by spraying with Dragendorff's reagent, modified by Munier and Deboeuf, followed by 30 perc e n t hydrogen peroxide.
DANIELLE A. GIRON-FOREST AND W. DIETER SCHONLEBER
72
values st mobile phase 1 mobile phase 2 R
compound bromocr i p t i n e
2-bromo-a-ergocryptinine
1 . 0 (Rf 0.5) 1.5
a-ergocryptinine (isomer of precursor) a-ergocryptine (precursor) 2-bromo-lysergic a c i d 2-bromo-isolysergic a c i d 2-bromo-lysergamide 2-bromo-isolysergamide
1.4 0.6 0.0
0.0 0.5 0.5
1 . 0 (Rf 0.7) 1.1 1.0 0.5 0.25 0.35 0.15 0.35
Mobile phase 3 may be used f o r t h e d e t e c t i o n and s e m i q u a n t i t a t i v e determination of r e s i d u a l N-bromosuccinimide. Thereby, t h e p l a t e i s sprayed with water and then placed i n a c h l o r i n e atmosphere f o r 10 minutes. Excess c h l o r i n e i s removed by p l a c i n g t h e p l a t e i n a stream of w a r m a i r f o r another 1 0 minutes. A f t e r spraying with o - t o l u i d i n e reagent, the eval u a t i o n i s made a g a i n s t a d i l u t i o n of N-bromosuccinimide. i s 0.3 with r e s p e c t t o The d e t e c t i o n l i m i t i s 0 . 1 pg, t h e R st bromocriptine R f value. A high performance t l c system has been developped f o r t h e in-process-control (28) using Merck s i l i c a g e l HPTLC p l a t e s , no. 5628, a s t h e s t a t i o n a r y phase and tetrahydrofuran/ chloroform/n-heptane/methanol/conc. ammonia 20:20:57:7:1 p e r volume a s t h e mobile phase. The chromatography ( 6 cm ascending) i s c a r r i e d o u t without preceding chamber s a t u r a t i o n . The compounds separated a r e v i s u a l i z e d by uv a t 254 and 366 nm, r e s p e c t i v e l y , and by i o d i n e vapour. Rf of bromocriptine i s 0.27. The p o t e n t i a l by-products y i e l d s p o t s a t R 1.5 s (2-bromo-a-ergocryptinine) , and 0.55 (a-ergocryptiney 2-Bromo-lysergic a c i d remains a t the s t a r t i n g p o i n t .
.
Beside t h e modified Dragendorff's reagent/hydrogen peroxide a l r e a d y mentioned, a v a r i e t y of spraying reagents has been used f o r t h e v i s u a l i z a t i o n of bromocriptine. They a r e compiled i n t h e following l i s t .
BROMOCRIPTINE METHANESULPHONATE
reagent
spraying r e a g e n t s f o r bromocriptine detection l i m i t colour on s i l i c a g e l Merck no. 5715
Dragendorff (Munier,Deboeuf) + 30 p e r c e n t H 2 0 2 0.05 p e r c e n t aqueous permangana t e van U r k ' s r e a g e n t cinnamic aldehyde formaldehyde/hydrochloric acid formaldehyde/sulphuric a c i d chlorine/o-toluidine folin/ammonia ninhydrin/uv d e t . 360 iodine/potassium i o d i d e E h r l i c h ' s reagent
brown yellow grey yellow grey violet violet grey red brown orange
The i d e n t i t y of methanesulphonic a c i d may be determined by t l c on c e l l u l o s e p l a t e s , Merck no. 5728, with ethanol/ water/conc. ammonia 80:16:4 (v/v/v) a s a mobile phase. Detection i s achieved by spraying with acid-base i n d i c a t o r s , e.g. bromocresol green o r s i m i l a r s p e c i e s . Rf of methanesulphonic a c i d i s 0.5 ( t h a t of bromocriptine base = 0.9). 7.43 G a s Chromatography GC cannot be a p p l i e d t o t h e a n a l y s i s of bromocriptine m e s i l a t e due t o i t s low v o l a t i l i t y and i t s thermal i n s t a b i l i t y . A procedure according t o 29 o r 30, which claims e x c e l l e n t i d e n t i f i c a t i o n and q u a n t i t a t i o n on t h e b a s i s of well-defined p e p t i d e s e c t i o n p y r o l y s i s products, h a s n o t y e t been attempted. However, GC i s very u s e f u l determining t h e r e s i d u a l r e c r y s t a l l i z a t i o n s o l v e n t butanone-2. The c o n d i t i o n s a r e t h e following:
Column : Porapak Q 80/100 mesh, i n 1.8 m x 2mm g l a s s Temperatures: i n j e c t o r 240 OC, column 130 O C flame i o n i z a t i o n d e t e c t o r , 240 OC. 7.44 High Performance Liquid A s e r i e s of HPLC systems have been u t i l i z e d both f o r assay and p u r i t y of bromocriptine m e s i l a t e . S a t i s f a c t o r y procedures have been accomplished both on s t r a i g h t phase ( s i l i c a g e l ) and on reversed phase ( o c t a d e c y l s i l a n i s e d s i l i c a g e l ) columns.
74
DANIELLE A. GIRON-FOREST AND W. DIETER SCHONLEBER
HPLC-conditions s tr ai gh t-phase: -s t a t i o n a r y phase: s i l i c a g e l , 5 pm, i n s t a i n l e s s s t e e l 25 cm x 3 mm i.d. mobile phase: water-saturated dichloromethane/methanol 100:2 (v/v) uv d e t e c t i o n a t 254 nm. F i g . 11 shows a chromatogram of bromocriptine mesilate spiked w i t h dodecylbenzene, p o t e n t i a l by-products and t h e p r e c u r s o r . The flow was 1.7 ml/minute ( 3 1 ) . Key: 1 = dodecylbenzene, 2 = bromocriptinine, 3 = a-ergocrypt i n i n e , 4 = bromocriptine, 5 = a-ergocryptine ( p r e c u r s o r ) .
reversed - - - -phase, --
zyste?l_I:
s t a t i o n a r y phase: Merck F@-18, 1 0 pm i n s t a i n l e s s s t e e l 25 c m x 4.6 mm i . d . mobile phase: g r a d i e n t : 35 t o 60 p e r c e n t B w i t h i n 60 min. A = water, 0 . 2 p e r c e n t t r i e t h y l a m i n e added B = a c e t o n i t r i l e , 0.2 p e r c e n t t r i e t h y l a m i n e added. uv d e t e c t i o n a t 280 nm. This system was found optimal f o r t h e p u r i t y t e s t . Fig. 1 2 shows a chromatogram of t h e drug substance spiked with p o t e n t i a l by-products and the precursor. The flow was s e t a t 4.0 ml/minute. Key: I = 2-bromo-a-ergocryptinine, I1 = a-ergocryptinine, 111 = a-ergocryptine ( p r e c u r s o r ) , I V = bromocriptine, V = 2-bromo-lysergamide, V I = 2-bromo-lysergic a c i d , V I I = 2-bromo-isolysergamide.
reversed-p&azeL --ZyEtgm-II-
(26) :
s t a t i o n a r y phase: Merck RP-18, 10 pm i n s t a i n l e s s s t e e l , 25 cm x 4.6 mm mobile phase: 0.01 M ammonium carbonate o r 0.05 M ammonium hydrogen carbonate s o l u t i o n / a c e t o n i t r i l e 35:65 i s o c r a t i c , flow 1 . 5 ml/min.
BROMOCRIPTINE METHANESULPHONATE
75
I
1
3
I Figure 11.
5
High Performance Liquid Chromatogram of Bromocriptine Mesilate, spiked with Dodecylbenzene, Precursor and p o t e n t i a l By-products. Adsorption Mode, i s o c r a t i c , Uv-detection a t 254 nm
DANIELLE A. GIRON-FOREST AND W. DIETER SCHONLEBER
76
5
1 c
0
c 2
Figure 1 2 .
4
6
8
10
12
L 14
L 16
18
20 min
High Performance Liquid Chromatogram of Bromocriptine M e s i l a t e , spiked w i t h Precursor and p o t e n t i a l By-products. Reversed-phase Mode, Solvent Gradient, Uv-detection a t 280 nm.
BROMOCRIF'TINE METHANESULPHONATE
7.5
71
D i f f e r e n t i a l Scanning Calorimetry
D i f f e r e n t i a l scanning c a l o r i m e t r y cannot be a p p l i e d t o q u a n t i f y t h e p u r i t y of t h e drug substance f o r t h e reasons mentioned i n 2.31 and 2.34. However, i t may be v a l u a b l e i n q u a l i t a t i v e comparisons from sample t o sample o r batch t o batch on t h e b a s i s of t h e i r corresponding d i f f e r e n t i a l scanning c a l o r i m e t r y p a t t e r n s . 7.6
Phase S o l u b i l i t y Analysis
For phase s o l u b i l i t y a n a l y s i s , a c e t o n i t r i l e appears t o be t h e most s u i t a b l e s o l v e n t . A t y p i c a l p l o t i s given i n f i g u r e 13 along w i t h t h e experimental conditions. 7.7
Analysis of t h e Dosage Form
The i d e n t i f i c a t i o n o f bromocriptine m e s i l a t e i n t h e dosage form c a n be c a r r i e d o u t by t h i n l a y e r chromatography using Merck p l a t e s with dichloromethane/methanol/formic a c i d 78:20:2 (v/v/v) and subsequent u v - v i s u a l i z a t i o n a t 254 and 360 run. Using t h i s method, i t i s important t o only a i r - d r y t h e s p o t a f t e r a p p l i c a t i o n t o t h e p l a t e , s i n c e more vigorous evaporation of t h e s o l v e n t w i l l g i v e r i s e t o a r t i f a c t s ( 3 2 ) . Bromocriptine can a l s o be i d e n t i f i e d a s t h e base by i r spectroscopy a f t e r e x t r a c t i o n from t h e dosage form with ethanol and removal of t h e s o l v e n t , both i n s o l u t i o n and i n a KBr p e l l e t ( 3 3 ) . Bromocriptine m e s i l a t e i n P a r l o d e l a t a b l e t s may be assayed i n a non-specific way by d i r e c t uv-spectrophotometry following e x t r a c t i o n with methanol ( 3 2 )
.
Fluorimetry i n 0 . 1 N hydrochloric a c i d has been a p p l i e d during t h e measurement of d i s s o l u t i o n r a t e of t h e dosage forms with e x c i t a t i o n a t 335 and emission a t 425 nm, r e s p e c t i v e l y (26)
-
A s p e c i f i c a s s a y of bromocriptine m e s i l a t e i n t h e dosage form may be c a r r i e d o u t by t l c followed by uv-spectrophotometry ( 2 6 ) (The system can a l s o s e r v e f o r i d e n t i f i c a t i o n p u r p o s e s ) . The drug substance i s e x t r a c t e d with methanol i n t h e absence of l i g h t , t h e chromatographic c o n d i t i o n s a r e : Merck p l a t e s F 254, mobile phase: dichloromethane/dioxane/ ethanol abs./conc. ammonia 180:15:5:0.1 per volume. The s p o t corresponding t o bromocriptine i s e x t r a c t e d with methanol, and t h e c o n c e n t r a t i o n i s determined a t about 300 nm by spec tropho tometry.
78
DANIELLE A. GIRON-FOREST AND
SYSTEfl COMPOSITION: MG OF SAMPLE PER
Figure 13.
w. DIETER SCHONLEBER
G OF SOLVENl
Phase Solubility Analysis Plot of Bromocriptine Mesilate, dried in High Vacuum for 15 Hours. Solvent: dry Acetonitrile, Vibration for 24 hrs. in the Absence of Light. Slope 1.41~0.05 %.
BROMOCRIF'TINE METHANESULPHONATE
79
A f u r t h e r s p e c i f i c assay i s t h e HPLC-determination of bromocriptine m e s i l a t e following e x t r a c t i o n with methanol from t h e dosage form using RP-18 a s t h e s t a t i o n a r y and aceton i t r i l e / O . O l M ammonium carbonate s o l u t i o n 65:35 a s t h e mobile phase. Uv-detection wavelength i s s e t a t 300 nm ( 2 6 ) .
For t h e d e t e c t i o n and e s t i m a t i o n of degradation products
i n dosage forms, a s o l v e n t g r a d i e n t , c o n t a i n i n g t h e components mentioned above, i s u t i l i z e d with advantage. 7.8
Determination i n Body F l u i d s and T i s s u e s ( 2 3 )
Due t o i t s p o t e n t e f f i c a c y i n t h e treatment of hyperprolactinemia and acromegaly, bromocriptine i s administered i n low doses leading t o minute c o n c e n t r a t i o n s i n body f l u i d s and t i s s u e s . Therefore, none b u t t h e most s e n s i t i v e a n a l y t i c a l methods can be used t o measure i t s c o n c e n t r a t i o n i n b i o l o g i c a l specimens. The only method so f a r a p p l i c a b l e f o r pharmacok i n e t i c s t u d i e s with bromocriptine i s t h e u s e of t h e r a d i o a c t i v e l y l a b e l l e d drug, measurement of t o t a l r a d i o a c t i v i t y and i t s f r a c t i o n a t i o n by chromatographic s e p a r a t i o n techniques f o r t h e assay of p a r e n t drug and major metabolites. Recently, a radioimmunoassay k i t f o r t h e a n a l y s i s of picogram q u a n t i t i e s of unchanged bromocriptine i n body f l u i d s has become a v a i l a b l e . G a s chromatography, mass fragmentography and l i q u i d chromatography a l s o appear t o be s u i t a b l e f o r determining bromocriptine i n plasma from p a t i e n t s with P a r k i n s o n ' s d i s e a s e which a r e on treatment a t high dose l e v e l s . These c u r r e n t l y developped procedures permit q u a n t i t a t i v e determinations down t o c o n c e n t r a t i o n s of 0.5 (GC) , 1 . 0 (MF), and 1 0 ng/ml (LC), respectively ( 3 4 ) . The p a t t e r n of m e t a b o l i t e s i n b i l e (animals o n l y ) and i n u r i n e have been i n v e s t i g a t e d using column chromatography (Amberlite XAD 2 and Sephadex D E A E ) , t l c and reversed phase HPLC i n combination with r a d i o a c t i v i t y monitoring. The p r i n c i p a l metabolites have been i s o l a t e d from t h e b i l e of r a t s t r e a t e d with high doses of bromocriptine. The s t r u c t u r e of t h e i s o l a t e d m e t a b o l i t e s was e l u c i d a t e d by means of spectroscopic techniques.
DANIELLE A. GIRON-FOREST AND
80
w. DIETER SCHONLEBER
8.
References
1. 2.
F.Troxler and A.Hofmann, Helv.Chim.Acta 2, 2160 (1957) Handbook of Experimental Pharmacology, Vol. 49:"Ergot Alcaloids and Related Compounds", B.Berde and H.O.Schild, Ed., Springer-Verlag, Berlin, Heidelberg, New York, 1978 E.Fluckiger, F.Troxler, and A.Hofmann, German Offenlegungsschrift no. 1 926 045 (1969) E. Kovacs and E.Fluckiger, Experientia 30, 1172 (1974) J.K.Murdoch, Can.J.Hosp.Pharm. (1977) 149 H.Gjonnoes, Tidsskr.Nor.Laegeforen 97, 1405 (1977) A.Saarinen, V.Myllila, M.Reunanen, and E-Hokkanen, Duodecim 93, 1219 (1977) Triangle, Sandoz Journal of Medical Science, g(1)(1978) Symposium on Bromocriptine, Special Supplement, The Medical Journal of Australia, Vol 2, no. 3 (1978) W.J.Weiner, P.A.Nausieda, and H.I.Klawans, Neurology 28, 734 (1978) H.R.Schneider, P.A.Stadler, P.Stutz, F.Troxler,and J.Seres, Experientia 33, 1412 (1977) W.D.Schonleber , A.L. Jacobs, and G. A.Brewer, jr. :"Dihydroergotoxine mesilate" in Analytical Profiles of Drug Substances 1,81 B. Kreilgaard, "Ergotamine tartrate" in Analytical Profiles of Drug Substances 6, 113 T.Inone, Y.Nakahara, and T.Niwaguchi, Chem.Pharm.Bul1. 20, 409 (1972) D.Voigt, S.Johne, and D.Groger, Pharmazie 29, 697 (1974) H.P.Weber, Sandoz Ltd., personal communication H-Bethke, B.Delz, and K.Stich, J.Chromatog. 123, 193 (1976) A.Hofmann: Die Mutterkornalkaloide, F.Enke Verlag, Stuttgart, GFR, (1964) P. Gull and P.A.Stadler, Sandoz Ltd., personal communication Sandoz stability report for drug substance Sandoz stability reports for Parlodel capsules and tablets This part was kindly contributed by E.Schreier, Sandoz Ltd. A.Ehmann, J-Chromatog. 132, 267 (1977) V.Creutzburg-Biermanova, Sandoz Ltd., personal communication
3.
4. 5. 6. 7. 8. 9. 10. 11.
12.
13.
14.
L
15. 16. 17. 18.
19.
20. 22. 23. 24. 25.
BROMOCRIPTINE METHANESULPHONATE
26. 27. 28. 29. 30.
31. 32.
33. 34.
81
Control procedure for dosage form, Sandoz Ltd. Control procedure for drug substance, Sandoz Ltd. R.Stampfli, Sandoz Ltd., personal communication F.J.W.Van Mansvelt, J.E.Greving, and R.A.De Zeeuw, J.Chromatog. 151, 113 (1978) T.A.Plomp, J.G.Leferink, R.A.A.Maes, J.Chromatog. 151, 121 (1978) H.P.Keller, Sandoz Ltd., personal communication W-Ableidinger,Sandoz Ltd., personal communication M.Devaud, Sandoz Ltd., personal communication N.-E.Larsen, R.Oehman, M.Larsson, E.F.Hvidberg, to be published in Clin. Chem. Acta.
Acknowledgments The authors are indebted to many colleagues at SandozWander Ltd. for their most valuable help, in particular to Messrs. H.-R. Loosli, H.P. Weber and E. Schreier. The technical assistance for the proper presentation of the mass spectrum by Prof. W. Simon, at the Swiss Federal Institute of Technology in Zurich, is gratefully acknowledged. Furthermore, the authors wish to express special thanks to Miss Moret for her secretarial assistance in preparing this manuscript.
Analytical Profiles of Drug Substances, 8
CALCITROL Eileen Debesis I. 2.
3. 4. 5. 6.
7. 8.
Description I . I Name, Formula, Molecular Weight I .2 Appearance, Color, Odor Physical Properties 2.I Infrared Spectrum 2.2 Nuclear Magnetic Resonance Spectrum 2.3 Ultraviolet Spectrum 2.4 Mass Spectrum 2.5 Melting Range 2.6- Differential Scanning Calorimetry 2.7 Thermogravimetric Analysis 2.8 Hot Stage Microscopy 2.9 Solubility 2.10 X-Ray Powder Diffraction 2.1 I Optical Rotation Synthesis Stability and Degradation Drug Metabolic Products Methods of Analysis 6. I Elemental Analysis 6.2 Chromatographic Methods 6.2 I Thin-Layer Chromatography 6.22 High Performance Liquid Chromatography 6.23 Gas Chromatography-Mass Spectrometry 6.3 Biological Methods 6.3 I Radioimmunoassay 6.32 Protein Binding Assay 6.33 Bioassay 6.4 Polarography Acknowledgments References
83
Copyright @ 1979 by Academic Press. Inc. All rights of reproduction in any form reserved.
ISBN 0-12-260808-9
EILEEN DEBESIS
84
1.
Description 1.1 Name, Formula, Molecular Weight Calcitriol is 1 a, 2 5 - d i h y d r o x y c h o l e c a l c i f e r o l .
MW = 416.65 27"44'3
1.2 Appearance, Color, Odor Calcitriol is an odorless white crystalline powder. 2.
Physical Properties 2.1 Infrared Spectrum The infrared spectrum of calcitriol is shown in Figure 1 (1). The spectrum was recorded on a Perkin-Elmer Model 283 Grating Infrared Spectrophotometer and was measured in a KBr pellet which contained 1 mg of calcitriol in 300 mg of KBr. Figure 1: a.
b. c. d.
The following absorptions have been assigned for OH stretching (bonded): 3391 cm-l Aliphatic CH stretching: 2943,12872 cm-l CH deformation: 1468, 1318 cmC-0 stretching: 1056 cm-
2.2 Nuclear Magnetic Resonance Spectrum (NMR) The NMR spectrum of calcitriol, recorded on a Varian XL-lOO/Nicolet TT-100 pulsed Fourier Transform NMR spectrometer, with internal deuterium lock, is shown in Figure 2 (2). The spectrum was recorded using a solution of 0.84 mg of sample dissolved in 50 microliters of CD30D (100%D) containing 1% v/v tetramethylsilane in a 1.7 mm capillary tube. The spectral assignments are given in Table I.
WAVELENGTH (MICRONS)
2.5
3.0
4.0
5.0
6.0
8.0
10
I
I
I
I
I
I
I
I
16 20 25 1
I
I
100 -
0
I
I
I
I
I
I
I
Figure 1 Infrared Spectrum oE Calcitriol
I
I
I
!
87
CALCITRIOL
H
Table I NMR Spectral Assignments for Calcitriol Proton
Chemical Shift (a)
Multiplicity
-CH3(C18)
0.57
Sing1et
-CH3(C21>
0.95
Doublet
-CH3(C26,27 \
\
X H 2 , ;CH HO. ;CH ~
1
-1.16
Singlet
-1.38-3
Complex
4.08
Comp 1ex
4.32
Triplet
4.90, 5.28
Complex
6.07, 6.32
AB Quartet JAB = 11 Hz
/ -
Ho> I CH -
- CH2
HDO + 3 x OH (exchangeable protons) 4.78
EILEEN DEBESIS
88
2.3 Ultraviolet Spectrum The ultraviolet spectrum of calcitriol (1 mg of Calcitrio1/100 ml of absolute ethanol) in the region of 220 to 400 nm exhibits one maximum at 264 nm (E = 1.9 x 10 ) and one minimum at 226 nm. The spectrum is shown in Figure 3 (3). Mass Spectrum The low resolution mass spectrum of calcitriol is shown in Figure 4 (4). The spectrum was obtained using a Varian MAT CH5 spectrometer, which was interfaced with a Varian data system 620 I. The data system accepts the output of the spectrometer, calculates the masses, compares the intensities to the base peak, and plots this information as a series of lines whose heights are proportional to the intensities, 2.4
'
The molecular ion was measured at m/e = 416. Other characteristic masses were observed at m/e = 398, 380 and 362, corresponding to the l o s s of one, two and three molecules of water, respectively, from the molecular ion; m/e = 383, corresponding to the loss of water and CH3 from the parent peak; and m/e = 365, corresponding to the l o s s of two water molecules and one CH from the molecular ion. The base peak is 3 observed at m/e = 134, and corresponds to the
2.5
+Hf$!
..
moiety H
Melting Range Calcitriol melts at 111-115"C (3).
2.6 Differential Scanning Calorimetry Melting was accompanied by decomposition (5). Thermogravimetric Analysis Calcitriol was subjected to thermogravimetric analysis on a Perkin-Elmer Model TGS-1 Thermogravimetric Analyzer. The sample exhibited two overlapping weight losses. The initial weight loss, of 0.4%, began at 55°C and ended at 105"C, and was due to surface moisture or solvent. The second weight l o s s , due to decomposition, amounted to 2.5% at 205"C, 7.5% at 255"C, 33% at 305"C, and 93% at 355°C (5). 2.7
2.8 Hot Stage Microscopy As observed on a Mettler Hot Stage FP 52 with FP5 controller, the sample appeared as birefringent needle-like crystals which melted from 115-117°C. The sample did not recrystallize from the melt (5).
CALCITRIOL
89
0.6
0.5
0.4 W
0
z a
3 0.3 8
m U
0.2
0.I
0 250
300 NANOMETERS
Figure 3 Ultraviolet Spectrum of Calcitriol
350
Q)
a Kn
91
CALCITRIOL
2.9 Solubility Extensive solubility data is not readily obtainable due to the scarcity of calcitriol. The material is slightly soluble in methanol, ethanol, ethyl acetate and tetrahydrofuran ( 3 ) . 2.10 X-Ray Powder Diffraction The X-ray powder diffraction data for calcitriol are presented in Table I11 ( 3 ) ; instrumental conditions are given below. The diffraction pattern is shown in Figure 5. Instrument and Operating Conditions Instrument
Guinier-De Wolff Camera
Generator
GE XRD-6 50 KV, 12.5 mA
Detector
Film
Sample
As is
Densitometer"
Gelman DCD-16
Optics
Tungsten Lamp 575 nm Visible mode
Detector
Silicon phototransistor
Optical density
0.25
Beam exit slit
0.53 mm
*The diffraction pattern was recorded on film; the density of the individual lines in the pattern was determined by densitometry.
o
m
u
id a
a c.
93
CALCITRIOL
TABLE I11
Calcitriol Powder Diffraction Data 20
I/Io**
26.52 13.33 22.41 20.89 18.01 28.97 27.33 23.70 33.55 30.54 31.77 17.19 24.95 21.54 28.04 32.66 19.46 20.35 16.07 11.37 8.03 34.18 12.07
4.993 9.863 5.892 6.316 7.314 4.578 4.847 5.577 3.968 4.348 4.183 7.662 5.302 6.129 4.727 4.072 6.776 6.480 8.192 11.559 16.343 3.896 10.889 A
100 90 88
82 70 66 49 44 36 34 33 33
26 26 15 12 12 12 2
2 2 2
1
(interplanar distance)
*d
--
**I/Io
= percent relative intensity (based on maximum
2 Sin 0
intensity of 1.00)
2.11 Optical Rotation The specific rotation of calcitriol in absolute methanol, measured at 589 nm and 2SoC, was +48' ( 7 ) .
EILEEN DEBESIS
94
Synthesis Several procedures for the synthesis of calcitriol have et a1.(8) and Norman been reported in the literature. Parren -et al. (9) described the preparation of calcitriol from 25-hydroxyvitamin D3. Uskokovic and others (10-18) have described lengthier syntheses utilizing more readily available starting materials. A typical reaction scheme, utilizing 1 a, 25-diacetoxy-7-dehydrocholesterol as the starting material, is shown in Figure 6. 3.
Stability and Degradation Calcitriol must be protected from air and light. The drug substance exhibits good stability when stored at -15'C to -25'C in an argon atmosphere. The material is stable at room temperature when dissolved in a vegetable oil derivative, containing antioxidants, such as is used in calcitriol soft gelatin capsules (19). 4.
5.
Drug Metabolic Products Calcitriol may be absorbed directly into the intestine or bone, or may be hydroxylated to form 1 a, 24, 25-trihydroxycholecalciferol prior to intestinal absorption (20-24). Methods of Analysis 6.1 Elemental Analysis A typical elemental analysis of a sample of calcitriol is presented in Table IV (7);
6.
TABLE IV Elemental Analysis of Calcitriol E 1ement
% Theory
C H
77.84 10.64 11.52
0
% Found
77.53 10.75 11.92 (by difference)
2 o 2 v
0 ,
yz
g
x3R
I 0
O--
0
r
0 I
I
8
m
rn
1
1
0
r
8
'.
L
.rl V
0
r(
c,
k
.rl *+-I
I .rl
EILEEN DEBESIS
96
6.2 Chromatographic Methods 6.21 Thin-Layer Chromatography (TLC) The following TLC procedure is useful for determining the purity of calcitriol. It separates the previtamin, 1 a, 25-dihydroxyprecholecalciferol. A silica gel GF plate is activated by heating for one hour at 105OC and is then cooled in a desiccator. A low actinic all glass chromatographic chamber is equilibrated with the developing solvent, and 0.8 mg of calcitriol is applied to the plate from ethyl acetate. The plate is developed in an ascending mode in ethyl acetate:spectroquality heptane:methanol (100:10:2) for 15 cm. After air drying, the plate is viewed under shortwave ultraviolet radiation, then sprayed with a 15% w/v solution of phosphomolybdic acid in ethanol, followed by heating at 105OC for 10 minutes to develop the colors. The approximate R f values are summarized in Table V ( 3 ) . TABLE V Summary of TLC Data Compound 1 a, 25-Dihydroxyprecholecalciferol Calcitriol
Approximate R 0.4 0.5
6.22 High Performance Liquid Chromatography High performance liquid chromatography is used to determine the purity of calcitriol, and to separate it from related compounds. Using a 10 micron silica column of 25 cm length, and a mobile phase of spectroquality heptane: ethyl acetate:methanol (50:SO:l) at a flow rate of 1.7 ml/ minute, separation and quantitation are achieved. p-Dimethylaminobenzaldehyde may be used as an internal standard to compensate for variations in injection technique and instrumental conditions. With a 254 nm ultraviolet absorbance detector, 0.01 ug of calcitriol may be detected ( 3 ) . This procedure, with a mobile phase of spectroquality heptane:ethyl acetate:methanol (70:25:5) is also useful for analyzing calcitriol in soft gelatin capsules. The capsule fill solution may be injected directly. The amount of calcitriol in the capsule is determined by comparison to a calcitriol reference standard, prepared in a medium similar to the capsule fill ( 3 ) .
97
CALCITRIOL
6.23 Gas Chromatography - Mass Spectrometry Halket and Lisboa (25) examined several Vitamin D derivatives by capillary gas chromatography coupled with mass spectrometry. This technique offered the advantages of great sensitivity and separating power. Retention times and fragmentation patterns for ergocalciferol, cholecalciferol and calcitriol were reported. 6.3 Biological Methods 6.31 Radioimmunoassav Several workers (26-32) have reported on the use of radioimmunoassay for measuring calcitriol at very low (pg) levels in serum. 6.32 Protein Binding Assays Various protein binding techniques are reported (32-42) for the determination of calcitriol in plasma. Generally, a preliminary purification step is required to avoid interference from other plasma components. 6.33 Bioassays Stern. et al. (43.44) reDorted a bioassav technique based on fetal rat bone absorption of calcitriol. Parkes and Reynolds (45) developed an in-vitro bioassay using duodenal tissue from chicken embryos. .
.
<
A
6.4 Polarography Calcitriol drug substance may be analyzed polarographically, using a glassy carbon working electrode. The limiting current of the observed oxidation wave (E 0.96 v> is linear with concentration in the 0.01 tol6203 m~ region (46). 7.
Acknowledgments The author wishes to thank the staffs of the Scientific Literature Department and Research Records Office of HoffmannLa Roche Inc., Nutley, NJ.
EILEEN DEBESIS
98
8.
References 1. 2. 3. 4. 5.
6.
7. 8. 9.
10.
11. 12.
13. 14. 15. 16. 17. 18. 19. 20.
Ng, S., Hoffmann-La Roche, Inc. Personal Communication. Grant, Anne, Hoffmann-La Roche, Inc. Personal Communication. Rubia, Linda, Hoffmann-La Roche, Inc. Personal Communication. Benz, W . , Hoffmann-La Roche, Inc. Personal Communication. Ramsland, Arnold, Hoffmann-La Roche, Inc. Personal Communication. Macri, Frank, Hoffmann-La Roche, Inc. Personal Communication. Scheidl, F . , Hoffmann-La Roche, Inc. Personal Communication. Paaren, H. E., Hamer, D. E., Schnoes, H. K., and DeLuca, H. F . , Proc. Nat2. Acad. S c i . USA, 75, 2080 (1978). Norman, A. W., Myrtle, J. F., Midgett, R. J., and Nowicki, H. G., U.S. 3 , 772, 150 (November 13, 1973); CA 80:105146g (1974). Uskokovic, M. Baggiolini, E., Mahgoub, A., Narwid, T., and Partridge, J. J. , Vitamin D and ProbZems Related t o Uremic Bone Disease, Walter de Gruyter, Berlin, New York, 279 (1975). Okamura, U. H., Am. Chem. Soc. Abstr. Pap. 275th ACS Natl. Meet., Anaheim, California, Mar. 13-17, 1978, MEDI #32 (1978). Matsunaga, I., Ochi, K., Nagano, H., Shindo, M., Ishikawa, M., Kaneko, C., and DeLuca, F . H., to Chugai Pharmaceutical Co., Ltd. Japan Kokai 76 100,056 (September 3, 1976); CA 8639014313 (1977). Suda, T. , Horiuchi, N., and O g a t c E. , Tampakushitsu Kakusan Koso, 21, 844 (1956). DeLuca, H. F., TetrahehTn Lee&, 1972, 4147. Cohen, Z., Keinan, E . , Mazur, Y., and Ulman, A., J . Org. Chern., 41, 2651 (1976). Mielczarek, I., Wiad. Chem., 28, 813 (1974). 33, Kaneko, C. , Yuki Gosei KagakuTyokai Shi, 75 (1975). Barton, D. H. R., Hesse, R. H., Pechet, M. M., and Rizzardo, E., J . Chem. Soc., Chem. Commun., 1974, 203. Johnson, J. B., Hoffmann-La Roche, Inc. Personal Communication. Napoli, J. L., Vitamin D and Its Metabolites, Annu. Rep. Med. Chem., 10, 295 (1975).
r,
CALCITRIOL
21. 22. 23. 24. 25. 26. 27. 28. 29. 30.
31. 32. 33. 34.
35. 36.
99
Kumar, R., and Deluca, H. F., Biochm. Biophys. Res. Commun., 69, 197 (1976). Kumar, R., Harnden, D., and DeLuca, H. F., Biochemistry, 15, 2420 (1976). Harnden, D., Kzar, R., Holick, M. F., and DeLuca, H. F., Science, 193,493 (1976). Castillo, L., DeLuca, H. F., and Ikekawa, N., J . BioZ. Chem., 252, 1421 (1977). Halket, J. M., and Lisboa, B. P., Acta. Endocrinol., (Copenhagen), 87, (Suppl. 215), 120 (1978). Clemens, T. L., Hendy, G. N., Graham, R. F., Baggiolini, E. G., Uskokovic, M. R., and O'Riordan, J. L. H., Endocrinology, 102 (Suppl.), 490 (1978). Schaefer, P. C., LifschitrM. D., Fadem, S. Z. and Goldsmith, R. S., Endocrinology, 102, (Suppl.), 320, (1978). Clemens, T. L., Hendy, G. N., Graham, R. F., Baggiolini, E. G., Uskokovic, M. R., and O'Riordan, J. L. H., J . Endocrinol. 77, 49P (1978). Clemens, T. L., Hendy, G.N., Graham, R. F . , Baggiolini, E. G . , Uskokovic, M. R., and O'Riordan, J. L. H., Clin. Sci. Mol. Med. Med., 54, 329 (1978). Fairney, A . , Turner, C., Baggiolini, E . G., Uskokovic, M. R., in Vitamin D: BiochLmioal, Chemical, and Clinical Aspects Related t o Calciwn MetaboZism, A. W. Norman, K. Schaefer, J. W. Coburn, H. F. DeLuca, D. Fraser, H. G. Grigoleit, D. von Herrath [eds.], Walter de Gruy-ter, Berlin, New York, 459 (1977). Eisman, J. A . , Hanistra, A . J., Kream, B. E., DeLuca, H. F., Arch. Biochem. Biophys., 176, 235 1976). Etsuko, A . , Suda, T., Nakano, H., Igaku No A y w n i , 102, 509 (1977). Brumbaugh, P. F . , Haussler, D. H., Bressler, R., and Haussler, M. R., Science, 183, 1089 (1974). Caldas, A . E., Gray, R. W., Lemann, J., Jr., J . Lab. CZin. Med., 91, 840 (1978). Shimura, F . , and TamGa,.M., Vitamins, 52, 173 (1978). Horst, P. L., Merchant, C . , Shephard, R., Hamstra, A . Jorgensen, N. A . , DeLuca, H. F . , J . Dairy S c i . , 60, (Suppl. l), 123 (1977).
EILEEN DEBESIS
100
37.
38.
39. 40.
41. 42. 43. 44.
45.
46.
Kream, B. E., Eisman, J. A., DeLuca, H. F., in Vitamin D: Biochemical, Chemical and Clinical Aspects Related t o Calcium Metabolism, A. W. Norman, K. Schaefer, J . W. Coburn, H. F. DeLuca, D. Fraser, H. C. Grigoleit, and D. von Herrath, [eds.], Walter de Gruyter, Berlin, New York, 501 (1977). Haussler, M. R., Hughes, M. R., Pike, J. W., McCain, T. A,, in Vitamin D: Biochemical, Chemical and Clinical Aspects Related t o Calcium Metabolism, A. W. Norman, K. Schaefer, J . W. Coburn, H. F. DeLuca, D. Fraser, H. C. Grigoleit, and D. von Herrath, [eds.], Walter de Gruyter, Berlin, New York, 473 (1977). Norman, A. W., Henry, H., Bishop, J. E., Coburn, J. W., CZin. Res., 26, 423A (1978). Eisman, J. A., Hamstra, A. J., Kream, B. E., DeLuca, H. F., Science, 193, 1021 (1976). Hughes, M. R., Baylink, D. J., Jones, P. G., Haussler, M. .R., J. CZin. Inuest. , 58, 61 (1976). Brumbaugh, P. F., Haussler, D. H., Bursac, K. M., Haussler, M. R., Biochemistry, 13, 4091 (1974). Stern, P. H., Hamstra, A. J., Dxuca, H . F., Bell, N. H., J. Clin. Edocrinol. Metab., 46, 891 (1978). Stern, P. H., Phillips, T. E., Lucas, S. V., Hamstra, A. J., DeLuca, H. F., Bell, N. H., in Vitamin D: Biochemical, Chemical and Clinical Aspects Related t o Calciwn Metabolism, A. W. Norman, K. Schaefer, J. W. Coburn, H. F. DeLuca, D. Fraser, H. G. Grigoleit, D. von Herrath, [eds.], Walter de Gruyter, Berlin, New York, 459 (1977). Parkes, C. O., Reynolds, J . J . , Moz. Cell. Endocrinol., 7, 25 (1977). Rucki, R. J., Hoffmann-La Roche, Inc. Personal Communication.
Analytical Profiles of Drug Substances, 8
CHLORTETRACYCLINE HYDROCHLORIDE George Schwartzman I ;Lola Wayland, Thomas Alexander Kenneth Furnkranz, George Selzer, and the USASRG * I.
Description I . I Drug Properties I .2 Physical Description and Optical Crystallography 1.3 Chemical Properties 1.4 Structure I .5 The FDA Chlortetracycline Standard 2. Physical Properties 2. I Thermal Properties (DTA, TGA) 2.2 X-Ray Powder Diffraction 2.3 Solubility 2.4 Acid-Base Properties 2.5 Polymorphism3. Spectral Properties (Optical) 3.1 Ultraviolet 3.2-Infrared 3.3 Spectropolarimetry 3.4 Fluorescence 4. Spectral Properties (Other) 4. I Proton NMR 4.2 ' T - N M R 4.3 Mass Spectrometry 5 . Chromatography 5 . I Paper and Thin-Layer 5.2 Gas-Liquid 6. Manufacture 6. I Fermentation 6.2 Isolation 7. Stability 8. Analytical Methods 8. I Microbiological 8.2 Chemical 9. References *The US.Antibiotics Standards Research Group (USASRG) is an ad hor collaboration of antibiotics researchers at the U S . Food and Drug Administration. Contributors to this monograph from the Bureau of Drugs include: T. Alexander. R. Barron, V. Folen. K. Furnkranz. G . Mack (Baltimore District), M. Maientbal. G. Mazzola (Bureau of Foods). G . Schwartzman. G. Selzer. E. Sheinin. J. Taylor, L.Wayland. and J. Weber. The USASRG was formed at the request of P. Weiss. National Center for Antibiotics Analysis. Individual contributions are referenced where possible. 'Retired. Copyright @ 1979 by Academic Press, Inc. All rights of reproduction in any form reserved. 101 ISBN 0-12-260808-9
GEORGE SCHWARTZMAN ET A L .
I02
1.
DESCRIPTION
1.1 Drug P r o p e r t i e s C h l o r t e t r a c y c l i n e h y d r o c h l o r i d e (CTC-HCL) i s the h y d r o c h l o r i d e s a l t of a n a n t i b i o t i c s u b s t a n c e produced by t h e growth of Streptomyces a u r e o f a c i e n s (Fam. Streptomycetaceae) I t was d i s c o v e r e d i n 1948 by Duggar (1).
.
CTC-HC1 is a broad-spectrum a n t i b i o t i c and a n t i protozoan a c t i v e a g a i n s t many Gram-positive b a c t e r i a , some Gram-negative b a c t e r i a , s p i r o c h e t e s , amebae, and c e r t a i n l a r g e v i r u s e s . S t a p h y l o c o c c i have become g e n e r a l l y r e s i s t a n t to t h e drug, and d r u g - r e s i s t a n t s t r a i n s may b e found among o t h e r b a c t e r i a l genera and s p e c i e s g e n e r a l l y s e n s i t i v e t o i t . C r o s s - r e s i s t a n c e t o o t h e r a n t i b i o t i c s of t h e t e t r a c y c l i n e family is a u t o m a t i c ( 2 ) . Organisms may be c o n s i d e r e d s u s c e p t i b l e i f t h e Minimum I n h i b i t o r y Concentration (MIC) is n o t more t h a n 4.0 pg/ml and i n t e r m e d i a t e i f t h e M I C is 4.0-12.5 pg/ml ( s e e Table 1). T e t r a c y c l i n e s are r e a d i l y absorbed and are bound t o plasma p r o t e i n s i n v a r y i n g d e g r e e s . They a r e c o n c e n t r a t e d by t h e l i v e r i n t h e b i l e and e x c r e t e d i n t h e u r i n e and f e c e s a t high c o n c e n t r a t i o n s and i n a b i o l o g i c a l l y a c t i v e form. The mode of a c t i o n a g a i n s t microorganisms i n v o l v e s t h e i n h i b i t i o n of phosphorylation p r o c e s s e s i n b a c t e r i a l c e l l s ( 3 ) . TABLE 1 (5) Antimicrobial Spectrum of Chlortetracycline Minimum Inhibitory Microorganism Concentration (Vg/ml)
E.
Micrococcus pyrogenes aureus 209P Micrococcus pyrogenes v z . aureus 1248A Streptococcus pyrogenes Streptococcus Q Streptococcus faecalis Micrococcus flavus Diplococcus pneumoniae Sarcina lutea ~Bacillus subtilis Escherichia Haemophilus influenzae Klebsiella pneumoniae Neisseria catarrhalis Aerobacter aerogenes Proteus vulgaris Pseudomonas aeruginosa Salmonella schottmuelleri Salmonella typhi Shigella dysenteriae Brucella bronchiseptica Mycobacterium tuberculosis Mycobacterium friedmanii Mycobacterium smegmatis Mycobacterium s p . Candida albicans Clostridium butyricum Pasteurella multocida Vibrio percolans
0.292 0.39 0.29 0.147 0.39 0.292 0.098 0.147 0.195 1.45 0.312 0.29 0.098 1.17 4.6 25 3.12 1.17 3.12 0.292 0.147 0.122 0.073 0.58 100 0.078 0.049 0.098
CHLORTETRACYCLINE HYDROCHLORIDE
103
1.2
Physical Description and Optical Crystallography CTC-HC1 is a yellow, odorless powder composed mainly of crystals in the shape of small hexagons, and has the following optical crystallographic characteristics (4):
a: 1.635; optic sign negative; 2V = 59" (calc.);
8:
1.706; orthorhombic; extinction parallel; and
y: 1.730; symmetrical It is stable in air, but is slowly affected by light (6). 1.3
Chemical Properties CTC-HC1 is the HC1 salt of amphoteric CTC; it is multifunctional with two chromophores. It is a parachlorophenol with an aYf3-unsaturatedketone in conjugation. The second chromophore involves another a,B-unsaturated ketone that is in conjugation with an anomalously behaving amide (7). The tertiary amine is responsible for the basic character and the phenolic group is acidic. CTC is fluorescent and can be assayed polarographically (8). A particularly intriguing aspect of the chemistry of the compounds of the tetracycline family is their ability to form metallic complexes. CTC shares in this intensively studied capability, which is very likely related to the therapeutic activity (9). This property is also used in the purification (10) and analysis (11) of CTC.
1.4
Structure C22H23ClN208.HCl Empirical Formula 515.35 Molecular Weight
7-Chloro-4-(dirnethylamino)-1,4,4a,5,5a,6,11,12aoctahydro-3,6,10,12,12a-pentahydroxy-6-methyl-l,ll-dioxo-2naphthacenecarboxamide monohydrochloride (CAS-64-72-2) (6,12-14) (Figure 1).
1.5
The FDA Chlortetracycline Standard The current official FDA Chlortetracycline Working Standard is chlortetracycline hydrochloride, Lot W501-632B95-1 (9/29/53), obtained from Lederle, which markets the antibiotic under the proprietary name Aureomycin. The current working standard has an assigned potency of 1000 pg/mg (the term pg applied to chlortetracycline means the chlortetracycline activity (potency) contained in l u g of the FDA Chlortetracycline Master Standard (Lot #990-107-141-1),which is also chlortetracycline hydrochloride).
I05
CHLORTETRACYCLINE HYDROCHLORIDE
The Working S t a n d a r d is s t o r e d i n l o t s of 250 mg a t -2O"C, p r o t e c t e d from l i g h t and m o i s t u r e , a t t h e h a t i o n a l C e n t e r f o r A n t i b i o t i c s A n a l y s i s , Washington, DC.
2.
PHYSICAL PROPERTIES 2.1 Thermal P r o p e r t i e s D i f f e r e n t i a l Thermal A n a l y s i s (DTA) and Thermal G r a v i m e t r i c A n a l y s i s (TGA).CTC-HC1 i s s t a b l e u n t i l i t b e g i n s t o decompose e x o t h e r m i c a l l y a t a p p r o x i m a t e l y 230°C ( F i g u r e s 2 and 3 ) ( 1 5 ) . The compound d o e s n o t l o s e any m a s s u n t i l t h e f i n a l d e c o m p o s i t i o n t a k e s p l a c e . No polymorphs have b e e n s e e n i n t h e samples examined. 2.2
X-Ray Powder D i f f r a c t i o n The X-ray d i f f r a c t i o n p a t t e r n of t h e FDA Working S t a n d a r d h a s been d e t e r m i n e d . It d e m o n s t r a t e s c r y s t a l l i n e s t r u c t u r e ; t h e d a t a are l i s t e d i n T a b l e 2 ( 1 6 ) . TABLE 2 X-Ray D i f f r a c t i o n Data
(1)
1/11
9.10 8.48 (7.75a D(7.43 6.65 6.38 (5.72 D(5.61 5.28 5.16 D(4.96 (4.88 4.68 4.54 4.42 4.29 4.24 (4.15 D(4.09 3.88 3.80 3.71 3.64 3.57 3.52 3.37
11 12 56 44 13 43 81 42 61 8 8 15 3 40 100 70 25 52 78 37 31 59 33 16 25 23
d
3
=
Doublet.
d (i) 3.34 3.27 3.23 (3.17 D(3.12 3.095 2.982 2.948 2.910 (2.878 D(2.854 2.788 2.710 D ( 2 . 653 (2.632 2.560 2.482 2.440 2.421 2.390 2.343 2.290 2.235 2.210 2.170 2.142 2.093
1/11
17 37 16 73 74 38 8 9 47 25 31 35 36 14 10 30 22 13 27 12 24 7 14 37 13 23 21
d 2.060B D(1.985 (1.962 1.897 1.880 1.868 1.856 1.827 1.805 1.784 ~(1.748 (1.737 1.705 1.682 1.638 1.631 1.608 1.595 1.583
1/11
13 11 13 12 10 13 13 8 9 6 8 11 9 6 5 4 5 4 4
GEORGE SCHWARTZMAN ET AL.
106
120'
140"
Figure 2.
120°
Figure 3.
160'
180" 200'
220'
240"
Differential thermogram of CTC-HC1.
160'
200"
240°
Thermal gravimetric analysis curve of CTC-HC1.
CHLORTETRACYCLINE HYDROCHLORIDE
I07
2.3
Solubility The s o l u b i l i t y of a n t i b i o t i c s , i n c l u d i n g CTC-HC1, w a s r e p o r t e d by Andrew and Weiss (17). CTC-HC1 i s a n amphoteric s u b s t a n c e and consequently i t is solu'ble i n aqueous a c i d and b a s e . However, i t can r a p i d l y degrade i n t h e s e s o l v e n t s . Its s o l u b i l i t y i n w a t e r is about 8 mg/ml and i n methanol about 1 7 mg/ml. I n h i g h e r m o l e c u l a r weight a l c o h o l s , t h e s o l u b i l i t y of CTC-HC1 i s c o n s i d e r a b l y le ss t h a n i n methanol. For p r a c t i c a l purposes, i t i s i n s o l u b l e i n many common s o l v e n t s such a s t h e a l i p h a t i c hydrocarbons, benzene, I t i s r e a d i l y s o l u b l e i n p y r i d i n e and e t h e r , and chloroform. t o t h e e x t e n t of about 5 mg/ml i n formamide. P y r i d i n e is an u n d e s i r a b l e s o l v e n t because of i t s b a s i c i t y , and formamide i s n o t d e s i r a b l e because of t h e d i f f i c u l t y i n o b t a i n i n g and maintaining i t a s a s t a b l e solvent.
2.4
Acid-Base P r o p e r t i e s
CTC e x h i b i t s t h r e e a c i d i c d i s s o c i a t i o n c o n s t a n t s when t i t r a t e d i n aqueous s o l u t i o n s ( 1 8 ) . Stephens e t a l . (19)
i d e n t i f i e d t h e t h r e e a c i d i c groups ( F i g u r e 4 ) , and r e p o r t e d thermodynamic pKa v a l u e s of 3.30, 7 . 4 4 , and 9.27. Leeson e t a l . (20) a s s i g n e d pKa v a l u e s t o t h e f o l l o w i n g a c i d i c groups:
pKa
Assignment
3.30
Tricarbonylmethane System (A)
7.44
P h e n o l i c Diketone System (B)
9.27
Dimethylamino System (C)
Kalnins and B e l e n ' s k i i (21) v e r i f i e d t h e assignments by i n f r a r e d (IR) spectroscopy. The pH o f a 10 mg/ml aqueous s o l u t i o n , as d e s c r i bed i n t h e Code of F e d e r a l R e g u l a t i o n s monograph f o r CTC-HC1 (22) should l i e between 2.3 and 3.3. 2.5
Polymorphism I n r e c e n t y e a r s , w i t h growing concern about t h e r e l a t i v e b i o a v a i l a b i l i t i e s of d i f f e r e n t samples of t h e same drug s u b s t a n c e , polymorphism h a s become of p r i m e i n t e r e s t . Miyazaki and co-workers (23) have r e p o r t e d t h e e x i s t e n c e of The X-ray powder d i f f r a c two c r y s t a l l i n e forms of CTC-HC1. t i o n p a t t e r n s , I R s p e c t r a , d i s s o l u t i o n b e h a v i o r s , and h y g r o s c o p i c i t i e s t h a t t h e y r e p o r t e d were d i s t i n c t l y d i f f e r e n t and t h e r e w e r e d i s c r e p a n c i e s i n t h e b i o a v a i l a b i l i t i e s . I n l a t e r work on two forms of CTC b a s e p r e p a r e d by c r y s t a l l i z i n g from water o r methanol, t h e X-ray p a t t e r n s and
CHLORTETRACYCLINE HYDROCHLORIDE
I09
water c o n t e n t s were d i f f e r e n t , b u t o t h e r p h y s i c a l p r o p e r t i e s were i n d i s t i n g u i s h a b l e . T h e r e a p p e a r e d t o be no d i f f e r e n c e i n b i o a v a i l a b i l i t y ( 2 4 ) . No polymorphs were found i n t h e FDA CTC s t a n d a r d . 3.
SPECTRAL PROPERTIES (OPTICAL) 3.1 Ultraviolet Medium
Maxima (nm)
0 . 1 N HC1 0 . 1 N NaOH Methanol
368, 340sh, 322sh, 265, 229 345, 283, 253, 222 372, 342sh, 322sh, 2 6 2 s h , 253, 233
See F i g u r e 5 ( 2 5 ) . 3.2
Infrared The I R a b s o r p t i o n s p e c t r a of CTC-HC1 a r e shown i n F i g u r e s 6 and 7 . S p e c t r a were r u n on a Perkin-Elmer Model 467 g r a t i n g s p e c t r o p h o t o m e t e r as a K C 1 p e l l e t ( 1 mg/200 mg K C I ) , The s p e c t r a are e s s e n and as a N u j o l m u l l ( 2 0 mg/3 d r o p s ) . t i a l l y i d e n t i c a l . The CTC-HC1 s p e c t r u m may a l s o b e f o u n d i n a c o m p i l a t i o n of I R s p e c t r a of Drug R e f e r e n c e S t a n d a r d s by Hayden e t a l . ( 2 6 ) . Major a b s o r p t i o n f r e q u e n c i e s h a v e b e e n compiled (27) and a s s i g n m e n t s h a v e b e e n made on inany of t h e bands(28-31). Some of t h e m a j o r f r e q u e n c i e s and band a s s i g n ments are:
&
x
3360
2.98
vNH of NH2 (asym.)
3315
3.02
vNH of NH2 (sym.)
3200-3450
2.90-3.12
vOH ( a l c o h o l i c , masks NH)
2800-2400
3.57-4.17
t e r t i a r y amine h a l i d e s a l t , g r o u p of b r o a d bands
1675
5.97
vc-0
1582
6.32
6NH2
1450
6.90
6CH ( b e n d i n g of CH3)
1368
7.31
VCN
1042
9.60
OH ( d e f o r m a t i o n , a l c o h o l s )
GEORGE SCHU ,RTZMAN ET AL.
110
a
b
m v)
0 XI 00
B
2 0
m
0
Figure 5 .
WAVELENGTH (nm) Ultraviolet absorption spectra of CTC-HC1 i n a , 0.1N HC1; b , 0.1N NaOH; and c , methanol.
a,
c, rl rl
a
-ai V
rl
v)
M
(d
W 0
t
B 2 a
8
I800 1600 1400 WAVELENGTH (CM")
Figure 7.
1200
Infrared absorption spectrum of CTC-HC1 a s Nujol mull.
100
CHLORTETRACYCLINE HYDROCHLORIDE
113
3.3
Spectropolarimetry Because c o n f i g u r a t i o n a l i n f o r m a t i o n can be d e r i v e d from o p t i c a l r o t a t o r y d i s p e r s i o n and c i r c u l a r d i c h r o i s m s c a n s , c o n s i d e r a b l e work h a s been conducted u s i n g t h e s e t e c h n i q u e s t o s t u d y t h e t e t r a c y c l i n e s ( 3 2 ) . The a b s o l u t e c o n f i g u r a t i o n of CTC w a s determined u s i n g o p t i c a l r o t a t o r y d i s p e r s i o n d a t a (33) S p e c t r a l c u r v e s are p r e s e n t e d i n F i g u r e s 8 and 9. The c i r c u l a r d i c h r o i s m spectrum is similar t o t h a t p r e s e n t e d by Mitscher e t a l . ( 3 4 ) , e x c e p t t h a t t h e v a l u e s d i f f e r by a f a c t o r of about 1.5. I n Table 3, d a t a o b t a i n e d by M i t s c h e r and i n FDA l a b o r a t o r i e s are compared.
3.4
Fluorescence The CTC-HC1 FDA Working Standard g i v e s a y e l l o w f l u o r e s c e n c e under 1or.pwave u l t r a v i o l e t (W) l i g h t (375 m) (35). The e x c i t a t i o n (324 and 357 nm) and emission (443 nm) s p e c t r a of t h i s s t a n d a r d d i s s o l v e d i n 0.05N NaOH (11.4 mg/50 ml) a r e p r e s e n t e d i n F i g u r e 10.
TABLE 3 Molecular E l l i p t i c i t i e s of CTC Wavelength (nm) M i t s c h e r ' s Valuea FDA Value (X 103) (X 103) 236 254 288 318 355 ( s h )
+10 -31 +4 8 -24
+2 3 -48 +88 -32 -12
-14 aThese v a l u e s w e r e o b t a i n e d from t h e g r a p h i n R e f e r e n c e
4.
Ratio
0.43 0.64 0.54 0.73 1.09 34
.
SPECTRAL PROPERTIES (OTHER) P r o t o n NMR The 60 MHz NMR s p e c t r a of CTC-HC1 i n DMSO-d6 and i n methanol-d4 are shown i n F i g u r e s 11 and 1 2 , r e s p e c t i v e l y . The s h a r p s i g n a l s due t o t h e methyl groups are r e a d i l y a s s i g n a b l e ; t h e i r chemical s h i f t s and i n t e n s i t i e s are c o n s i s t e n t w i t h t h e s t r u c t u r e . The 2 methylene p r o t o n s a t C-5 are n o t e q u i v a l e n t and g i v e two sets of m u l t i p l e t s . Only one m u l t i p l e t is a s s i g n a b l e i n t h e methanol spectrum: t h e s i g n a l c e n t e r e d a t 2.20 ppm. I n DMSO-db t h e s e p r o t o n s appear between 1 . 5 and 2 . 3 ppm. The o n l y methine p r o t o n a c t u a l l y a s s i g n e d i s t h e one a t C-4. The c l o s e p r o x i m i t y t o t h e p o s i t i v e l y charged N c a u s e s a downfield s h i f t away from t h e o t h e r s i g n a l s . When D20 i s added t o t h e DMSO-db s o l u t i o n , t h e H-4 s i g n a l remains c o n s t a n t However, t h e two amide p r o t o n s , o r i g i n a l l y a t 9.15 and 9.55 ppm, exchange w i t h t h e deuterium and a r e no l o n g e r observed. These s i g n a l s were n o t observed i n methanol-d4, a g a i n , due t o
4.1
~-
NOIWMSIO W O l V l O Y lWl1dO
I I4
<
115
AlISN3lNI
I I6
I I7
d
I
u X
V I3 u
5
k
a,
CI V
8
c
2
b
0
w
b
CHLORTETRACYCLINE HYDROCHLORIDE
119
deuterium exchange. Data from t h e l i t e r a t u r e ( 3 6 ) , based on a spectrum o b t a i n e d i n DMSO-db, a r e i n c l u d e d i n T a b l e 4. As c a n be s e e n from t h e t a b l e , t h e s e v a l u e s are g e n e r a l l y u p f i e l d from o u r r e s u l t s . Although t h e s e d i f f e r e n c e s were unexpected, no e x p l a n a t i o n w i l l be a t t e m p t e d h e r e (37). TABLE 4 Chemical S h i f tsa Proton
L i t e r a t u r e (36) 1.7
DMSO-dh
1.88 ( s )
2.7
Solvent Methanol-dq 1.98 ( s )
2.93 ( s )
3.05 ( s )
6.4
-
7.0
7.58 (d)
7.55 ( d )
6.4
- 7.0
6.98 ( d )
6.93 ( d )
4.36 ( b r . s )
4.10 ( d )
4.0
1.7
-
2.1
8.4, 8 . 9
1.5
-
2 . 3 (m,s)
2.20 (m)b
9.15, 9.55
n o t observedC
2.7
not assignedd
not assignedd
2.7
not assignedd
n o t assignedd a S p e c t r a were o b t a i n e d on a Perkin-Elmer R-12B equipped w i t h a N i c o l e t TT-7 F o u r i e r t r a n s f o r m a c c e s s o r y . Chemical s h i f t s are r e p o r t e d i n ppm downfield from i n t e r n a l TMS. M u l t i p l i c i t i e s a r e i n d i c a t e d as s = s i n g l e t , d = d o u b l e t , and m = m u l t i p l e t . bThis m u l t i p l e t r e p r e s e n t s one of t h e H-5 p r o t o n s . The chemical s h i f t of t h e o t h e r one w a s n o t a s s i g n e d . CThese p r o t o n s exchange w i t h t h e deuterium of t h e s o l v e n t and t h u s are n o t observed. dThe chemical s h i f t s of t h e s e p r o t o n s are n o t a s s i g n e d . They a r e obscured by t h e -N(CH3)2 a n d / o r t h e s o l v e n t .
4.2
I3C NMR
Proton-noise decoupled and s i n g l e - f r e q u e n c y o f f resonance decoupled carbon-13 NMR s p e c t r a were determined f o r t h e CTC Working Standard ( F i g u r e 1 3 ) . The observed chemical s h i f t s of t h e 22 carbon atoms compare c l o s e l y w i t h t h o s e r e p o r t e d by Frank (38). The o n l y s i g n i f i c a n t d i f f e r e n c e observed w a s t h a t of t h e dimethylamino carbons which were found a t 48.5 ppm r a t h e r t h a n a t F r a n k ' s r e p o r t e d v a l u e of 4 1 ppm. This d i f f e r e n c e i n chemical s h i f t s can probably be a s c r i b e d t o d i f f e r i n g amounts of w a t e r p r e s e n t i n t h e DMSO-db s o l v e n t s and hence i n t h e pH of t h e s e r e s p e c tive solutions.
t
V
rl
T
V H V 0
Ict
5
k V a,
4J
4 !z 8 V m
4
m rl
a, k
3
m h
-4
CHLORTETRACYCLINE HYDROCHLORIDE
121
S p e c t r a were d e t e r m i n e d u s i n g a p u l s e w i d t h of 4 p s e c o n d s , which c o r r e s p o n d s t o a f l i p a n g l e of 18" and a 1 second p u l s e d e l a y t i m e . The 4000 Hz spectrum w a s d e s c r i b e d u s i n g 8192 d a t a p o i n t s . The o b s e r v e d r e s o n a n c e l i n e s of CTC-HC1 t h e i r a s s i g n m e n t s are shown i n T a b l e 5 .
(39) and
'CABLE 5 Observed Resonance L i n e s o f CTC-HC1 and T h e i r Assignments Carbon Assignment Chemical S h i f ta CcH3
C-4a C-5a N (CH-3)2 c-4 C-6 C-12a c- 2 C-lla C-lOa c-9 c-7 C-8 C-6a c-10 corn2 c-12 c- 3
c-1 c-11
25.1 27.0 34.9 42.0 48.5 68.3 70.4 73.3 95.5 106.1 117.0 118.9 121.3 139.7 143.6 160.8 172.0 175.3 187.1 192.1 193.3
DMSO-d6, p a r t s p e r m i l l i o n from TMS (0.00 ppm). quadruplet, t = t r i p l e t , d = doublet.
q t d d q d
d d
q =
Mass S p e c t r o m e t r y Mass s p e c t r a l s t u d i e s , i n c l u d i n g low v o l t a g e t e c h n i ques and a c c u r a t e m a s s measurements, have been r e p o r t e d by Hoffman (40) on t e t r a c y c l i n e and e i g h t r e l a t e d compounds. A s a r e s u l t of good s p e c t r a l c o r r e l a t i o n s among t h e s e compounds, t h e m a j o r f r a g m e n t a t i o n p r o c e s s e s are d i s c u s s e d i n terms of two compounds i n t h e series: 50,,6-anhydrotetracycline and dedimethylaminotetracycline, w i t h o n l y a s e l e c t e d number of i o n s r e p o r t e d f o r CTC. F u r t h e r s t u d i e s on t h e s e a n t i b i o t i c s , i n c l u d i n g CTC, w e r e conducted by M o r r i s and C a i r n s ( 4 1 ) . However, l i t t l e i n f o r m a t i o n on t h e i r r e s u l t s is i n c l u d e d i n t h e extended a b s t r a c t of t h e m e e t i n g , and a f u l l r e p o r t h a s n o t 4.3
122
GEORGE SCHWARTZMAN ET A L .
been p u b l i s h e d . P e r s o n a l communications w i t h t h e a u t h o r s i n d i c a t e t h a t t h e r e s u l t s of t h e i r work a r e i n c l o s e agreement with d a t a reported here. The f r a g m e n t a t i o n p a t t e r n of CTC can be d i s c u s s e d i n terms of t h r e e d i f f e r e n t mechanisms. These are: a. P r o c e s s e s r e s u l t i n g from t h e c a p a c i t y of t h e dimethylamino group t o d i r e c t l o s s e s of small fragments t o g e t h e r w i t h i t s a b i l i t y t o r e t a i n and s t a b i l i z e t h e p o s i t i v e charge. b. Fragmentation of t h e D r i n g system w i t h c h a r g e r e t e n t i o n on t h e f u s e d r i n g p o r t i o n of t h e molecule. c. Fragmentation of t h e D r i n g system w i t h c h a r g e r e t e n t i o n elsewhere t h a n on t h e f u s e d r i n g moiety. The mass spectrum of CTC, shown i n F i g u r e 1 4 ( 4 2 ) , is c h a r a c t e r i z e d by a r e a s o n a b l y i n t e n s e r ; o l e c u l a r i o n a t m / e 4 7 8 w i t h t h e concomitant i s o t o p e peak a t P+2 r e p r e s e n t i n g one c h l o r i n e atom i n t h e r i n g system. Although i t h a s been suggested t h a t t h i s c h l o r i n e atom b e employed as a t r a c e r v i a t h e 3 7 ~ 1i s o t o p e r a t i o f o r d e t e c t i o n of s p e c i e s c o n t a i n i n g t h e A r i n g and a d j u n c t r i n g systems, many of t h e s e i o n s are of such low r e l a t i v e i n t e n s i t y t h a t t h i s would have o n l y l i m i t e d u s e f u l n e s s toward t h a t end, e x c e p t perhaps a t h i g h e r mass values. The dominance of t h e f r a g m e n t a t i o n p r o c e s s e s by t h e p r e s e n c e of t h e 4-dimethylamino group i v e s r i s e t o t h e i n t e n s e i o n s a t m / e 4 4 , m / e 58 (CH3)2-i=CH2, m / e 7 1 (CH3)2ftCH=CH2, and m / e 84 (CH3)2-$=CH-CH=CH2. The i o n a t m / e 98 (C+8NO+) a p p e a r s t o i n v o l v e a c y c l i z a t i o n of t h e dimethylamino group w i t h e l e m e n t s of t h e D r i n g . Of p a r t i c u l a r n o t e i s t h e l o s s of 43 atomic mass u n i t s from t h e m o l e c u l a r i o n t o g i v e t h e i n t e n s e i o n a t m / e 435 and from t h e i o n a t m / e 443 t o y i e l d m / e 400 ( F i g u r e 1 5 ) . The p r e s e n c e of t h e amide f u n c t i o n a l group i s i n d i c a t e d by o b s e r v a t i o n s of s u c c e s s i v e l o s s e s of NH3 and OH ( a s w a t e r ) from t h e m o l e c u l a r i o n t o y i e l d u l t i m a t e l y t h e i o n a t m / e 443. The l o s s of water a t m/e 460 a p p e a r s t o be s l i g h t l y f a v o r e d over t h e competing l o s s of NH3 a t m / e 462 from t h e abundances of t h e r e s p e c t i v e i o n s . Fragmentation of t h e D r i n g can p r o v i d e t h e d u a l purpose of d e t e r m i n i n g t h e s u b s t i t u e n t a t t h e 4 p o s i t i o n (dimethylamino i n t h e case of CTC) a n d / o r h e l p t o l o c a t e f u n c t i o n a l i t i e s e l s e w h e r e i n t h e r i n g system. This,however, r e q u i r e s a d e t a i l e d examination of a n a l o g s such a s i n t h e work of Hoffman ( 4 0 ) . The i o n a t m / e 365 w i l l l o c a t e t h e s u b s t i t u e n t s a t t h e 2 and 3 p o s i t i o n s of t h e D r i n g by d e t e r m i n a t i o n of t h e mass of t h e l o s t s u b s t i t u e n t and a l s o g i v e e v i d e n c e c o n c e r n i n g t h e e x t e n t of s u b s t i t u t i o n on t h e A , B, and C r i n g s . T h i s
SPEC.
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2 0 0 3 9 LS CHLORTETRRCYCLINE HCL
NO. 44
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z
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-
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170
MASS T O CHRRCE RRIIO
Figure 14. Electron impact mass spectrum of CTC-HC1. Instrument: Varian MAT 311; source temperature sufficient to produce vaporization. (Chemical ionization using ammonia as reagent gas gave MH+ as base peak. 1
GEORGE SCHWARTZMAN ET A L .
I24
365 435
461
460
400 I
I70
275 -
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370
Figure 15.
Major fragmentation pathways of CTC involving molecular ion and other significant high mass ions. Underlined m/e values indicate confirmation by accurate mass measurements.
CHLORTETRACYCLINE HYDROCHLORIDE
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knowledge p l u s t h e observed s h i f t of t h e i o n a t m / e 170 s h o u l d s u f f i c e t o a l l o w p o s t u l a t i o n of t h e s u b s t i t u t i o n ( F i g u r e 1 6 ) . 5.
CHROMATOGRAPHY 5.1 Paper and Thin Layer Some of t h e e a r l y r e p o r t s on t h e chromatography of t h e t e t r a c y c l i n e a n t i b i o t i c s p r i o r t o 1957 are of l i m i t e d v a l u e . Fischbach and Levine (43) d e s c r i b e d a c o n t i n u o u s ascending t e c h n i q u e and B e r t i and C i m a (44) r e p o r t e d an ascending method u s i n g aqueous sodium a r s e n i t e as t h e mobile s o l v e n t . Other a u t h o r s (45,46) r e p o r t e d descending t e c h n i q u e s and b i o a u t o g r a p h i c means f o r l o c a t i n g t h e zones of a c t i v i t y . A l l of t h e s e methods f a i l t o show t h e p r e s e n c e of t h e e p i m e r i c form of t h e t e t r a c y c l i n e s and i n most i n s t a n c e s s t r e a k i n g of t h e s p o t s i s a problem. A b a s i c improvement i n t h e paper chromatography of t h e s e a n t i b i o t i c s w a s a c h i e v e d by S e l z e r and Wright (47) and K e l l y and Bryske ( 4 8 ) when t h e y r e p o r t e d methods f o r t h e p r e t r e a t m e n t of t h e paper w i t h comp l e x i n g a g e n t s t o bind t h e m e t a l l i c i o n s which may be p r e s e n t . The t e t r a c y c l i n e s are w e l l known f o r t h e i r a b i l i t y t o form complexes w i t h p o l y v a l e n t c a t i o n s . T h i s p r o p e r t y changes t h e i r s o l u b i l i t y c h a r a c t e r i s t i c s i n t h e m o b i l e s o l v e n t s and o f t e n r e s u l t s i n troublesome s t r e a k i n g . To overcome t h i s d i f f i c u l t y , S e l z e r and Wright used paper dipped i n M c I l v a i n e ' s b u f f e r (pH 3.5) which c o n t a i n s c i t r a t e i o n s c a p a b l e of b i n d i n g t h e metallic i o n s . The chromatograms were developed w i t h a m i x t u r e of n i t r o m e t h a n e , chloroform, and p y r i d i n e (20:10:3) on paper s t i l l damp from t h e t r e a t m e n t w i t h the buffer solution. For t h e same purpose, K e l l y and Bryske used p a p e r impregnated w i t h 0.1N disodium ethylenediaminetetraacetate (EDTA) and two mobile s o l v e n t s : t h e o r g a n i c phase from a m i x t u r e of E-butanol, ammonia, water (4:1:5) and t h e o r g a n i c phase from a m i x t u r e of g - b u t a n o l , a c e t i c a c i d , water ( 4 : l : 5 ) . Disodium EDTA (0.1N) works as w e l l as M c I l v a i n e ' s b u f f e r when i t is used t o t r e a t t h e paper i n t h e method of Walton e t a l . ( 4 9 ) . A c i r c u l a r paper chromatographic method a l s o u s i n g paper dampened w i t h M c I l v a i n e ' s b u f f e r (pH 4.5) w a s r e p o r t e d by Urx e t a l . ( 5 0 ) . They used a m i x t u r e of chloroform and c - b u t a n o l ( 4 : l ) as t h e mobile s o l v e n t . Most of t h e methods i n which t h e paper i s t r e a t e d with a c h e l a t i n g a g e n t are c a p a b l e of showing a s e p a r a t i o n of some of t h e t e t r a c y c l i n e d r u g s from e a c h o t h e r and from t h e i r r e s p e c t i v e e p i m e r i c forms. They a r e a l s o c a p a b l e of r e v e a l i n g t h e p r e s e n c e of common d e g r a d a t i o n compounds of t h e s e d r u g s . The u s u a l method of d e t e c t i n g chromatographed t e t r a c y c l i n e a n t i b i o t i c s i n v o l v e s fuming t h e paper w i t h ammonia vapor and o b s e r v i n g t h e yellow f l u o r e s c e n c e under UV l i g h t . A s l i t t l e as 0.2-0.5 pg can b e v i s u a l i z e d by t h i s technique.
2 ; :&f (
I
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,N$ CH3 CH3
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-6
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CH, CH3
Mf Figure 16.
II
N+ / \
CH3 CH3
W e 170
Proposed structures for ions at m/e 365 and m/e 170 for use in determination of ring substituents.
CHLORTETRACYCLINE HYDROCHLORIDE
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Some of t h e f e a t u r e s t h a t are s u c c e s s f u l f o r t h e chromatography of t h e t e t r a c y c l i n e s o n paper have been adapted t o t h i n l a y e r chromatography (TLC). Complexing a g e n t s are almost always used i n t h e p r e p a r a t i o n of t h e p l a t e s a n d , i n a d d i t i o n , s e v e r a l methods f o r h y d r a t i n g t h e p l a t e s by t h e a d d i t i o n of g l y c e r i n a n d / o r p o l y e t h y l e n e g l y c o l have been reported. Several i n v e s t i g a t o r s f i n d i t d e s i r a b l e t o acidwash t h e i n o r g a n i c s u p p o r t i n o r d e r t o remove m e t a l l i c c a t i o n s . These TLC methods are much more time-consuming t h a n most of t h e paper chromatographic p r o c e d u r e s because of t h e s p e c i a l care o f t e n r e q u i r e d t o p r e p a r e and s t o r e t h e TL,C d a t e s . For t h i s r e a s o n , where a p p l i c a b l e , t h e p a p e r chromaHowever, f o r q u a n t i t a t i v e t o g r a p h i c methods .are p r e f e r a b l e . a n a l y s i s of t h e t e t r a c y c l i n e epimers and d e g r a d a t i o n p r o d u c t s , TLC i s u s u a l l y c o n s i d e r e d t o b e b e t t e r t h a n p a p e r chromatography. I n 1964, Somanini and Anker (51) d e s c r i b e d a method u s i n g K i e s e l g u h r l a y e r s impregnated w i t h a b u f f e r s o l u t i o n c o n t a i n i n g g l y c e r i n . Nishimoto e t a l . (52) r e p o r t e d t h e u s e of s i l i c a g e l l a y e r s t r e a t e d w i t h EDTA. I n 1967, Ascione e t a l . (53) p u b l i s h e d a method u s i n g l a y e r s made from acid-washed diatomaceous e a r t h . They p r e p a r e d p l a t e s c o n t a i n i n g 0.1N EDTA, g l y c e r i n , and p o l y e t h y l e n e g l y c o l 400. Other i n v e s t i g a t o r s (54,55) have d e s c r i b e d methods which are m o d i f i c a t i o n s of improvements of t h e methods p r e v i o u s l y p u b l i s h e d .
5.2
G a s and L i q u i d Chromatography I n v e s t i g a t o r s have found i t q u i t e d i f f i c u l t t o chromatograph t h e t e t r a c y c l i n e s by g a s - l i q u i d t e c h n i q u e s . Often, o n l y fragments o f t h e o r i g i n a l sample are o b t a i n e d (56). T s u j i and Robertson (57) d i d manage t o chromatograph s i l y l a t e d CTC u s i n g 3% methyl s i l i c o n e on Gas-Chrom Q and o t h e r s t a t i o n a r y phases. However, w i t h t h e a d v e n t of r e f i n e d h i g h p r e s s u r e l i q u i d chromatographic (HPLC) t e c h n i q u e s , i n t e r e s t i n g a s chromatographic methods f o r t h e t e t r a c y c l i n e s has diminished. A number of p a p e r s have appeared r e p o r t i n g t h e HPLC s e p a r a t i o n of CTC from i t s isomers a n d / o r o t h e r t e t r a c y c l i n e s . There i s n o t a consensus of o p i n i o n as t o t h e most s a t i s f a c t o r y approach; t h u s , i t a p p e a r s t h a t a t t h i s t i m e one must s t i l l v e r i f y t h e o p t i m a l system f o r a p a r t i c u l a r i n s t r u m e n t . Methods found i n t h e l i t e r a t u r e f o r CTC a r e d e s c r i b e d i n Table 6. EDTA is added t o p r e v e n t t h e f o r m a t i o n of complexes of t h e t e t r a c y c l i n e s w i t h m e t a l l i c s u r f a c e s . Other chromatographic t e c h n i q u e s t h a t have been a p p l i e d t o t h e t e t r a c y c l i n e s , i n c l u d i n g CTC, i n v o l v e low p r e s s u r e column chromatography. Ascione e t a l . (64) developed a semiautomated system whereby sample s o l u t i o n s are a u t o m a t i c a l l y i n j e c t e d o n t o a column of diatomaceous e a r t h mixed w i t h
TABLE 6 High P r e s s u r e L i q u i d Chromatography of CTC
Mobile Phase
S t a t i o n a r y Phase
20% Methanol, 80% 0.05M ammonium c a r b o n a t e , 0.02M EDTA
C8/Lichrosorb 1 0 pm, 25 c m x 3 . 2 mm
Phosphate b u f f e r i n 13% methanol, 0.85 ml/min., pH 2.5
Zipax-hydrocarbon polymer, 2 . 1 x 1000 mm
Aqueous p e r c h l o r a t e - c i t r a t e b u f f e r mixed w i t h CH3CN
Sil-X, 13 Urn, 5 x 125 mm
EDTA, N a C l i n 30% methanol, pH 9.9
Ion-X-SA,
NH3,
a n i o n exchanger
EDTA, PO4, isopropanol-water, pH 7.6, 2 ml/min.
UBondapak c18, 300 x 4 mm
EDTA, NO3, 9.6% e t h a n o l , pH 9 , 1 rnllmin.
Zipak, 1.8 x 1000 mm
Migration T i m e (min. )
Ref.
34.5
58
6
59
1.3
60
3
61
11.6
62
22
63
CHLORTETRACYCLINE HYDROCHLORIDE
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a s o l u t i o n of EDTA and p o l y e t h y l e n e g l y c o l . CTC i s e l u t e d w i t h t h e o r g a n i c phase of a m i x t u r e of chloroform, benzene, aqueous s o l u t i o n of EDTA, and p o l y e t h y l e n e g l y c o l . Ragazzi and Veronese (65) s e p a r a t e d CTC from o t h e r t e t r a c y c l i n e s by means of g e l permeation chromatography.
6.
MANUFACTURE 6.1 Fermentation A medium ( c o n t a i n i n g c o r n s t e e p l i q u o r ; c a l c i u m c a r b o n a t e : s u c r o s e ; ammonium, f e r r o u s , manganese, and z i n c s u l f a t e s ; and ammonium, c o b a l t , and magnesium c h l o r i d e s ) i s s t e r i l i z e d and d i l u t e d w i t h water t o t h e d e s i r e d c o n c e n t r a t i o n . It is i n o c u l a t e d w i t h Streptomyces a u r e o f a c i e n s , k e p t a t 27"C, and a e r a t e d and a g i t a t e d f o r %60 h o u r s , w i t h l a r d o i l added t o c o n t r o l foaming ( 6 6 ) . 6.2
Isolation The mash from t h e Streptomyces a u r e o f a c i e n s ferment a t i o n b r o t h i s a c i d i f i e d and f i l t e r e d . The f i l t r a t e i s a d j u s t e d t o t h e d e s i r e d pH, u s u a l l y 7-8.5, and v a r i o u s f l o c c u l a t i n g o r c h e l a t i n g a g e n t s may be added ( e . g . , v i n y l acetatem a l e i c a n h y d r i d e copolymer, sodium EDTA, ammonium o x a l a t e , Arquad). The p r e c i p i t a t e i s ( 1 ) s t i r r e d w i t h f i l t e r a i d , f i l t e r e d , s t i r r e d w i t h HCI., r e f i l t e r e d , mixed w i t h 2e t h o x y e t h a n o l , f i l t e r e d , washed, and t h e f i l t r a t e s are combined, a c i d i f i e d w i t h HC1, N a C l i s added, and t h e c r y s t a l s a r e c o l l e c t e d , washed w i t h 2-ethoxyethanol, water, and e t h a n o l , and d r i e d ( 6 7 ) , o r (2) e x t r a c t e d i n t o methyl i s o b u t y l k e t o n e , t h e e x t r a c t s are combined, f i l t e r e d , and a c i d i f i e d w i t h H C 1 , and t h e c r y s t a l s are c o l l e c t e d and washed w i t h w a t e r , 2-ethoxyethanol, and i s o p r o p a n o l , and vacuumd r i e d . I f t h e c r y s t a l s are g r e e n i s h , t h e y a r e t r e a t e d w i t h sodium h y d r o s u l f i t e a t pH 1 . 8 , f i l t e r e d , washed, and d r i e d as i n ( 1 ) above (68).
7.
STABILITY CTC-HC1, a s a d r y powder, i s a s t a b l e y e l l o w c r y s t a l l i n e material. The s i t u a t i o n i n aqueous s o l u t i o n , however, i s q u i t e d i f f e r e n t . I n sodium hydroxide s o l u t i o n s , CTC is c o n v e r t e d t o iso-CTC on s t a n d i n g ( 6 9 ) . The s o l u t i o n becomes c o l o r l e s s and e x h i b i t s a s t r o n g b l u e f l u o r e s c e n c e under UV l i g h t . D i l u t e s o l u t i o n s of CTC, i n pH 7.5 b u f f e r , make t h e same c o n v e r s i o n a t 100°C. I n a c i d s o l u t i o n s , CTC i s c o n v e r t e d t o anhydro-CTC ( 7 0 ) . T h i s change is g r e a t l y a c c e l e r a t e d by h e a t i n g and r e s u l t s i n a yellow p r o d u c t t h a t h a s a maximum absorbance a t 445 nm. I n a d d i t i o n , CTC undergoes r e v e r s i b l e e p i m e r i z a t i o n of t h e 4-dimethylamino group ( 7 1 ) . T h i s o c c u r s s l o w l y i n w a t e r o r methanol b u t i s h a s t e n e d i n b u f f e r s o l u t i o n s i n t h e r a n g e
GEORGE SCHWARTZMAN ET AL.
I30
of pH 2-6. The rate of e p i m e r i z a t i o n i s u n d e t e c t a b l e i n s o l u t i o n s more a c i d i c t h a n pH 2 ( 7 2 ) . The a n t i m i c r o b i a l a c t i v i t y of t h e epimer is probably z e r o . The s l i g h t a c t i v i t y found f o r t h i s material i s probably due t o t h e reemergence o f CTC under t h e t e s t c o n d i t i o n s . I n a f a s h i o n analogous t o t h a t of CTC, i t s epimer can be converted t o epianhydro-CTC i n a c i d s o l u t i o n .
8.
ANALYTICAL METHODS 8.1 Microbiological The m i c r o b i o l o g i c a l methods used f o r t h e determinat i o n of CTC potency i n body t i s s u e s and f l u i d s , b u l k p r o d u c t s , and p h a r m a c e u t i c a l f o r m u l a t i o n s can b e s e p a r a t e d i n t o two (1) a g a r d i f f u s i o n p l a t e method t e s t i n g procedures: ( c y l i n d e r - p l a t e ) and ( 2 ) t u r b i d i m e t r i c method. 1. Agar d i f f u s i o n p l a t e method ( c y l i n d e r - p l a t e ) : T h i s method is employed f o r d e t e r m i n i n g t h e potency of CTC i n human and animal p h a r m a c e u t i c a l formulat i o n s , b u l k p r o d u c t s , serum, t i s s u e s , u r i n e , d a i r y p r o d u c t s , and animal f e e d s . The c y l i n d e r - p l a t e procedure i s d e s c r i b e d by Grove and Randall (73) and t h e Code of F e d e r a l R e g u l a t i o n s (74). A d d i t i o n a l methods u s i n g t h i s a s s a y are d e s c r i b e d by K r a m e r e t a l . (75). The o f f i c i a l f i n a l a c t i o n method f o r CTC a s s a y i n animal f e e d s i s d e s c r i b e d i n t h e A s s o c i a t i o n of O f f i c i a l A n a l y t i c a l Chemists' O f f i c i a l Methods of A n a l y s i s
(76). 2.
method: T h i s method i s used i n l i e u of t h e d i f f u s i o n p l a t e method f o r human and animal p h a r m a c e u t i c a l f o r m u l a t i o n s and b u l k p r o d u c t s . The t u r b i d i m e t r i c method i s d e s c r i b e d i n t h e Code of F e d e r a l R e g u l a t i o n s (77). 8.2
T u rbidimetric -
Chemical The p h y s i c a l s t r u c t u r e o f CTC h a s provided a good s o u r c e of c h a r a c t e r i s t i c s u s e f u l f o r t h e a n a l y s i s of t b i s a n t i b i o t i c . Although t i t r i m e t r i c (78) and p o l a r o g r a p h i c (79) methods have been r e p o r t e d , t h e most u s e f u l p r o c e d u r e s have been based on t h e s p e c t r o s c o p i c p r o p e r t i e s of CTC and i t s d e r i v a t i v e s (80). I n 1949, Levine e t a l . (81) p u b l i s h e d two p r o c e d u r e s f o r t h e a s s a y of CTC. One method w a s based on t h e c o n v e r s i o n of CTC by h e a t i n g i n a c i d t o t h e more i n t e n s e l y yellow anhydro-CTC d e r i v a t i v e . The o t h e r method w a s based on measuri n g t h e b l u e f l u o r e s c e n c e of iso-CTC, which w a s p r e p a r e d by h e a t i n g CTC i n pH 7.5 phosphate b u f f e r . O t h e r s have d e s c r i b e d m o d i f i c a t i o n s of t h e s e methods f o r v a r i o u s purposes. Hiscox (82) s u g g e s t e d t h e d i r e c t spect r o p h o t o m e t r i c a s s a y of CTC i n e i t h e r a c i d o r a l k a l i n e s o l u t i o n a t v a r i o u s UV wavelengths. The p o s s i b l e c o n t a m i n a t i o n of CTC w i t h o t h e r t e t r a c y c l i n e d r u g s w a s a d d r e s s e d by C h i c e a r e l l i e t
CHLORTETRACYCLINE HYDROCHLORIDE
131
a l . ( 8 3 ) . They c o r r e c t e d f o r t h e p o s s i b l e p r e s e n c e of t e t r a c y c l i n e i n CTC u s i n g t h e f a c t t h a t t h e former i s unchanged i n d i l u t e a l k a l i w h i l e CTC is converted t o t h e c o l o r l e s s isoCTC The t e t r a c y c l i n e which may be p r e s e n t i s t h e n converted t o a n anhydro d e r i v a t i v e by h e a t i n g i n a c i d and i s measured s p e c t r o p h o t o m e t r i c a l l y . Feldman e t a l . ( 8 4 ) developed t h e a l k a l i n e d e g r a d a t i o n method t o measure CTC i n f e r m e n t a t i o n mash and Spock and Katz (85) used t h i s method t o determine CTC i n animal f e e d premixes. The n a t u r a l f l u o r e s c e n c e of CTC and i t s d e r i v a t i v e s has been used e x t e n s i v e l y t o determine s m a l l amounts of CTC i n b i o l o g i c a l m a t e r i a l s . Kohn (86) showed t h a t t h e f l u o r e s c e n t complex formed by CTC w i t h calcium i o n s and b a r b i t a l could be e x t r a c t e d from animal t i s s u e s i n t o an o r g a n i c s o l v e n t and t h e n measured spectrofluorometrically. The i n t e n s e f l u o r e s c e n c e of anhydro-CTC was used by Hayes and DuBuy (87) t o determine CTC i n animal t i s s u e s , t i s s u e c u l t u r e c e l l s , and b a c t e r i a . P o i g e r and S c h l a t t e r (88) e x t r a c t e d CTC from biol o g i c a l material i n t o e t h y l acetate as t h e CTC-calcium t r i c h l o r o a c e t a t e i o n p a i r . The f l u o r e s c e n c e of t h e a n t i b i o t i c w a s t h e n enhanced by t h e a d d i t i o n of magnesium i o n s and a base.
.
GEORGE SCHWARTZMAN ET
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AL.
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Analytical Profiles of Drug Substances, 8
DOBUTAMINE HYDROCHLORIDE RaJk H . Bishara and Harlan B. Long I.
2.
3. 4. 5.
6.
7.
Description I . I Nomenclature I . I . 1 Chemical Name I . I .2 Nonproprietary Name I . I . 3 Proprietary Name 1.2 Formula I .2.1 Empirical 1.2.2 Structural I . 3 Molecular Weight I .4 Appearance, Color, Odor, and Taste Physical Properties 2. I Melting Range 2.2 Simple Solubility Profile 2.3 pHRange 2.4 Dissociation Constant (pKa) 2.5 Thermal Analyses 2.5. I Differential Thermal Analysis 2.5.2 Thermogravimetric Analysis 2.6 Crystallinity 2.6. I Crystalline Habit 2.6.2 X-Ray Powder Diffraction 2.7 Ultraviolet Spectrum 2.8 Infrared Spectrum 2.9 Nuclear Magnetic Resonance Spectrum 2.10 Mass Spectrum Synthesis Stability-Degradation Absorption, Metabolism, and Excretion 5.1 In Dog 5.2 In Man Methods of Analysis 6. I Elemental Analysis 6.2 Chloride Identity 6.3 Nonaqueous Titration 6.4 Chloride Determination 6.5 Chromatography 6.5.I Thin-Layer Chromatography 6.5.2 Gas Chromatography 6.5.3 High Performance Liquid Chromatography Analysis of Biological Samples 7. I Enzymatic Assay 7.2 Chromatographic Assays 7.2.1 Thin-Layer Chromatography 7.2.2 Gas Chromatography 7.2.3 High Performance Liquid Chromatography 7.3 Mass Spectrometry (GUMS) 139
Copyright 0 1979 by Academic Press, Inc. All rights of reproduction in any form reserved. ISBN 0-12-260808-9
RAFIK H. BISHARA AND HARLAN B. LONG
140
8. Analysis of Pharmaceutical Formulations 8. I Chromatographic Assays 8. I . 1 Thin-Layer Chromatography 8.1.2 Gas Chromatography 8.1.3 High Performance Liquid Chromatography 8.2 Spectrophotometric (UV) 9. Acknowledgments 11. References
1. Description 1.1 Nomenclature 1.1.1 Chemical Name (f)-4-[2-[ [3-(4-Hydroxyphenyl)-lmethylpropyl]amino]ethyl]-1,2-benzenediol, hydrochloride 1.1.2 NonDrowietarv Name Dobutamine hydrochloride 1.1.3 Proprietary Name
DOBUTREF 1.2 Formula 1.2.1 Empirical C, 8H23N03 * HC 1 1.2.2 Structural
HO
CH3
HO&)CH2-CH2-NH-LH-CH
2 C H 2 0 0 H HCI
DOBUTAMINE HYDROCHLORIDE
141
1 . 3 M o l e c u l a r Weight 337.85 1 . 4 Appearance, C o l o r , Odor, and Taste White t o o f f - w h i t e , s l i g h t l y b i t t e r taste.
o d o r l e s s powder w i t h a
2. P h y s i c a l P r o p e r t i e s 2 . 1 M e l t i n g Range 189
-
191°C
2 . 2 Simple S o l u b i l i t y P r o f i l e The sample is s o n i c a t e d f o r one m i n u t e a t ambient t e m p e r a t u r e . Solvent
Water pH 1 . 2 (USP X I X ) pH 4 . 5 (USP X I X ) pH 7 . 0 (USP X I X ) Ethanol Methanol Pyr i d i n e Oc t a n o l D i e t h y l ether Ethyl acetate Chloroform Benzene Cyc lohexane
mg/ m 1 >3.33 >2.50 >3.33 >3.33 >5.00 > l o . 00 >5.00
2 . 3 DH Ranne T h e pH of a 5% w/v s o l u t i o n i n a water/ e t h a n o l (1: 1) s o l u t i o n is a b o u t 4 . 9 .
2 . 4 Dissociation Constant The pKa i n dimethylformamide/water is 9 . 4 5 .
(66:34)
RAFIK H. BISHARA AND HARLAN B. LONG
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2.5 Thermal Analyses
2.5.1 Differential Thermal Analysis
A DTA thermogram of dobutamine hydrochloride, at a heating rate of 5°C per min. in a nitrogen atmosphere of 40 cc per min., shows (figure 1) an endotherm at 196°C which appears to indicate a melt, 2.5.2. Thermogravimetric Analysis
A TGA thermogram of dobutamine hydrochloride, run simultaneously with the DTA, shows (figure 1) no weight loss until 233°C which results from decomposition. 2.6 Crystallinity
2.6.1 Crystalline Habit Dobutamine hydrochloride generally crystallizes in a random manner usually from an oil (1). This results in a nondescript crystalline formation. In only few cases does the drug exhibit any crystalline habit of interest. Upon careful and patient crptallization small thin plates and/ or small needles are formed. 2.6.2 X-Rav Powder Diffraction The following data describe the pattern for dobutamine hydrochloride, where d is equal to the integplanar spacing measured in terms of Angstroms (A). The ratio I/I, is the intensity of the X-ray maxima based upon a value of 100 for the strongest line. A b indicates a broad line resulting from failure to-resolve two closely spaced diffraction maxima.
Figure 1.
Thermogravimetric Analysis and Differential Thermal Analysis Thermograms of Dobutamine Hydrochloride
RAFIK H. BISHARA AND HARLAN B. LONG
144
0
CU-Ni- X 1.5418 A
d 9.07 6.87 6.37 5.27 4.98 4.50 4.13 4.04 3.78 3.60 3.44 3.18 3.11 3.01 2.86
d -
1/11
7 5 7 18b 18
2.74 2.63 2.51 2.40 2.35
100 16 61 45 45 16b 18 7 14 7
1/11
14 9 16 5 2
2.27 2.22 2.14 2.11 2.06 2.01 1.99 1.95
7 7 7
2 . 7 U l t r a v i o l e t SDectrum The u l t r a v i o l e t s p e c t r u m o f d o b u t a m i n e h y d r o c h l o r i d e i n m e t h a n o l is g i v e n i n f i g u r e 2 . The s p e c t r u m e x h i b i t s maxima a t 2 8 1 and 223 nm w i t h molar a b s o r p t i v i t i e s of 4 , 7 6 8 and 1 4 , 4 0 0 , r e s p e c t i v e l y . When a q u e o u s p o t a s s i u m h y d r o x i d e is a d d e d t o t h e m e t h a n o l i c s o l u t i o n o f d o b u t a m i n e hydroc h l o r i d e t h e maxima a t 2 8 1 a n d 223 s h i f t t o 293 ( e = 6 , 1 0 0 ) and 240 nm, r e s p e c t i v e l y . T h e s e s h i f t s are r e v e r s i b l e by a d d i t i o n of h y d r o c h l o r i c a c i d . When t h e a b s o r p t i o n s p e c t r u m o f t h e d r u g is r e c o r d e d i n water r a t h e r t h a n m e t h a n o l , s l i g h t s h i f t s i n peak p o s i t i o n s and i n t e n s i t i e s are observed : x max = 278 nm ( e = 4 , 1 1 2 ) X max = 220 nm ( E = 1 3 , 5 0 0 ) . 2 . 8 I n f r a r e d Spectrum The i n f r a r e d s p e c t r u m of d o b u t a m i n e hydroc h l o r i d e i n a p o t a s s i u m bromide d i s k is g i v e n i n f i g u r e 3. Major band a s s i g n m e n t s are a s f o l l o w s :
DOBUTAMINE HYDROCHLORIDE
145
10
5
WAVELENGTH, nm
Figure 2 .
U l t r a v i o l e t Spectrum of Dobutamine Hydrochloride
.Ooo
c
Figure 3.
Infrared Spectrum of Dobutamine Hydrochloride
147
DOBUTAMINE HYDROCHLORIDE
Band P o s i t i o n , cm-' 3400, 3300 and 3140 2960 and 2840 2700 and 2450 (weak bands) 1610, 1530, 1520 and 1450 1440, 1390 and 1380 1360, 1280-1190 ( s e v e r a l bands) 1150 and lower
Assignment phenolic 0-H s t r e t c h i n g C-H s t r e t c h i n g (overl a p i n g 0 - H bands 1 Mainly NH2, NH s t r e t c h i n g Aromatic r i n g s t r e t c h i n g C H 2 , C H 3 , C-H bending phenolic C-0 s t r e t c h i n g Mainly s k e l e t a l and a r o matic C-H bending
2 . 9 N u c l e a r Magnetic Resonance Spectrum T h e 60 MHz p r o t o n NMR Spectrum of dobutamine h y d r o c h l o r i d e i n d e u t e r a t e d d i m e t h y l s u l f o x i d e is g i v e n i n f i g u r e 4. Assignments of t h e bands are as follows:
d
c
i
I
I
H2
I I I
,
CH2-CH2-N+CI -
c I
-
I
a,
.l4
a Lc 0
0
0
rl Jz
Lc
h
a a,
X d
cd
E
.rl
c,
7 0
n
P 0
w E 1 Lc
DOBUTAMINE HYDROCHLORIDE
149
Chemical Shift (ppm) Multiplicity Area Assignment 1.3 doublet 3 a 1.9 unresolved 2 b mu 1t ip 1et 2.5 unresolved 2 C (overlapping solvent) 3.0 unresolved 5 d,e,f triplets 6.8 overlapping 7 aromatic protons mu 1t ip lets 8.9 very broad 5 g,h,i,j singlet 2.10 Mass Spectrum The mass spectrum of dobutamine hydrochloride given in figure 5 shows the molecular ion of the free base at m/e 301. The major fragmentation consists of a cleavage beta to the nitrogen to yield peaks at m/e 123 and 178 with relative intensities, to the base peak, of 15.2 and 97.6%, respectively. The base peak is at m/e 107.
3. Synthesis
A mixture of crotonic acid, thionyl chloride, and a catalytic amount of dimethylformamide is stirred in a solvent such as benzene to give 2butenoyl chloride ( I ) . The Friedel-Crafts reaction of methoxybenzene ( 1 1 ) with ( I ) using AlC1, in carbon disulf ide yields 1-( 4-methoxyphenyl)-2buten-1-one ( 1 1 1 ) . 3,4-Dimethoxybenzeneethanamine ( I V ) is then condensed with ( 1 1 1 ) to give 3-"2(3,4-dimethoxyphenyl)ethyl]amino]-l-(4-methoxypheny1)-1-butanone ( V ) . This ketone is reduced with hydrogen over Pd/C to give N-[2-(3,4dimethoxyphenyl)ethyl]-4-methoxy-a-methylbenzenepropanamine ( V I ) . An alternate .synthesis f o r compound ( V I ) involves the reduction of 4-(4methoxyphenyl)-3-buten-2-one ( V I I ) with hydrogen over Raney nickel to yield the corresponding butanone ( V I I I ) , which is then condensed with ( I V ) to produce the imine ( I X ) . Compound ( 1 x 1 is then reduced again with hydrogen over Pd/C to give ( V I ) .
150
Figure 5 .
RAFIK H. BISHARA A N D HARLAN B. LONG
Mass Spectrum of Dobutamine Hydr och l o r ide
DOBUTAMINE HYDROCHLORIDE
151
A second alternate synthesis of compound (VI) in-
volves the reaction of 4-methoxy-a-methylbenzenepropanamine (X) with 3,4-dimethoxybenzeneacetic acid (XI) at 200°C to yield 3,4-dimethoxy-N-[3(4-methoxyphenyl)-l-methylpropyl]benzeneacetamide (XII), which is then reduced with borane in THF to produce (VI). The trimethoxy secondary amine (VI) is demethylated by refluxing its solution in glacial acetic acid and HBr to yield dobutamine hydrobromide (XIII). Compound (XIII) is added to aqueous methanol then small amounts of hydrochloric acid are added to produce dobutamine hydrochloride (XIV). The flow diagram of the synthesis presented above (2) is shown in figure 6 .
4. Stability-Degradation Dobutamine hydrochloride is quite stable to refluxing in acid and to heating in air for 20 hours at 115°C (2). However, the drug is very rapidly oxidized to the corresponding aminochrome at pH 11-13. Approximate kinetic measurements suggest a half life of 30-45 minutes. This is similar to catecholamines which produce aminochromes that undergo further rapid and complex oxidations and/or condensations. These reactions yield products of unknown structure which finally are converted to dark colored polymers related to the melanins. Photolysis of an aqueous solution of the drug at 40-50°C for 5 days using a 325 w mercury lamp in the presence of oxygen also produced the aminochrome as the photooxidation product. 5. Absorption, Metabolism, and Excretion 5.1 In Dog The short plasma half-life of dobutamine (1-2 minutes) was found by Murphy et al. ( 4 ) to be due to the rapid redistribution of the drug from the plasma to the tissue. However, plasma halflife of radioactivity following the administration of 14C-dobutamine was 1.9 hours. The major circulating metabolite is the glucuronide conjugate of 3-0-methyldobutamine. During a continuous intravenous infusion of dobutamine, the plasma level of the parent drug reach a maximum withi’n 8 to 10 minutes, while those of the metabolites peak be-
RAFIK H . BISHARA A N D HARLAN B. LONG
152
I
Figure 6.
Synthesis of Dobutamine Hydrochloride
DOBUTAMINE HYDROCHLORIDE
I53
tween 3 and 4 hours. Dobutamine and/or its metabolites are eliminated via the urine and bile in both the dog and rat (5). After 4 8 hours from administering 14C-dobutamine to dogs, 67% of the radioactivity was excreted in urine and 20% in feces. Dogs with canulated bile ducts excreted 30 to 35% of the administered drug in the bile. The major urinary metabolites are the glucuronide conjugates of both dobutamine and 3-0-methyldobutamine. At very high doses of the drug, small amounts of hydroxylated dobutamine and hydroxylated 3-0-methyldobutamine were observed in the urine. The exact position of the extra hydroxyl group was not determined. The metabolites were not observed at therapeutic dosages. 5 . 2 In Man Serum levels of dobutamine reached a maximum of 20 ng/ml during a 15-minute infusion of dobutamine at a rate of 2 pg/Kg/min. and declined to 3 ng/ml within 5 minutes after the infusion. Rapid clearance from the plasma is indicated by its short half-life of approximately 2 minutes. Dobutamine is rapidly metabolized by methylation and conjugation to 3-0-methyldobutamine and conjugates of dobutamine. The major portion of the metabolites are excreted in the urine within the first 2 hours following infusion and the remainder within 6 hours. Metabolism and excretion in man are similar to the processes described above in the dog. F o r the detailed pharmacological and biochemical properties of dobutamine, the reader should consult the profile by Weber and Tuttle ( 5 ) . 6 . Methods of Analysis
6 . 1 Elemental Analysis ( A s C18H23N03-HC1) Element
C H
N 0 c1
Theory ( % > 63.99 7.16 4.15 14.21 10.49
I54
RAFIK H. BISHARA A N D HARLAN B. LONG
6 . 2 Chloride I d e n t i t y About 5 m l of d o b u t a m i n e h y d r o c h l o r i d e s o l u t i o n i n water, 1 mg/ml, is a c i d i f i e d w i t h t w o d r o p s of c o n c e n t r a t e d n i t r i c a c i d . When a d r o p of 0 . 1 N s i l v e r n i t r a t e is a d d e d t o t h i s s o l u t i o n a w h i t e p r e c i p i t a t e is formed which is r e a d i l y s o l u b i l i z e d by t h e a d d i t i o n of 3 d r o p s of ammonium h y d r o x i d e . T h i s i n d i c a t e s t h e p r e s e n c e of c h l o r i d e i o n . 6 . 3 Non-Aaueous
Titration
The s e c o n d a r y amine f u n c t i o n of d o b u t a m i n e h y d r o c h l o r i d e may b e d e t e r m i n e d by p o t e n t i o m e t r i c t i t r a t i o n w i t h p e r c h l o r i c a c i d using g l a c i a l acetic a c i d as a nonaqueous s o l v e n t . M e r c u r i c a c e t a t e is used t o t i e up t h e c h l o r i d e i o n . 6 . 4 Chloride Determination A s a m p l e o f d o b u t a m i n e h y d r o c h l o r i d e cont a i n i n g a t l e a s t 2 mg o f c h l o r i n e is i g n i t e d i n a S c h o n i g e r f l a s k c o n t a i n i n g 20 m l o f water. T h r e e d r o p s o f d i p h e n y l c a r b a z o n e ( 5 mg/ml) i n m e t h a n o l a r e added t o t h e s o l u t i o n of t h e c o m p l e t e l y b u r n e d s a m p l e . M e r c u r i c n i t r a t e , 0 . 5 N, is t h e n u s e d t o t i t r a t e t h i s s o l u t i o n t o t h e f i r s t s i g n of rose c o l o r , u s i n g a 1 m l microburette:
percent chlorine = m l m e r c u r i c n i t r a t e X n o r m a l i t y X 35.5 X 1 0 0 mg s a m p l e p e r c e n t p u r i t y of d o b u t a m i n e h y d r o c h l o r i d e = p e r c e n t c h l o r i n e f o u n d X 100 percent chlorine theory 6 . 5 Chromatographv
6 . 5 . 1 T h i n L a y e r Chromatography The Rf v a l u e f o r d o b u t a m i n e hydroc h l o r i d e when c h r o m a t o g r a p h e d on a s i l i c a g e l 6 0 F254 t h i n l a y e r p l a t e d e v e l o p e d by e t h y l a c e t a t e / n p r o p a n o l / w a t e r / a c e t i c a c i d (100/40/ 15/5 v / v / v / v ) i n an u n s a t u r a t e d chamber is a b o u t 0 . 6 7 . The s p o t of t h e d r u g may b e v i s u a l i z e d u n d e r s h o r t w a v e l e n g t h UV l i g h t ( 2 5 4 nm), or u n d e r w h i t e l i g h t a f t e r e x p o s u r e t o iodine vapors.
DOBUTAMINE HYDROCHLORIDE
155
6.5.2 Gas ChromatograDhv Silylated dobutamine hydrochloride (by reaction with N-trimethylsilylimidazole) may be chromatographed on a 3 foot glass column packed with 3% OV-225 on Chromosorb G AW-DMCS (100/120 mesh). The column is operated at 230°C using helium as a carrier gas at the rate of 60 ml/min. The retention time of the drug is approximately 4 minutes. A flame ionization detector is used. n-Triacontane is used as an internal standard. 6.5.3 High Performance Liquid Chromatography Dobutamine hydrochloride may be analyzed on a C,, reversed-phase column eluted with 75% 0.05M KH2P04, pH 4.4, and 25% methanol at 2 ml/minUte. The compound is detected at 280 nm. The retention time of the drug is approximately 6 minutes. 7. Analvsis of Biological Samples 7.1 Enzymatic Assay
Plasma levels of dobutamine hydrochloride are determined by reaction of the drug with 3Hme thyl-S-adenosy lmethionine in the presence of catechol 0-methyl-transferase. The radioactivity of the labeled methyl derivative is determined by a liquid scintillation counter using an external standard. The final recovery of added dobutamine as 3H-CH3-dobutamine is 24.9 f 1.3% in the range of 2 to 170 ng/ml ( 4 ) . When 14C-dobutamine is administered the samples are counted by a double isotope method.
7.2 Chromatographic Assays 7.2.1 Thin Layer Chromatography A Silica gel G plate is developed with a 15% aqueous solution of NaHSO,. The Rf Values in this system for dobutamine and 3-0-methyldobutamine are 0.50 and 0.35, respectively ( 4 ) .
156
RAFIK H. BISHARA AND HARLAN B . LONG
7.2.2Gas Chromatography Plasma and urine levels of the drug are determined by chromatographing the trimethylsilyl derivative of dobutamine on a 6-foot column packed with 3.0% UC-W98 silicon gum rubber (methylvinyl) on Diatoport S operated at 260°C. The hydrogen flame detector is maintained at 280°C. Helium flow rate is 60 ml/min. The retention time of dobutamine derivative (TMS) under these conditions is 3.8 minutes. This method measures plasma levels as low as 1 bg/ml (4). The levels of free and conjugated 3-0-methyldobutamine in plasma and urine are determined using electron capture detection of the pentafluoropropionate derivative of the metabolite. A 4-fOOt coiled column is packed with SP-2100 and maintained at 240°C. The temperature of the 63Ni electron capture detector is 250°C. The retention time of the pentafluoropropionate derivative is 1.6 minutes. Plasma levels as low as 50 ng/ml are readily measured using this method. 3-Hydroxy-N3-(4-hydroxyphenyl)-l-methyl-N-propyl)phenethylamine hydrobromide is used as an internal standard. 7.2.3. High Performance Liquid Chromatography Dobutamine hydrochloride may be determined in plasma levels, after extraction, on a C,, reversed-phase column eluted with 22% acetonitrile-78% 0.1 M phosphate buffer (pH 2.0) at 2 ml/minute. The drug and its metabolite are detected by a fluorescent detector with an excitation wavelength of 195 nm and a 330 nm emission cut off filter. The retention times of dobutamine and the 3-methoxy metabolite are 5.2 and 7.9 min., respectively. The lower limit of sensitivity is 10 ng/ml. Reproducibility is f 5% over a 25-300 ng/ml range. Nylidrin is used as an internal standard (6). 7.3 Mass Soectrometrv (GC/MS) The biological samples are analyzed with an LKB 900 GC mass spectrometer containing a 4-foot coiled glass column packed with 1% UC-W98 on Gas Chrom 9 . The column is maintained at 240°C and the
DOBUTAMINE HYDROCHLORIDE
157
flow rate of helium is 60 ml/min. The ion source voltage is 70 eV. The retention times of the trimethy Is ily 1 dobutamine and trimethy Is ilyl-3-0methyldobutamine are 3.8 and 3 . 6 min., respectively. The mass spectrum of the dobutamine-TMS shows a molecular ion at 517 and fragments at 250 and 2 6 7 . The spectrum of the derivatized metabolite has a molecular ion at 459 with major fragments at 250 and 2 0 9 . This fragmentation pattern confirms the presence of the methyl group on the catechol moiety. 8. Analysis of Pharmaceutical Formulations 8 . 1 Chromatographic Assays
8.1.1 Thin Layer Chromatography
Samples are dissolved in methanol. The insoluble excipients are removed by centrifugation. The solution is applied on a silica gel plate using the same conditions as listed previously in section 6 . 5 . 1 . Additional detection sensitivity may be obtained by spraying with a 6% solution of ferric chloride followed by a 2% solution of potassium ferricyanide. 8 . 1 . 2 Gas Chromatography
Samples are extracted into ethyl acetate from pH 9.0 buffer.. After evaporation of the solvent, n-triacontane, the internal standard, in pyridine/chloroform is added to the residue. The trimethylsilyl derivative is formed and chromatographed according to the details mentioned in section 6 . 5 . 2 . 8 . 1 . 3 High Performance Liquid Chromatography
Samples are dissolved in water to a concentration of approximately 0.5 mg/ml and injected directly into the liquid chromatograph without additional preparation. The conditions of section 6 . 5 . 3 apply also to the analysis of formu lat ions.
RAFIK H. BISHARA A N D HARLAN B. LONG
158
8.2 Spectrophotometric (UV)
Dobutamine hydrochloride may be determined spectrophotometrically in 0.5 M hydrochloric acid at the maximum of 278 nm. If excipients interfere, the drug may be extracted into ethyl acetate from pH 9 buffer followed by extraction into 0.5 M hydrochloric acid for the UV measurement. 9. Acknowledgments The authors are thankful to Dr. A. Hunt, Mr. H. W. Smith and Dr. A . D. Kossoy for their help in generating and permission to use the UV, crystallinity and stability degradation data.
References 1. H.W. Smith, personal communication, Eli Lilly and Company, Indianapolis, Indiana 46206.
2. R.R. Tuttle and J. Mills, French Patent No. 2,182,947 (1973); Ger. Offen. No. 2,317,710 (1973) and U.S. Patent No. 3, 987,200 (1976). 3. A.D. KOSSOY, personal communication, Eli Lilly and Company, Indianapolis, Indiana 46206.
4. P.J. Murphy, T.L.Williams and D.L.K. Kau, J. Pharmacol. Exp. Ther., 199,423 (1976). 5 . R. Weber and R.R. Tuttle, in M.E. Goldberg
(Editor), Pharmacological and Biochemical Properties of Drug Substances, American Pharmaceutical Association, Academy of Pharmaceutical Sciences, Washington, D . C . (1977) p. 109.
6. D.W. McKennon and R.E. Kates, J. Pharm. Sci., 67, 1756 (1978).
The literature is surveyed through January, 1979.
Analytical Profiles of Drug Substances, 8
ERYTHROMYCIN William L . Koch 1.
2.
3.
4. 5. 6.
Description I , I Name, Formula, Structure, and Molecular Weight I . 2 Appearance. Color, and Odor Physical Properties 2. I Solubilities 2.2 Infrared Spectrum 2.3 Ultraviolet Spectrum 2.4 Thermal Gravimetrk Analysis 2.5 Differential Thermal Analysis 2.6 X-Ray Diffraction 2.7 Nuclear Magnetic Resonance 2.8 pKa Methods of Analysis 3.1 Ultraviolet Assay 3.2 Gas Chromatographic Analysis 3.3 Colorimetric Analysis 3.4 Thin-Layer Chromatography 3.5 Microbiological Analysis 3.6 High Performance Liquid Chromatography Stability Bioavailability References
159
Copyright @ 1979 by Academic Press, Inc. All rights of reproduction in any form reSeNed. ISBN 0-12-260808-9
WILLIAM L. KOCH
I60
1.
Description 1.1
Name, Formula, S t r u c t u r e , and Molecular Weight Erythromycin, erythromycin A CH3 CH3
\/
Erythromycin A c3 7H6 7 N 0 1 3
Mol. w t . :
733.92
Erythromycin is a m a c r o l i d e a n t i b i o t i c c o n s i s t i n g of t h e a g l y c o n e , e r y t h r o n o l i d e A; t h e aminosugar, desosamine; and t h e n e u t r a l s u g a r , c l a d i n o s e . Using NNIR and CD s t u d i e s , 1 * 2 t h e conformation f e a t u r e s were deduced ( F i g . 1 ) .
WILLIAM L. KOCH
162
1.2
Appearance, Color, and Odor
The compound is a w h i t e c r y s t a l l i n e powder, p r a c t i c a l l y odorless, and h a s a b i t t e r taste. 2.
P h y s i c a l Propert ies 2.1
Solubilities
Webs et al.3 reported t h e s o l u b i l i t y of e r y t h r o m y c i n summarized i n T a b l e 1.
2.2
I n f r a r e d Spectrum
The i n f r a r e d s p e c t r u m of e r y t h r o m y c i n is commonly u s e d f o r its i d e n t i f i c a t i o n . F i g u r e 2 shows t h e s p e c t r u m of a 75 mg./ml. chlo_soform s o l u t i o n . The bands a t 1685 and 1730 c m are due t o t h e k e t o n e c a r b o n y l and t h e l a c t o n e c a r b o n y l , r e s p e c t i v e l y . The a b s o r p t i o n p e a k s a r e d u e t o t h e ethers between 1000 and 1200 cm' and m i n e f u n c t i o n s . T h e CH2 b e n d i n g is e v i d e n c e d by peaks between 1340 and 1460 cm' , and a l k a n e s r e t c h i n g p e a k s a p p e a r between 2780 Hydrogen bonded OH and wa er and 3020 cm' a p p e a r a s bands between 3400 and 3700 cm'
t.
2.3
1.
U l t r a v i o l e t Spectrum
The u l t r a v i o l e t s p e c t r u m of e r y t h r o mycin in m e t h a n o l e x h i b i t s Xmax a t 288 MI. The c v a l u e of 31.1 and t h e Xmax a r e c o n s i s t e n t w i t h t h e n +n* t r a n s i t i o n of C = 0 . 4
ERYTHROMYCIN
I63
TABLE 1 S o l u b i l i t i e s of Erythromycin Solvent
Isooct ane Petroleum e t h e r Cyclohexane Carbon d i s u l f i d e Carbon t e t r ach l o r i d e Toluene Benzene Diethyl ether Chloro f o m Ethylene c h l o r i d e Methyl e t h y l k e t o n e Acetone 1,4-Dioxane Isoamyl a c e t a t e Ethyl a c e t a t e Isoamyl a l c o h o l Pyr i d i n e Formam i d e Benzyl a l c o h o l Isopropanol Ethanol M e t hano 1 Ethylene g l y c o l Water
*
mg. / m l 0.477 4.69 0.2* 5.05 7 7 7 7 7 7 7
20 20 20 20
20 20 20 > 20 7 20 7 20 > 20 9.65
> 20 > 20 7 7 7 7
>
20 20 20 20 20 2.1
Weiss reported t h i s v a l u e a s > 20. found 0 . 2 i n our l a b o r a t o r i e s .
W e
10
I
I
I
I
3600
3200
2800
2400
Fig. 2.
I
1
I
2000 1800 1600 WAVENUMBER CM-'
I
I
I
1
UOO
1200
1000
800
Infrared abeorption spectrum of erythromycin
I65
ERYTHROMYCIN
2.4
Thermal Gavimetric A n a l y s i s
A TGA o f erythromycin h y d r a t e i n d i c a t e s a loss o f v o l a t i l e s o f about 4 2 , t h e n decomposit i o n s t a r t i n g a t 195OC.S 2.5
D i f f e r e n t i a l Thermal A n a l y s i s
A DTA o f erythromycin h y d r a t e shows an endotherm a t a b o u t 128'C., i n d i c a t i n g simult a n e o u s loss o f v o l a t i l e s and m e l t i n g . A DTA o f erythromycin a n h y d r a t e i n d i c a t e s m e l t i n g s t a r t i n g a t 193'C., t h e n decomposition.6
2.6
X-Ray D i f f r a c t i o n
The x-ray powder d i f f r a c t i o n p a t t e r n s o f erythromycin d i h y d r a t e and a n h y d r a t e are shown i n T a b l e 11. R a d i a t i o n : C r / V , X 2.2896.7 2.7
Nuclear Magnetic Resonance
The spectrum shown i n F i g u r e 3 was o b t a i n e d a s a CDsOD s o l u t i o n u s i n g a V a r i a n T-60A 60mHz i n s t r u m e n t , General band a s s i g n ments a r e l i s t e d i n T a b l e I11 a c c o r d i n g t o Underbr ink.
*
2.8
pKa
The pKa f o r erythromycin i n 66% DMF/34X w a t e r is 8.6.
WILLIAM L. KOCH
166
TABLE I1 X-Ray Eowder Diffract ion Data Erythromycin D ihydr at 8
Anhydr at e
ZLLa 19.02 15.63 13.40 11.14 10.11 9.74 8.43 7.79 7.24 6.79 6.43 6.31 6.02 5.71 5.46 5.20 5.01 4.85 4.78 4.57 4.51 4.43 3.91 3.75 3.58 3.35 2.98 2.23 2.06
50 10 70 60 60 80 100 60 70 15 60 60 15 70 20 70 10 60 50 20 30 40 20 10 05 02 02 02 02
11.84 9.01 8.57 7.26 6.73 6.40 6.12 5.43 5.05 4.99 4.60 4.42 4.25 4.12 4.00 3.90 3.78 3.39 3.30 3.16 2.99 2.90
10 50 100 10 100 20 40 30 40 30 30 20 20 20 10 10 10 10 10 10 10 10
WILLIAM L. KOCH
168
TABLE I11
NMR S p e c t r a l Assignments of m y t h r o m y c i n Solvent :
0 3 OD
Instrument:
V a r i a n T-60A 6 0 mHz
Proton ( 8 ) c!!3a2
-
A l l methyls not l i s t e d above
Resonance P o s i t i o n (PPM) .9
1-1.5
o r below
Peak Type Unresolved triplet Overlapping s i n g l e t s and doublets
2.35
Singlet
3.35
S i n g l e t (overlapping solvent mu 1t i p l e t )
O t h e r p r o t o n s (methyne and m e t h y l e n e ) g i v e u n r e s o l v e d and o v e r l a p p i n g m u l t i p l e t s i n t h e 60 mHz s p e c t r u m of t h e CD30D s o l u t i o n .
ERYTHROMYCIN
3.
169
Methods of Analysis
3.1
U l t r a v i o l e t Assay
The u l t r a v i o l e t chemical a s s a y f o r erythromycin remains l a r g e l y unchanged from t h a t described by Kuzel e t a l . 9 i n 1954. T h i s procedure is e s s e n t i a l v 8.8 follows. The reference s t a n d a r d , a l k a l i reagent, and b u f f e r s o l u t i o n s a r e prepared p r i o r t o t h e assay.
Phosphate b u f f e r pH 7 . 0 is prepared by d i s s o l v i n g 13.6 g. KH2FO4 (anhydrous) and 27.2 g. KzHFOl (anhydrous) i n s u f f i c i e n t p u r i f i e d water t o make 5 liters. The r e f e r e n c e s t a n d a r d s o l u t i o n is prepared by d i s s o l v i n g about 35 mg. a c c u r a t e l y weighed erythromycin s t a n d a r d i n 100 m l . methanol in a 250 m l . v o l u m e t r i c f l a s k . T h i s is d i l u t e d w i t h phosphate b u f f e r pH 7 . 0 t o 250 m l . , mixed, and allowed t o cool t o room t e m p e r a t u r e , t h e n a g a i n d i l u t e d t o t h e mark and mixed w e l l . The a l k a l i reagent is prepared by s l u r r y i n g 42 g. Na3F04*12Hz0 i n about 125 m l . 0 . 5 N NaOH i n a 250 m l . v o l u m e t r i c f l a s k . An add i t i o n a l 100 m l . p u r i f i e d water is added and t h e s l u r r y heated on t h e steam b a t h t o aid i n s o l u t i o n . The s o l u t i o n is cooled s l o w l y t o room temperature and d i l u t e d t o 250 m l . w i t h p u r i f i e d w a t e r , t h e n filtered p r i o r t o use.
Four 10 m l . a l i q u o t s of t h e s t a n d a r d s o l u t i o n are p i p e t t e d i n t o separate 25 m l . v o l u m e t r i c f l a s k s , two are labelled s t a n d a r d and t h e others blank. One m l . of 0 . 5 N HzSOd is added t o t h e blank f l a s k s and they are allowed t o s t a n d a f t e r mixing a t room temperature for 60 minutes f 5 minutes. Two ml. of p u r i f i e d water a r e added t o t h e s t a n d a r d f l a s k s . A t t h e end of t h i s time, 1.0 m l . of 0 . U NaOH is added t o t h e blank f l a s k s and t h e i r c o n t e n t s s w i r l e d
WILLIAM L. KOCH
I70
t o m i x . Then, 2 . 0 m l . of a l k a l i r e a g e n t s a r e added t o a l l f o u r f l a s k s , t h e y a r e s w i r l e d t o m i x and p l a c e d i n a 60.C. water b a t h f o r 15.0 m i n u t e s . The f l a s k s a r e t h e n cooled r a p i d l y i n a n ice b a t h , b r o u g h t t o room t e m p e r a t u r e , t h e n d i l u t e d t o 2 5 . 0 m l . w i t h p u r i f i e d w a t e r . The W a b s o r b a n c e is r e a d a t 236 nm. v e r s u s p u r i f i e d w a t e r i n 1.0 cm. s i l i c a c e l l s . The b l a n k v a l u e s a r e s u b t r a c t e d from t h e s t a n d a r d v a l u e s and t h e a v e r a g e n e t a b s o r b a n c e u s e d f o r c a l c u l a t ion. Bulk e r y t h r o m y c i n raw m a t e r i a l is t r e a t e d t h e same a s t h e s t a n d a r d . F o r m u l a t i o n s a r e made up t o t h e same c o n c e n t r a t i o n a s t h e s t a n d a r d i n m e t h a n o l and b u f f e r and 10 m l . a l i q u o t s u s e d for chromophore development.
The s u l f u r i c a c i d t r e a t e d a l i q u o t r e p r e s e n t i n g t h e b l a n k forms a c y c l i c ether anhydroerythromycin.10 The a l k a l i n e t r e a t m e n t c a u s e s t h e f o r m a t i o n of a n n,R u n s a t u r a t e d k e t o n e (9-keto-10-ene) h a v i n g its a b s o r b a n c e max inum a s a s h o u l d e r a t 236 nm. ( c 6000) . I 1 9 1 2 T h u s , any o t h e r W a b s o r b i n g s p e c i e s a r e measured w i t h t h e b l a n k and s u b t r a c t e d from t h e a b s o r b a n c e before c a l c u l a t i o n of t h e e r y t h r o m y c i n c o n c e n t r a t i o n . A t y p i c a l s p e c t r u m is shown i n F i g u r e 4 . 3.2
Gas Chromatographic Assay
T s u j i and Robertson13 r e p o r t e d a g a s chromatographic procedure for erythromycin u s i n g a n OV-225 column o r a PPE-20 column. T h e proc e d u r e i n v o l v e s s i l y l a t i n g 10 mg. e r y t h r o m y c i n w i t h a m i x t u r e of t r i m e t h y l c h l o r o s i l a n e , N , O - b i s t rime t h y 1si l y l a c e t am i d e , and N - t r imethy 1si l y l Ten i m i d a z o l e i n p y r i d i n e f o r 24 h o u r s a t 75'C. micrograms a r e i n j e c t e d o n t o t h e column (3 mm. x 1850 mm., 3% OV-225 o n GCQlOO-120 mesh o r 3 mm. x 1850 mm. 3% PPE-20 on S u p e l c o p o r t a t 275OC.) of a n F and M model 400 gas c h r o m a t o g r a p h e q u i p p e d w i t h a f l a m e i o n i z a t i o n detector. They r e p o r t b e i n g a b l e to s e p a r a t e e r y t h r o m y c i n s A , B, C ,
171
ERYTHROMYCIN
1.0
v)
0.5
0.0
I
I
220 240 260 280 300 nm Fig. 4 .
W s p e c t r a of sample and blank a f t e r
chrornophore development
172
WILLIAM L. KOCH
anhydroerythromycin A, and erythralosamine. Good agreement w i t h t h e microbiological a s s a y is shown. However, t h e biggest drawbacks appear t o be in s i l y l a t i o n time and t h e i n s t a b i l i t y of t h e GC column, 3 weeks a t 275°C. These authors1 4 l a t e r report u s i n g t h e GC method for e n t e r i c coated t a b l e t s of e r y t h r o mycin, g i v i n g a recovery of 99.8% and a coeff i c i e n t of v a r i a t i o n of 2.3% based o n placebo
tablets s p i k e d w i t h erythromycin. 3.3
Colorimetric Assays
Two procedures are worthy of note here. The first, published i n 1967 by Kuzel and C o f f e y l s i s based on t h e i o n p a i r dye complex of bromcresol p u r p l e (5' ,5"-dibromo-oc r e s o l - s u l f o n p h t h a l e i n ) and t h e desosamine moiety of erythromycin i n pH 1.2 b u f f e r . The method l a c k s s p e c i f i c i t y for erythromycin, measuring a l l t e r t i a r y amines; however, it is q u i t e s e n s i t i v e and precise, being r o u t i n e l y used for concentrations of 250 mcg. erythromycin/ml. i n t a b l e t s i n f e r m e n t a t i o n broth. A and 20-100 mcg./ml. more r e c e n t method by Sanghavi and Chandramohan16 is a l s o based on a complex of t h e desosamine moiety, but t h e y u s e p-dimethyl amino benzaldehyde a s t h e coupling a g e n t , The procedure is non-spec i f ic , but s e n s it i v e and l i n e a r over a c o n c e n t r a t i o n range of 10-35 mcg./ml. ,
3.4
Thin Layer Chromatography
Egon S t a h l l 7 described four TLC systems. Table IV summarizes the s o l v e n t s and R f ' s o n s i l i c a gel G.
ERYTHROMYCIN
I73
TABLE IV
Solvent Methanol
.16
Chlorof orm-me t hano 1 95
+
.03
5
Chloroform-methanol
.29
Butanol-acet ic acid-water 6 0 + 20 + 20
.39
50
+
Detect i o n
EL
50
Brownish-green color after spraying w i t h 10%s u l f u r i c acid and h e a t i n g 5-10 minutes a t 8OoC.
Spraying w i t h 10%molybdophosphoric acid i n alcohol, followed by h e a t i n g produces a b l u e s p o t on a yellow background. The s p o t d i s a p p e a r s i n 2 hours.
--
Vilim e t a l . l * d e v i s e d a TLC i d e n t i f i c a t i o n s y s t e m f o r erythromycin b a s e , s t e a r a t e , e s t o l a t e and e t h y l s u c c i n a t e . T h i s combination cannot d i f f e r e n t i a t e between t h e e s t o l a t e and ethylsuccinate. Our l a b o r a t o r i e s l 9 have developed a system s e p a r a t i n g erythromycin e s t o l a t e , e r y t h r o mycin base, and anhydroerythromycin on a s i l i c a g e l 6 0 F-254 p l a t e u t i l i z i n g e t h a n o l , methanol, t r i e t h y l a m i n e , 170:30:1. V i s u a l i z a t i o n is made by s p r a y i n g w i t h 0.15% x a n t h y d r o l and 7 . 5 % a c e t i c acid i n water. T a b l e V summarizes t h e R f ' s .
TABLE V_
Component Erythromycin Base
Rf 0.30
Color Violet
Anhydroerythromgc i n
0.43
Violet
Er y t hromyc i n Es t ol a t e
0.60
Violet
WILLIAM L. KOCH
I74
3.5
M i c r o b i o l o g i c a l Analysis
Kavanagh and Dennen2 r e p o r t microb i o l o g i c a l t u r b i d i m e t r i c and p l a t e a s s a y s f o r erythromycin base i n A n a l y t i c a l Microbiology, vol. 1. Staphylococcus a u r e u s (ATCC 9144) is used for t h e t u r b i d i m e t r m c e d u r e . The bulk raw m a t e r i a l o f f i c i a l a s s a y is found i n 2lCFR 452.10 and t h e o f f i c i a l t a b l e t a s s a y is found i n The sample is d i l u t e d from 0.3 t o 21CFR452.110. 2.0 tig./ml. i n pH 7 . 0 b u f f e r and comparison is made t o a s t a n d a r d curve of 0 , 0 . 3 , 0 . 4 , 0 . 6 , 0 . 8 , 1 . 2 , 1 . 6 , and 2.0 !ig./ml. Sarcina lutea (ATCC 9341) is used f o r t h e p l a t e a s s a y . A i n e a r response i n t h e r a n g e of 0.5 2.0 ug./ml, is o b t a i n e d when pH 8 . 0 b u f f e r is used for sample and s t a n d a r d . I n b o t h methods, a s m a l l amount of methanol is used t o s o l u b i l i z e t h e erythromycin p r i o r t o b u f f e r i n g a t pH 7 . 0 or 8 . 0 .
-
-
3.6
High Performance Liquid Chromatography
Omura e t a1.21 used a r e v e r s e phase high performance l i q u m Z r o m a t o g r a p h i c column, JASCO PACK SV-02-500@, f o r macrolide a n t i b i o t i c s w i t h methanol, W15 a c e t a t e b u f f e r pH 4 . 9 , and a c e t o n i t r i l e (35:60:5) a s s o l v e n t . A v a r i a b l e wavel e n g t h W detector u s i n g t h e a b s o r p t i o n of t h e i n d i v i d u a l compounds gave t h e r e q u i r e d s e n s i t i v i t y . A l t e r a t i o n s of b u f f e r pH and t h e composition r a t i o of t h e mobile phase gave s e l e c t i v i t y f o r s e p a r a t i o n of i n d i v i d u a l macrolide a n t i b i o t i c s . 2. €I. Hash22 r e p o r t e d chromatographic c o n d i t i o n s f o r s e p a r a t i n g anhydroerythromycin from erythromycin u s i n g a normal phase C o r a s i l II@ s i l i c a g e l column, w i t h chloroform a s mobile phase and r e f r a c t i v e index detect ion.
White e t a l . 2 3 d e v i s e d a r e v e r s e phase high performance-riquid chromatographic procedure f o r erythromycin. R e f r a c t i v e index d e t e c t i o n was used s i n c e t h e compound absorbs weakly i n t h e W. A 10 inn C1,/Lichrosorb” r e v e r s e phase column was used w i t h 80% methanol, 19.9% w a t e r , 0.1% ammonium hydrochloride a s t h e developing s o l v e n t .
175
ERYTHROMYCIN
T s u j i and Goetz2' d e v e l o p e d a q u a n t i t a t i v e high performance l i q u i d chromatographic method f o r s e p a r a t i n g and m e a s u r i n g e r y t h r o m y c i n s A , B, and C , t h e i r e p i m e r s and d e g r a d a t i o n produ c t s . T h i s method u s e s a p o n d a p a k @ C1 r e v e r s e column w i t h a c e t o n i t r ile-met hanol-0.2M ammonium a c e t a t e - w a t e r (45 :10 :10 :25) a s s o l v e n t . The pH and c o m p o s i t i o n of t h e mobile p h a s e may be adj u s t e d t o o p t i m i z e r e s o l u t i o n and e l u t i o n volume. The a u t h o r s u t i l i z e d t h e p r o c e d u r e o n USP r e f e r e n c e s t a n d a r d and r e p o r t a r e l a t i v e s t a n d a r d d e v i a t i o n of f 0.64%. 4.
Stability
Erythromycin is u n s t a b l e i n a c i d i c o r a l k a l i n e s o l u t i o n s and shows its maximum s t a b i l i t y between pH 6 . 0 and 9.525. Its a q u e o u s , a l c o h o l i c 8 . 0 is s t a b l e f o r s o l u t i o n b u f f e r e d a t pH 7 . 0 a b o u t o n e week u n d e r r e f r i g e r a t i o n .
-
5.
Bioavailability
Maximum l e v e l s of e r y t h r o m y c i n i n serum a r e o b t a i n e d i n 1 t o 2 h o u r s a f t e r a s i n g l e dose. T h e U. S. D i s p e n s a t o r y 2 ' reports maximum serum l e v e l s of 0 . 2 i j g . / m l . 1 hour a f t e r a d m i n i s t r a t i o n of a 250 mg. d o s e , 0.6 !ig,/ml. 2 h o u r s a f t e r a 500 mg. dose, and 1 . 2 t g . / m l . 2 hours a f t e r a 1 g. dose. Higher blood l e v e l s a r e a c h i e v e d o n a m u l t i p l e d o s a g e s c h e d u l e . S i n c e it is a c i d l a b i l e , a r e s i s t a n t c o a t i n g is u s e d i n t a b l e t f o r m u l a t i o n s t o overcome t h e d e l e t e r i o u s e f f e c t of g a s t r i c f l u i d on e r y t h r o m y c i n b a s e ; o r t h e s t e a r a t e s a l t is p r e p a r e d w h i c h does n o t d i s s o l v e r e a d i l y i n t h e stomach, The B i o a v a i l a b i l i t y Monograph f o r E r y t h r o mycin27 p r o v i d e s d a t a f o r c o m p a r i s o n of s e v e r a l m a n u f a c t u r e r s * t a b l e t s of e r y t h r o m y c i n , T h e c r i t e r i a f o r b i o a v a i l a b i l i t y tests a r e d i s c u s s e d .
WILLIAM L. KOCH
176
6.
References
1. K. Gerzon, p e r s o n a l communication, L i l l y Research L a b o r a t o r i e s . 2. R. S. Egan, T. J. Perun, J. R. Martin, 9 , 2525and L. A. M i t s c h e r , T e t r a h e d r o n 2 2538 (1973). 3. P. J. Weiss, 1. L. Andrew, and W. W. Wright, A n t i b i o t i c s and Chemotherapy 7 ( 7 ) , 374-377 (1957) a 4. R. M. S i l v e r s t e i n and G. C. Bassler, S p e c t r o m e t r i c I d e n t i f i c a t i o n o f Organic Compounds, 2nd Ed., John Wiley and Sons, New York, p. 151. 5 . T. E. Cole, p e r s o n a l communication, L i l l y Research L a b o r a t o r i e s . 6. T. E. Cole, p e r s o n a l communication, L i l l y Research L a b o r a t o r i e s 7. H. A. R o s e , A n a l y t i c a l Chemistry -’ 26 938 (1954). 8. C , D. Under b r i n k , persona 1 communi c a t i o n , L i l l y Research L a b o r a t o r i e s . 9. N. R. Kuzel, J. M. Woodside, J. P. Comer, and E. E. Kennedy, A n t i b i o t i c s and Chemot h e r a p y 6 , 1234-1241 (1954). 10. P. Kuratii, P. H, Jones, R. S. Egan, and T. J. PBrun, l k p e r e n t i a 27 ( 4 ) , 362 (1971). 11. E. H. Flynn, M. V. S i g a l , J r . , P. F. W i l e y , K. Gerzon, J o u r n a l o f t h e American Chemical S o c i e t y 76, 3121-3131 (1954). 12. T. J. Perun, J o u r n a l o f Organic Chemistry 3 2 , 2324-2330 (1967). 13. K. T s u j i and J. €IRobertson, . Analytical Chemistry 43 ( 7 ) , 818-821 (1971). 14. J. H. Rober’tson and K. T s u j i , J o u r n a l o f -1 (lo), 1633Pharmaceutical S c i e n c e s 6 1635 (1972). 15. N. R. Kuzel and H. F. Coffey, Technicon Symposium (1966), V o l . 1, Automation in A n a l y t i c a l Chemistry, Medical, Inc. , White P l a i n s , N.Y., 1967, pp. 235-239.. 16. N. M. Sanghavi and H. S. Chandramohan, Canadian J o u r n a l o f Pharmaceutical Sciences 10 (2), 59-61 (1975).
.
-
1I1
ERYTHROMYCIN
17. E. S t a h l , Ed., Thin Layer Chromatography, A Laboratory Handbook, 2nd Ed., S p r i n g e r V e r l a g , N . Y . , 1969, pp. 572. 18. A. V i l i m , M. J. I s B e l l e , W. L. Wilson, and K. C. Graham, J o u r n a l of Chromatography 133, 239-244 (1977). 19. H. F. Hugar, p e r s o n a l communication, L i l l y Research L a b o r a t o r i e s . 20. D. W. Dennen, i n F. Kavanagh ( E d i t o r ) , A n a l y t i c a l Microbiology, V o l . 1, Academic Press (1963), pp. 209-294. 2 1. S. Omura, Y. S u z u k i , A. Nakagawa, and T. Hata, The J o u r n a l of A n t i b i o t i c s V o l . XXVI, NO. 12, 794-795 (1973). 22. Z. H. Hash, Methods i n Enzymology, V o l . LXIII, p. 3 0 8 , Academic mess, New York, 1975. 23. E. R. White, M. A. C a r r o l l , and J. E. Zarembro, The J o u r n a l of A n t i b i o t i c s , V O l . XXX, NO. 1 0 , 811-818 (1977). 24. K. T s u j i , J. F. Goetz, J o u r n a l of Chromatography, 147, 359-367 (1978). 25. F. Kavanagh, A n a l y t i c a l Microbiology, V o l . 1, Academic Press (1963), pp. 209294. 26. U. S. D i s p e n s a t o r y , 2 7 t h Ed., A. -01, R. P r a t t , and A. R. Gennaro E d i t o r s , J. B. L i p p i n c o t t , P h i l a d e l p h i a (1973), pp. 487. 27. C. H. N i g h t i n g a l e , J o u r n a l of t h e American Pharmaceutical A s s o c i a t i o n NS 16, ( 4 ) , 203-206 (1976).
-
Analytical Profiles of Drug Substances. 8
GRAMICIDIN Glenn A . Brewer I . Introduction 2. Chemistry 3. Description 3. I Composition, Formula, Molecular Weight 3.1 I GramicidinA(l1029-61-1) 3.12 Grarnicidin B ( I 1041-38-6) 3.13 Gramicidin C (9062-61-7) 3.14 Gramicidin D (1405-97-6) 3.2 Appearance, Color, Odor 4. Physical Properties 4.1 Spectra 4. I I Infrared Spectra 4. I2 Nuclear Magnetic Resonance Spectra 4.13 Ultraviolet Absorption Spectra 4.14 Fluorescence Spectra 4.15 Rarnan Spectra 4.2 Crystal Properties 4.2 I Crystalline Modifications 4.22 X-Ray Powder Diffraction 4.23 Crystal Density 4.24 Differential Thermal Analysis 4.3 Solubility 4.31 Solubility in Pure Solvents 4.32 Solubility in Solutions of Quaternary Ammonium Compounds 4.33 Solubility in Solutions of Other Surface Active Agents 4.4 Physical Properties of Solutions 4.41 Diffusion 4.42 Surface Tension 4.43 Specific Volume 4.4 Conformation 5. Production 5. I Fermentation 5.2 Isolation 5.3 Derivatives 6. Stability 6. I Stability in Solution 6.2 Effect of Light 6.3 Stability of Formulations 7. Analytical Methods. 7. I Identity Tests 7.2 Microbiological Assays
I79
Copyright @ 1979 by Academic Press. Inc. All rights of reproduction in any form reserved. ISBN 0-12-260808-9
I80 7.21 Dilution Methods 7.22 Dye Reduction Methods 7.23 Turbidimetric Assays 7.24 Agar Diffusion Assays 7.25 Potentiation of Microbiological Assays 7.3 Chemical Assays 7.31 Colorimetric Assays 7.32 Spectrophotometric Methods 7.33 Miscellaneous Methods 7.4 Electrochemical Methods 7.5 Hemolytic Methods 7 . 6 Enzymatic and Other Biochemical Methods 7.7 Chromatographic Methods 7.71 Counter Current Distribution 7.72 Paper Chromatography 7.73 Thin-Layer Chromatography 7.74 Electrophoresis 7.75 Column Chromatography 7.76 High Performance Liquid Chromatography 8. Reviews References
GLENN A. BREWER
GRAMICIDIN
1.
181
Introduction Gramiddin is a peptide antibiotic first isolated by
D u b o s in 1939l as a crude complex together with a second
peptide antibiotic known as tyrocidin. The mixture of the two antibiotics was called tyrothricin. Although the mixture was discovered about ten years after penicillin2, tyrothricin was the first antibiotic utilized in clinical practice. It was soon found that tyrothricin causes severe hemolysis when administered parenterally and was destroyed when given orally. The antibiotic complex or individual components are effective topically and are used in various cream, ointment, lotion and solution preparations alone or in combination with other antibiotics or topical steroids3. The aspect of gramicidin which is of most interest to the analytical chemist is the continued.study of the structure of the antibiotic,from its discovery to the present day. As more and more sophisticated separation and structural elucidation techniques have been deueloped, various scientists have applied these to the problem of understanding the complete structure of the gramicidin complex. Thus, we can trace the development of our understanding of the structure from the crude extract prepared by Dubosl to our current knowledge of not only the structure of the various components of gramicidin, but the conformation of the major fraction in s~lution.~It is indeed interesting that so many scientists have applied their knowledge and skill to solve this difficult structural problem,considering the relative minor role of this material product in modern medicine. 2.
Chemistry
Tyrothricin was obtained by acidification of the fermentation broth of Bacillus brevis to precipitate the antibiotic activity along with various proteins and then dissolving the antibiotic complex in alcohol. The alcohol was removed under vacuum, the residue was washed with ether, then redissolved in alcohol and finally reprecipitated with 1% sodium chloride5 6 . It was soon recognized that tyrothricin was not a pure compound but could be separated into a neutral fraction called gramicidin and a basic fraction called tyroci-
182
GLENN A. BREWER
dine by extraction with acetone and ether mixtures. The individual fractions were thought to be homogeneous because they were crystalline and had constant physical properties on recrystalli~ation~ 1' 1 1 1 2. At the time, these constant properties were considered to be sufficient proof to indicate chemical purity. A n empirical formula of C74H106N14014 was proposed for gramicidin based on elemental analysis and a Rast molecular The application of various bioweight determination'. chemical methods led the investigators to the conclusion that gramicidin was a peptide containing ten a-amino acid residues and a saturated aliphatic fatty acid containing 14 to 16 cabon atoms. It was established that a hydrolysate of gramicidin contained tryptophane and that histidine, arginine, tyrosine and ammonia were absent. The authors further noted that about half of the amino acid residues have the D-(unnatura1)configuration. This was shown by oxidation with d-amino acid oxidase' 1 2.
Other workers began to study the structure of gramicidin. Christensen and coworkers isolated crystalline tryptophane and leucine from a hydrolysate. They found no evidence for a fatty acid component and established that phenylalanine, proline and hydroxyproline were absent from a hydrolysate. These workers isolated alanine dioxpyridate from a hydrolysate and also established that gramicidin contained a compound with vicinal hydroxy and amino groups. They speculated that this compound might be serine or isoserine and proposed that gramicidin contains two tryptophane, 2 leucine, 2 or 3 alanine and 1 hydroxyamino residues or a multiple of this composition. Hotchkissl isolated optically and analytically pure d-leucine from the hydrolysate. This was the first nonenzymatic proof that d-amino acids actually occurred in gramicidin. He also noted the presence of an amino-hydroxy compound, but indicated that it was not isoserine. Gordon, Martin and Synge15 utilized their new and elegant technique, chromatography, to establish the amino acid composition of gramicidin. They proposed a 24 unit cyclic peptide consisting of six moles each of leucine, and tryptophane, 5 moles of valine, 3 moles of alanine and 2 moles each of glycine and unknown hydroxyamino compound. They confirmed that the leucine was the d-form while the tryptophane and alanine had the L-configuration. The
GRAMICIDIN
183
valine appeared to be racemic. Christensenl isolated the dipeptide valylvaline from completely hydrolyzed gramicidin. This worker later showed that he had isolated a racemic mixture of D(-)-valylD(-)-valine and I,(+)-valyl-L(t)-valine rather than dipeptides containing one d and one L-residue. l 7 Synge’’, using starch columns,confirmed the presence of valylvaline and identified L-valylglycine in partial hydrolysates. This unexpected finding triggered a good deal of work on the kinetics of peptide hydrolysis in an attempt to develop a rational explanation. Synge2’ isolated the elusive hydroxyamino compound by azeotropic distillation and identified it as 2-aminoethanol. He proposed a structure of 6 L-tryptophane, 6 D-leucine, 5 D and L-valine, 3 L-alanine, 2 glycine and 2 aminoethanol residues. There was some evidence that the preparations of gramicidin used in this structural work were not completely homogeneous15,22 but the evidence was not strong until Gregory and Craig2 separated crystalline gramicidin into three major fractions by counter current distribution. Fraction B contained only 55% as much tryptophane as Fraction A based on an ultraviolet analysis. The third fraction was called gramicidin C. Still using heterogeneous gramicidin,S ~ n g eisolated ~ ~ the D-leucylglycine, L-alanyl-D-valine and L-alanyl-Dleucine from partial hydrolysates of gramicidin. He also had less conclusive evidence for the tripeptides alanylvalylleucine or alanylleucylvaline. In a review paper, Dr. S ~ n g erecapitulated ~ ~ the early structural work on gramicidin and indicated that x-ray diffraction was incapable of distinguishing a gramicidin fraction purified by counter current analysis from the heterogeneous starting material. Hinman, Caron and ChristensenZ6 corrected the earlier report by Christensen16. They reported that the dipeptides found on the hydrolysis of gramicidin were D-valyl-L-valine and L-valyl- D-valine.
I84
GLENN A. BREWER
James and S ~ n g e speculated ~ ~ on the nature of the nonpeptide bonds in gramicidin. Hodgkin2' examined crystals of gramicidins A and B by x-ray diffraction. She estimated that the molecular weight of gramicidin A was approximately 3800, Previous estimates by chemical methods were approximately 7000. In 1953, Cowan and Hodgkin2' published a second report on gramicidin B. A provisional structure for gramicidin was proposed by Gavrilov and Akimova30.
Okuda and coworkers31 determined the amino acid compo~~ sition of gramicidins A, B and C. Ishii and W i t k ~ pestablished the complete optical assignment of the amino acids in gramicidin A using enzymatic degradation and quantitative gas chromatography. The composition established was 4 moles of L-tryptophane, 4 moles of D-leucine, 2 moles of D-valine, 2 moles of L-valine", 2 moles of L-alanine, 1 mole of glycine and 1 mole of aminoethanol. (*The authors actually found 1.6 moles of L-valine and 0.6 moles of L-isoleucine. This indicated the possibility of the non-homogeneity of gramicidin A . ) The evidence that gramicidin A was actually heterogeneous was obtained by Ramachandran3 using counter current distribution with more than 1000 transfers. The new gramicidin which contained isoleucine was called gramicidin D. This was an unfortunate choice of terminology since the crude mixture of gramicidin fractions had been previously called gramicidin D (gramicidin Dubos) to distinguish it from other gramicidins (S and J). Sarges and established the amino acid sequence of gramicidins A and D. The same authors also established the amino acid sequences of gramicidins B36 and C37. In addition, they synthesized gramicidins A and D3'. Gross and Witkop3' subjected commercial gramicidin to counter current distribution. They found that gramicidins A , B and C all consisted of a pair of congeners containing primarily valine-gramicidins (00-95%) with some isoleucine-gramicidins (5-20%) as minor components. In addition, they isolated a more hydrophilic, strongly antibiotic group of antibiotics which they called gramicidin D.
GRAMlCIDlN
185
Urry and coworkers4 41 proposed a left-handed helical structure for gramicidin A. This conformation can undergo ion induced relaxations which provides a mechanism for the movement of the ion along the channel. These workers confirmed this proposed structure by nuclear magnetic resonance spe~trometry~~. Using circular dichroism and nuclear magnetic resonance spectrometry, Veatch and coworkers4 established that four conformational species of gramicidin A exist in solution. Two were postulated to be helixes of opposite handedness. 3.
Description 3.1
Composition, Formula, Molecular Weight
The gramicidin of commerce is a complex of at least four compounds. The identified fractions are called gramicidins A, B, C and D. The major component of the mixture is gramicidin A. (See Section 2.) The mixture of gramicidins is called gramicidin The latter name is used to distinguish the gramicidin discovered by Dubos from gramicidins S and J. [1405-97-61 or gramicidin D (Dubos) [1393-88-01.
As discussed in Section 2, the chemical structure of the various fractions has now been elucidated. The general formula for gramicidin is shown below, where R and R ' are different amino acid residues depending on the particular type of gramicidin. HCO-R-Glycine-L-Alanine-D-Leucine-L-Alanine-D-ValineL-Valine-D-Valine-L-Tryptophane-D-Leucine-R'-D-LeucineL-Tryptophane-D-Leucine-L-Tryptophane-NHCH2CH2OH
3.11
Gramicidin A [11029-61-11
Gramicidin A consists of a pair of congeners containing primarily L-valine gramicidin A (8095%) but also containing L-isoleucine gramicidin A (5-20%)3 9 8 34.
GLENN A. BREWER
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3.111
L-Valine Gramicidin A [4419-81-21
R = L-valine R ’ = L-tryptophane N O ‘9gH140 20 17 Molecular Weight 1882.349 3.112
L-Isoleucine Gramicidin A [553603-81
R
=
L-isoleucine
R ’ = L-tryptophane
N O ‘100H142 20 17 Molecular Weight 1896.376 3.12
Gramicidin B [11041-38-61
Gramicidin B consists of a pair of congeners containing primarily L-valine ramicidin B but also containing L-isoleucine gramicidin B 3%
.
3.121
L-Valine Gramicidin B [4422-52-01 R = L-valine R’= L-phenylalanine N O C97H139 19 17 Molecular Weight 1843.312
3.122
L-Isoleucine Gramicidin B R = L-isoleucine R ’ = L-phenylalanine N O C98H141 19 17 Molecular Weight 1857.339
3.13
Gramicidin
C
[9062-61-71
Gramicidin C also consists of a pair of congeners containing primarily L-valine gramicidin C but also small amounts of L-isoleucine gramicidin C are present37. 3.131 L-Valine Gramkidin C [58442-65-21 R = L-valine R ’ = L-tyrosine C97H139N19018 Molecular weight 1859.312
I87
GRAMICIDIN
3.132
L-Isoleucine Gramicidin C R
=
L-isoleucine
R’= L-tyrosine
N
O
‘9BH141 19 18
Molecular Weight 1873.339 3.14
Gramicidin D [1405-97-61
As previously discussed, the term gramicidin D has been used to designate the entire gramicidin complex of gramicidins A, B, C, D or the isoleucine component of gramicidin A33. Gross and W i t k ~ phave ~ ~ used it to name a minor and still undefined, polar fraction of the gramicidin complex. In the rest of this Analytical Profile, the physical and chemical properties which will be described will be of the complex mixture of gramicidins A, B, C and D unless otherwise noted. 3.2
Appearance, Color, Odor
Gramicidin is described as a crystalline powder, which is white or nearly white and is odorless43. 4.
Physical Properties 4.1
Spectra 4.11
Infrared Spectra
The infrared spectrum of gramicidin has been reported by Hayden, et al.44. The infrared spectra of the U.S.P. gramicidin standard are presented in Figures 1 and 245. 4.12
Nuclear Magnetic Resonance Spectra
Nuclear Magnetic Resonance has been used to establish the conformation of the pure fractions of the gramicidin complex42. The proton resonance spectrum of the U.S.P. gramicidin standard is shown in Figure 346.
189
t
d
9
d
GRAM IC ID1N
191
4.13
Ultraviolet Absorption Spectra
The tryptophane content of the gramicidin complex was measured by the ultraviolet absorbanceY7. Cann has demonstrated the shift to longer wavelengths when acetic acid complexes with gramicidin4'. The ultraviolet spectrum of the gramicidin complex has been reported by Hayden and coworker^^^. Figure 4 presents the ultraviolet spectrum of the U.S.P. Reference standard taken in 95% ethanol".
4.14
Fluorescence Spectra
Sommermeyer and coworkers50 reported that solutions of gramicidin exhibit fluorescence when irradiated with soft x-rays. Gramicidin exhibits strong fluorescence in 95% ethanol. The excitation maximum is at 286 nm and the emission maximum is at 337 nm. The fluorescence intensity was linear with respect to concentration in solution5'. 4.15
Raman Spectra
Rothchild and Stanley studied the con. formation of Gramicidin A using Raman s p e c t r o ~ c o p y ~ ~Two types of conformation were found depending on the solvent used. 4.2
Crystal Properties 4.21
Crystalline Modifications
Dr. Synge noted that when gramicidin complex was crystallized from acetone, he obtained small crystals that were not suitable for x-ray diffraction25. When the sample was allowed to crystallize from alcoholic solution by slow evaporation, large chunky crystals were obtained. These gave very good x-ray diffraction patterns. Olesen and Szabo obtained crystals from ethanol and acetone53. They found the crystals to have different solubility, melting point and x-ray diffraction patterns. Since acetone is retained in the crystalline lattice, it was indicated that the forms are pseudopolymorphs.
I93
GRAMICIDIN 4.22
X-ray Powder Diffraction
A s was mentioned in Section 2, x-ray diffraction was used in an effort to establish the structure of the gramicidin complex25'2 8 ' 29. These studies were frustrated by the fact that the gramicidin was not chemically pure but was a mixture of components.
Belavtseva found that crystalline gramicidin was converted to amorphous gramicidin by the action of x-rays54. The powder x-ray diffraction pattern of the gramicidin U.S.P. reference standard is shown in Figure 5 5 5 . The relative peak intensities are presented in Table 1. TABLE 1 Relative Peak Intensities of U.S.P. Gramicidin Reference Standard as Measured by Powder X-Ray Diffraction 20 D (DEG.) (ANGSTROMS) 6.64 7.40 9.44 13.69 14.46 16.75 16.92 17.86 19.39 20.07 21.26 21.68 22.28 23.55 23.89
13.31 11.95 9.37 6.47 6.13 5.29 5.24 4.97 4.58 4.42 4.18 4.10 3.99 3.78 3.72
PEAK 143.5 104.1 28.4 31.1 28.6 46.5 45.3 48.7 63.8 50.7 38.8 39.5 37.2 36.2 34.6
REL. PEAK
AREA
REL. AREA
1.000 0.725 0.198 0.217 0.199 0.324 0.316 0.339 0.445 0.353 0.270 0.275 0.259 0.252 0.241
850.0 791.4 301.2 327.6 246.0 349.9 274.6 473.6 716.2 414.9 288.3 250.9 275.6 312.1 306.0
1.000 0.931 0.354 0.385 0.289 0.412 0.323 0.557 0.843 0.488 0.339 0.295 0.324 0.367 0.360
.GLENN A. BREWER
1 94
4.23
Crystal Density
Low and Richards used a density gradient column to study the density of crystals of "mixed gramicidir. fractions"56. 4.24
Differential Thermal Analysis
The U.S.P. gramicidin standard shows a small endothem at 161OC and a larger endotherm at 244OC. Both endotherms are broad57. 4.3
solubility 4.31
Solubility in Pure Solvents
The solubility of the gramicidin complex in a variety of solvents has been determined by Weiss and coworkers5*. TABLE 2 Solubility of Gramicidin Complex in Various Solvents
SOLVENT
SOLUBILITY mg/ml
Water Methanol Ethanol Isopropanol Isoamyl Alcohol Cyclohexane Benzene Toluene Petroleum Ether Isooctane Carbon Tetrachloride Ethylene Glycol
0.140 > 20 > 20 > 20 14.10 0.02 0.19 0.04
0.007 0.005 0.047 > 20
SOLVENT
SOLUBILITY mg/ml
Ethyl Acetate Isoamyl Acetate Methyl Ethyl Ketone Acetone Diethyl Ether Ethylene Chloride 1,4-Dioxane Chloroform Carbon Disulfide Pyridine Formamide Benzyl Alcohol
11.90 > 20 18.10 18.80 10.7 2.15 >20 >20 0.100 > 20 > 20 > 20
GRAMlCIDlN
195
4.32
Solubility in Solutions of Quaternary Ammonium Compounds
A number of reports have indicated that tyrothricin is more soluble in solutions of quaternary ammonium compounds , O.
When it was realized that tyrothricin was a mixture of antibiotics,the same principle was applied to gramicidin6 I 6 2 64 6 5 . The addition of quaternary pounds to gramicidin formulations to increase the solubility of the antibiotic in aqueous solution has been utilized66,67. 4.33
Solubility in Solutions of Other Surface Active Agents
A number of other materials have been shown to increase the solubility of gramicidin in aqueous solution. Alcohols6’, ~ a n t h o c i l l i n ~fatty ~, acid amides’O, fatty acid alcohols71, aliphatic and polyvinylpyrrolidone73 # 74.
4.4
Physical Properties of Solutions 4.41
Diffusion
The diffusion constants for the gramicidin complex were determined in acetic acid and ethanol solut i ~ n ~ The ~ . molecular weight range of gramicidin was calculated as 2800-5000. Polson using a similar method obtained a molecular weight of 300076. 4.42
Surface Tension
Gramicidin decreases the surface tension of aqueous solution7’. The bactericidal and hemolytic properties of gramicidin were destroyed by heat but the surface tension depression was not changed. Kemp and coworkers found that when they partitioned gramicidin between water and heptane, it migrated to the walls of the vessel7’.
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4.43
Specific Volume
Derechin and coworkers noted the anomalous behavior of gramicidin A in absolute ethanolirg. The apparent partial specific volume increased with decreasing concentration of gramicidin. The same was not true for aqueousethanol solutions. 4.44
Conformation
The conformation of gramicidin in aqueous solution has been extensively studied. A lipophilic lefthanded helical structure has been proposed for gramicidin A401 41. It was proposed that the mode of action of gramicidin is due to the formation of ion transport channels across biological membranes. Bamberg and coworkers have studied the single channel conductance of gramicidins A, B and C8 Significant differences between gramicidin A and B were found I
.
.
Cabon 13 NMR has been used to confirm the presence of a double helical dimer modela2. The conformation of gramicidin in various 84 I 86. organic solvents has also been established"I I
I
Circular dichroism at high pressures has been used to study the conformation of a derivative of gramicidin A in trifluoroethanol solutionsa7. Kyogoku and Kawano have prepared an extensive review of the use of NMR techniques to study the conformation of gramicidin and other antibiotics in solutionaa. Lotz and coworkers have used poly (y-benzylD-L-glutamate) as a stereochemical model to study the conformation of gramicidin Aa9. 5.
Production 5.1
Fermentation
The gramicidin complex was originally isolated by Dubos as a component of the antibiotic mixture called tyrothricin formed by an aerobic sporulating bacillus'.
GRAMICIDIN
197
Dubos and Hotchkiss found that a number of species of aerobic sporulating bacilli produced gramicidin’ I
Stokes and Woodward established that Bacillus brevis produces the antibiotic in stationary cultures of both complex natural and synthetic mediag0. They noted that production of the antibiotic occurred in an aerated synthetic medium but not in an aerated complex nitrogenous medium. Konikova and coworkers compared the productivity of two strains of bacilli in the production of gramicidingl. Lewis and coworkers studied the production of the antibiotic complex by Bacillus brevis in both natural and complex mediag2. They noted requirements for calcium, magnesium and manganese ions. Stokes patented a submerged culture fermentation production procedure utilizing a synthetic medium6. Appleby and coworkers studied the addition of vitamins to synthetic mediumg3. Konikova and Dobbert studied the effect of the addition of amino acids to a synthetic medium on the production of tyrothricing4. They found that these additions had no effect on antibiotic production although growth was stimulated. Udalova and Fedorova have studied the effect of different carbon sources on the yield of antibioticg5. A number of workers have described the production of tyrothricin in a synthetic medium supplemented with organic nitrogen compounds96r97r98r99r100. Several investigators have attempted to establish the biosynthetic pathways for the production of tyrothric~n101,102,103,104~ Akers, Lee and Lipmann have isolated two enzymes from Bacillus brevis that are responsible for the synthesis of the initial portion of the g r a m i ~ i d i n s ~ ~ ~ . 5.2
Isolation
Hotchkiss and Dubos have utilized solvent extraction to separate gramicidin and tyrocidine’ 5. Several patents have been issued on procedures for isolating grami: cidin from fermentation brothlo6 ,lo7,lo8.
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Derivatives
5.3
Shepel and coworkers have reported the properties of analogs of gramicidin A with shorter peptide chainslog. It has been found that the treatment of gramicidin with formaldehyde results in the formation of a compound with the same antibiotic activity but with much less hemolytic activity110 1 1 1 112,113,114. Various esters of gramicidin have also been prepared’ 5, 6 , 7. Although these compounds have reduced hemolytic activity, they also possess less antibiotic activity.
’ ’’ ’
6.
Stability 6.1
Stability in Solution
Nitti and Nislo have shown that gramicidin is stable to autoclaving in aqueous solutionll8. Certain aqueous solutions were patented because they produced stable gramicidin solutions’
’.
Ishii and Witkop have found that treatment of gramicidin A with 1.5N_hydrochloric acid in absolute methanol for one hour at room temperature selectively cleaved one peptide bond120. 6.2
Effect of Light
The ultraviolet inactivation spectrum for gramicidin has been published by Setlow and Doyle’’’. Sugimoto and coworkers have presented infrared, ultraviolet, visible and ESR spectra for gramicidin solutions irradiated with various amounts of ultraviolet light122. 6.3
Stability of Formulations
Buckwalter has indicated that gramicidin solutions in propylene glycol and carbowaxes are stable to aut~claving’’~. He also showed that the antibiotic can be solubilized in water with the aid of non-ionic wetting agents.
GRAMICIDIN
7.
I99
Analytical Methods 7.1
Identity Tests
Brustier and coworkers utilized the AdamkiewiczHopkins-Cole reaction as an identity test for gra~nicidinl~~. The test detects the indole ring structure of the tryptophane residue. Fischbach and Levine described the use of Ehrlich’s reagent as an identity test for grami~idinl~~. They also utilized a modified biuret reaction125. Ramachandran reported on the reaction of hydrazine with gramicidin to yield formic hydrazide126. This product was detected by a color reaction. 7.2
Microbiological Assays
Microbiological assays are the primary assay method for antibiotics. They provide sensitive but nonselective methods. A variety of microbiological methods have been described for the assay of gramicidin. The official method in the United States is the turbidimetric method described in the Code of Federal regulation^^^^^ 128. 7.21
Dilution Methods
Dilution assays are generally utilized as early microbiological methods before well defined standards are available. They have the advantage that one can compare the activity of one preparation to another without having a standard. Reedy and Wolfson have described a tube dilution assay for gramicidin12’. A n agar dilution assay using Micrococcus lysodeikticus has been reported’30.
7.22
Dye Reduction Methods
The addition of a dye that is reduced by the growing microorganisms gives a microbiological assay a sharper end point.
GLENN A. BREWER
200
Prevot reported on Janus green reduction methods with a number of different organisms’ 1 32.
’
DeFelip and coworkers use sodium resazurin as a dye to give a rapid assay in three to six hours133. 7.23
Turbidimetric Assays
Ceriotti has reported a turbidimetric assay using Micrococcus lysodeikticus’34. Berridge and Barrett have reported an assay with Streptococcus agalactiae which can be read after 4 hour i n c u b x l - 3 - 5 7 Kaiser and Camboni reported a turbidimetric assay utilizing Staphylococcus aureusl 3 6 . Kramer and Kirschbaum have reported an assay with Streptococcus faecalis’37. Leclercq has described a nephelometric assay for gramicidin138,139. Pain and coworkers have reported a turbidimetric assay utilizing lactic acid bacteria140. Kreuzig has described a turbidimetric assay utilizing Streptococcus faecalisl41. 7.24
Agar Diffusion Assays
Since gramicidin is not very soluble in aqueous solution, relatively few agar diffusion assays have been reported. Ceriotti has reported an agar diffusion assay for gramicidin utilizing Micrococcus lysodeikticus’34. Miller, Matt and Ciminera reported an agar diffusion assay for grami~idinl~~. Raitio and Bonn used this method to assay pharmaceutical preparations 43. The Swiss Pharmacopeia utilizes an agar diffusion assay with Sarcina l ~ t e a l ~ ~ .
GRAMICIDIN
20 1
Viola and Canestrini reported on an agar well technique with Sarcina Kreuzig has studied the agar diffusion assay for tyrocidine in detail using gel chromatography as an analytical technique146. 7.25
Potentiation of Microbioloaical Assavs
Nisonger reported that the addition of hexadecylpyridinium chloride to gramicidin potentiates the activity found by microbiological assay’4 7 . Forni found that traces of cobalt chloride enhances the activity of gramicidin toward Escherichia & and Staphlococcus aureus’4 8 . Gillissen indicated that while cationic surfactants like cetylpyridinium chloride have a synergistic effect, Tween 80 inhibits the activity of gramicidin14’. This effect was confirmed by Barr and Ticel5O. Casilli and Ragni assayed gramicidin in the presence of cetrimide without interference using a cetrimide resistant strain of Staphlococcus aureus’ 51. 7.3
Chemical Assays 7.31
Colorimetric Assavs
Rittenberg and coworkers used a colorimetric assay for tryptophane to determine tyrothricin in fermentation broth’ 5 2 . Kreuzig described a semi-automated colorimetric assay for gramicidin utilizing the reaction of tryptophane with perchloric acid-butanol and ferric chloride 141,153.
Pate1 and Naravane have published an assay utilizing p-dimethylaminobenzaldehyde and nitrite’ 54. Ivashkiv has used this reaction to assay gramicidin and tyrocidine in fermentation broth’ 5 5 . The antibiotics are separated by a simple solvent partition. 7.32
Spectrophotometric Methods
Oberzill has described a spectrophotometric assay for gramicidinl 56. Thombs and coworkers have used the
GLENN A. BREWER
202
absorbance of the peptide bond at 210 nm to measure gramicidin157. 7.33
Miscellaneous Methods
White and Secor have measured gramicidin by measuring the Kjeldahl nitrogen’58. 7.4
Electrochemical Methods
Kramarczyk and Berg have described an indirect polarographic assay for gramicidinl597.5
Hemolytic Methods
As has been mentioned previously, gramicidin has limited utility as an antibiotic because of its hemolytic activity (Section 1.0). Various workers have utilized the hemolytic property of the antibiotic as an assay tool. The hemolytic activity of gramicidin is probably due to its ability to form ion conducting channels in the membranes of red blood cells. The loss of isotonicity causes the cells to rupture.
Heilman and Herrell reported the first use of the hemolytic assay to the assay of gramicidin’60. Mann and coworkers compared the hemolytic activity of gramicidin and tyrocidine161. They reported that the addition of serum inhibits the hemolytic activity of gramicidin. Dimick reported that the hemolytic assay can be used to measure the concentration of antibiotic in fermentation broth162. Other authors have reported on modified hemolytic r n e t h o d ~ ~ ~ ~ , ’ ~ ~ , ’ ~ ~ . 7.6
Enzymatic and Other Biochemical Methods
Many antibiotics have been found to have inhibitory activity on enzyme systems. This inhibition can be utilized as the basis of an assay system. Creaser reported that Staphlococcus aureus forms an inducible 8-galactosidasel66, The production of this enzyme is inhibited by the addition of gramicidin. Strictly speaking, gramicidin does not inhibit the enzyme directly but this method could be used as the basis of a sensitive assay method
.
GRAMICIDIN
203
Gramicidin was found to uncouple the phosphorylation of ADP from the enzymatic reduction of ferricytochrome
c167,168,169,170,171,172,173,174~175~
Hinkson reported that gramicidin inhibited the photoreduction of NAD by photosynthetic bacterial 76. 7.7
Chromatographic Methods 7.71
Counter Current Distribution
Gramicidin was first shown to be heterogeneous by counter current distribution23 . A water-methanolchloroform-benzene (7:23:15:15) system was used to show the presence of two components. Craig later showed that gramicidin contained three crystalline components177. Stamm discussed the application of counter current distribution to the separation of gramicidins 78. Ramachandran showed that there were at least four components in gramicidin and gave the fourth component the name gramicidin D33. Goss and Witkop separated each of gramicidins A,B and C into a pair of congeners and identified the major congener as valine- ramicidin and the minor component as isoleucine-gramicidin3 7
.
Okamoto and coworkers showed that gramicidin could be separated into three fractions (A, B and C) using droplet counter current distribution’79. 7.72
Paper Chromatography
Snell, Ijichi and Lewis published a series of paper chromatographic systems capable of separating various antibiotics including gramicidinl Detection was by bioautography. Forni and Cavalli used the following systems on Whatman No. 1 paper to distinguish between bacterial peptide antibioticslS1. t-Butanol-Acetic Acid-Water (74:3:25) n-Butanol-Acetic Acid-Water (79:6:15) Acetone-Water (70:30) + Ammonia t-Butanol-Water (80:20)
+
Ammonia
GLFNN A. BREWER
204
Cunha and Baptista found that a butanolacetic acid-water (50:25:25) system using Schleicher and Schull 2043a paper buffered to pH 3.0 gave the best separation of peptide antibiotics182. The same authors utilized salting out chromatography to separate gramicidin and tyrothri~inl~~. Singh utilized anionic dyes to detect gramicidin on paper chr~matogramsl~~. Paris and Theallet described three paper chromatographic systems for gramicidin185. Mtschel and Lercher described two solvent systems for antibiotics186. The solvent systems were butanolpyridine-acetic acid-water (15:10:3:12) and water saturated butanol-water saturated ethyl ether-acetic acid (5:l:l) on Schleicher and Schull 204333 paper. The antibiotics were visualized by ninhydrin. DeFranca and coworkers described a system of 25 ml 9:l acetone-water, 5 ml chloroform, 2 ml ethylene glycol and 1 ml of ~ y r i d i n e l ~ ~They . claim the method is as accurate as the microbiological assay. 7.73
Thin Layer Chromatography
Nussbaumer utilized a solvent system of butanol-acetic acid-water (10:1:3 ) on acid Silica gel G1 Pitton described the following five thin layer systems for several antibiotics including gramicidinl
*’.
Water-Methanol-Butanol-Butyl Acetate-Acetic Acid (12:2.5:7.5:40:20) Water-Butanol-Pyridine-Acetic Acid (14:30:20:6) Water-Butanol-Pyridine-Acetic Acid (16:40:8:16)
Water-Butanol-Acetic Acid (39:55:6) Aqueous phase of Methanol-Ammonia-Chloroform (10:10:20) Guven and Ozsari reported some thin layer systems to use as identity tests for antibiotics including gramicidinl’ O . McGilveray and Stickland described two thin layer chromatographic systems to use to identify several antibiotics including gramicidinl l. Nekola published a thin layer chromatographic assay for gramicidin in fermentation brothlg2. The
205
GRAMICIDIN
broth was adjusted to pH 4.5 with HC1 and the antibiotics precipitated. The residue was dissolved in methanol and purified on an alumina column. The eluate was chromatographed on silica gel using water-methanol-butanol-butyl acetate-acetic acid (24:5:15:80). The absorbance of the gramicidin spot was then determined. Kreuzig reported a high performance TLC method for gramicidin in fermentation broth1 94. A Kieselgel 60 plate is developed with acetic acid-butyl acetate-butanolmethanol-water (40:80:15:5:12). The gramicidin spot was visualized by spraying with ethanolic 4-dimethylaminobenzaldehyde-HC1 and quantitated by scanning at 570 nm. 7.74
Electrophoresis
Cunha and Baptista reported an electrophoresis method to determine gramicidin in pharmaceutical preparations 9 5 . Paris and Theallet have described two Cunha and paper electrophoresis systems for gramicidin18’. Gomes have published paper electrophoresis methods for various peptide antibiotics196. Lightbown and DeRossi utilized agar electrophoresis to identify various antibiotics including gramicidinl97. 7.75
Column Chromatography
Moses has patented a process for the separaThe 80% aqueous tion of gramicidin from tyrothricin1 methanol solution is passed through a cation ion exchange resin in the hydrogen cycle followed by an anion resin in the hydroxyl cycle. Bartley and coworkers separated gramicidin from tyrocidine using Sephadex W 2 O 1 99. 7.76
High Performance Liquid Chromatography
Axelsen and Vogelsang have reported the separation of gramicidins A, B and C by HPLC using Zorbax ODS (5 pm) eluted at 6OoC with methanol-5 mM ammonium sulfate (37:13)200.
GLENN A. BREWER
206
8.
Reviews
A lar e number of general reviews have been written on gramicidin2?1, 202,20 3,204,205,206,207, 2 08 209 21 0,2 1 1 1 212121 3
214,215,216,217,218,219,220,221,222~
These reviews cover the chemical properties, biological properties and medical use of gramicidin.
A review on the analytical methods for gramicidin and other antibiotics has been prepared by Brewer and Platt224.
207
GRAMICIDIN
References 1. 2.
3. 4. 5. 6.
Dubos, R. J.; J. Exper. Med. 7 0 , 1 (1939) (C. -A. 33 69027 (1939)) . Fleming, A.; Brit. J. exp. Path. 10, 226 (1929) (C. A. 23 4961 (1929)). -Hussar, A. E. and Halley, H. L.; Antibiotics and Antibiotic Therapy, pages 174 and 175, Macmillian Co., N.Y. 1954.
Veatch, W. R., Fossel, E. T. and Blout, E. R.; Biochemistry 13, 5249-56 (1974); (G. 82 69437h (1975)) D u b o s , R. and Cattaneo, C. ; J. Exp. Med. 70, 249 (1939) ~.(C. _1 .. - A.-33 86787 (1939) 40 Stokes, J. L. ; U . S . Pat. 2,406,174 (1946); (G. -
.
65634 (1946))
7. 8. 9. 10. 11.
12. 13. 14. 15. 16. 17. 18. 19. 20.
.
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180. Snell, N.; Ijichi, K. and Lewis, J. C.; Appl. Micro- A. -50 5086d (1956)). biol. - 4, 13-17 (1956) (C. 181. Forni, P. V . and Cavalli, F.; Minerva med. 4545 (1958) (C. - A. -53 7306g (1959)). 182. daCunha, A. P. and Baptista, M. L. D. M.; Bol. escola farm.,Univ. Coimbra 19-20, 225-30 (1959-60) (G. 55 19136e (1961)). 183. daCunha, A. P. and Baptista, M. L. D. M.; Bol. escola farm., Univ. Coimbra 19-20, 217-24 (1959-60) (G. 55 21481g (1961)). 184. Singh, C.; Cesk. Farm. 12, 294-7 (1963) (C. - A. 61 2906b (1961)) . 185.
Paris, R. R. and Theallet, J. P.; Ann. Pharm. Franc. (G. 57 16746i (1962)) . Ritschel, W. A . and Lercher, H.; Pharm. Ztg. Ver. Apotheker-Ztg.106, 120-2 (1961) (C. A. 62 397h (1965)). DeFranca, F. P.; Rosemberg, J. A. and DeJesus, A. M.; Rev. Brasil. Farm. 50, 343-6 (1969) (C. - A. -73 28952t (1970)1 . Nussbaumer, P. A.; Pharm. Acta Helv. 2, 647-52 (1964) (C. - A. -62 3886e (1965)). Pitton, J. S.; Antibiot., Advan. Res., Prod. Clin. Use, Proc. Congr., Prague 490-5 (1964) (C. - A. -66 40743p (1967)). Guven, K. C. and Ozsari, G.; Eczacilik BuL. 9, 19-29 (1967) (C. - A. -68 71008c (1968)). McGilveray, I. J. and Strickland, R. D.; J. Pharm. Sci. -56, 77-79 (1967) (G. 66 40746s (1967)). Nekola, M.; 2. analyt. Chem. 268, 272-274 (1974) (C. .. - A. -81 103174m (19741). Kreuzig, F.; Fresenius' Z. anal. Chem. 282, 447-449 (1976) 86 60589j (1977)). 142, 441-447 (1977) (G. Kreuzig, F.; J. Chromatogr. 88 11966h (1978) ) . daCunha, A. P. and Baptista, M. L. D. M.; Bol. escola. A. farm., Univ. Coimbra 19-20, 331-40 (1959-60) (C. 55 19136i (1961)). -
20, 436-42 (1962) 186. 187.
188. 189.
190. 191. 192. 193. 194. 195.
(e.
2 I7
GRAMICIDIN
196.
daCunha, 0. R. P. and Gomes, M. E. B.; Bol. Escola Farm., Univ. Coimbra Ed. Cient. 22, 129-36 (1962) (C. - A. -61 1711d (1964)).
197.
Lightbown, J. W. and DeRossi, P.; Analyst (1965) (C. A. 62 1 1 6 3 0 ~(1965)).
3, 89-98
198. Moses, W.; U. S. Pat. 2,992,164 July 11, 1961 (C. A. 55 22721a (1961)). 199 *
Bartley, I. M.; Hodqson, B.; Walker, J. S.; Holme, G.; Biochem. J. 127, 489-502 (1972) (C. - A. -77 58417x (1972)) .
200.
Axelsen, K. S. and Vogelsang, S. H.; J. Chromatogr. 140, 174-78 (1977) (Anal. Abst. 34 5E31 (1978)).
201.
Dubos, R. J.; J. Pediatrics
2, 588-95
(1941)
(G.
40 376(5) (1946)). 202.
Lions, F.; Australian J. Sci. 6, 46-8 (1943) (C. A. -
38 21658 (1944)). -
16,215-19
203.
Gauze, G. F.; Advances in Modern Biol. (1943) (C . A. -38 138(5) (1944)).
204.
Hotchkiss, R. D.; Advances in Enzymology (1944) (G. 38 4623(6) (1944)).
205 -
A, 153-99
Petersen, H. K. J. and Vermehren, E.; Arch. Pharm. Chem. (G. 41 6306b (1947)) .
51, 109-28, 161-94 (1944)
206.
Hoogerheide, J. C.; Botan. Rev. 10, 599-638 (1944) 2 4913 (5) (1945))
207.
Bergol'ts, M. K h . ; 43 5551c (1949)). -
208.
Broch, P. J. F. and Jacob, F.; Farmatsiya 139-40 (1944) (C. A. 43 5826e (1949)). -Filho, A. R.; Rev. brasil. farm. 27, 335-61 (1946) (C. - A. -41 4193d (1947)).
209. 210.
(e.
.
Farmatsiya
z,35-8
(1944) (C. A.
I,
Massey, F. C.; Penna. Med. J.
49,
1090-4 (1946) (C. A.
43 3061a (1949)).
211. 212.
Rivoal, G.; Rev. sci. 3881d (1949)) .
86, 369-76
(1948)
(e. 43
Postovskil, I. Ya. and Bednyaqina, N. P.; Uspekhi Khim. 16, 3-28 (1947) (C. - A. -41 5578a (1947)).
213.
Macheboeuf, M.; Actualit& (C. - A. -47 5026d (1953)).
pharmacol.
214.
Werner, G.; Scientia Pharm. 45 10510a (1951)).
2,
19, 95-103
111-22 (1950)
(1951)
(G.
GLENN A . BREWER
218
215. 216.
Macheboeuf, M. and Gros, F.; Expos& ann. biochim. m6d. 12, 141-60 (1951) (C. - A. -46 8716e (1952)). - Tr6foue1, J.; Cheymol, J.; Nau, A.; Paul, R.; Pgnau, H.; Hagemann; Romain, R.; Ziegl6, M.; Vignalou, J. and Quevauviller, A.; The'rapie 2, 961-1029 (1956) (C. - A. -52 20665d (1958)).
Brunner, R.; Osterr. Apotheker Ztg. 11,455-60, 477-9 (1957) 52 57489 (1958)). 218. Baker, W. B.; Drug & Cosmetic Ind. 87,172-3, 258-62 (1960) 54 25568h (1960)). 219. Schumacher, E.; Schweiz. Arch. Tierheilk. 104, 350-60 (1962) (C. - A. -57 11307b (1962)). 220. DeLogu, I.; Corriere Farm. 21, 419-20 (1966) (C. A. 66 102608j (1967)). 221. Bogentoft, C.; Farm. Revy 67,749-51 (1968)( C. 70. 80793u (1969)1 . 217.
(u. (s.
222.
Hladky, S. B.; Drugs Transp. Processes Symp. 193-210 (1973) 82 149063~(1975)) .
223.
AkerS, H. A.; Lee, S. G. and Lipmann, F.; Biochemistry 16, 5722-9 (1977) (G. 88 17964p (1978))
224.
Brewer, G. A. and Platt, T. B.;Encyclopedia of Industrial Chemical Analysis Volume 5 pages 460-633 published by John Wiley & Sons, N.Y. 1967.
(u.
.
Analytical Profiles of Drug Substances, 8
GRISEOFULVIN Ecl~1at-dR . Tou1nley 1.
? -.
3. 4. 5. 6.
7.
8 9 I0
Description I . I Name, Formula. Molecular Weight I .2 Appearance, Color. Odor I . 3 Compendia1 References. Other Physical Properties 2.01 Circular Dichroisni 2.02 Nuclear Magnetic Resonance 2.03 Mass Spectrum 2.04 Ultraviolet Spectrum 2.05 Infrared Spectrum 2.06 X-Ray Diffraction 2.07 Fluorescence and Luminescence 2.08 Photolysis 2.09 Optical Rotation 2.10 Melting Range 2.11 Differential Scanning Calorimetry 2.12 Thermogravimetry 2.13 Electrophoretic Properties 2. I4 Solubilitv Production and Synthesis Impurities Stahility Drug Metabolic Products Methods of Analysis 7.01 Identification 7.02 Elemental Analysis 7.03 Spectrophotometric Analysis 7.04 Spectrofluorometric Analysis 7.05 Colorimetric Analysis 7.06 lodometric Analysis 7.07 Turbidimetric Analysis 7.08 Polarographic Analysis. 7.09 Chromatographic Analysis 7.091 Partition Column Chromatography 7.092 Paper Chromatography 7.093 Thin-Layer Chromatography 7.094 Gas chromatography 7.095 High Performance Liquid Chromatography 7.10 Biological Methods of Analysis Identification and Determination in Body Fluids Analysis of Dosage Forms Acknowledgments 219
Copyright 0 1979 by Academic Press. Inc. All rigtits of reproduction in any form reserved. ISBN 0-12-260808-9
EDWARD R. TOWNLEY
220
1.
Description 1.1 Name, Formula, Molecular Weight
Chemical Names (2S-trans)-7-Chloro-2',4,6-trimethoxy-6'-methylspiro [benxofuran-2(3H), 1'-(2) cyclohexene]3,4'-dione 7-chloro-4,6-dimethoxycoumaran-3-one-2-spir0-1'-(2~me thoxy-6'-me thylcyclohex-2'-en-4 '-one)
Generic Names Griseofulvin Trade Names Fulcin; Fulvicin UfF, Fulvicin PIG, Grifulvin; Grisactin; Grisovin, Gris-PEG, Grysio, Lamoryl, Likuden, NeoFulcin, Poncyl; Spirofulvin; Sporostatin. Formula and Molecular Weight
OCH
CH 0 3
c1
1' 7H17 ' 1 ° 6 1.2
CH
3
Molecular Weight
352.77
Appearance, Color, Odor Griseofulvin is a white, odorless, crystalline pow-
der. 1.3
Cornpendial References, Other Griseofulvin is listed in the following compendia: The United States Pharmacopia (1) The British Pharmacoepia (2) The Europeon Pharmacoepia ( 3 ) and the Merck Index (4). A previously published review (5) is a good source for physical and chemical data, production, use, occurrence and biological information.
GRISEOFULVIN
22 I
Physical Properties P h y s i c a l measurements by S c h e r i n g C o r p o r a t i o n are provided f o r Batch Number UGFP-1961. T h i s b a t c h i s chromatographic a l l y p u r e w i t h t h e e x c e p t i o n of 1.1% d e c h l o r o g r i s e o f u l v i n . 2.
2.01
C i r c u l a r Dichroism S p e c t r a The c i r c u l a r d i c h r o i s m s p e c t r a ( F i g u r e 1) w a s obt a i n e d on a 0.0155 mg/ml s o l u t i o n i n methanol w i t h a Cary Model 61 C i r c u l a r Dichroism Spectrophotometer. The f o l l o w i n g molar e l l i p t i c i t y v a l u e s were o b t a i n e d : Table I Molar E l l i pt i c it y
Wavelength nm 345 326 314 294 236 218
PI
+ + + +
shoulder shoulder shoulder peak peak peak
7,520 19,100 23,200 43,700
+110,000
- 97,500
2.02
Nuclear Magnetic Resonance S p e c t r a The p r o t o n NMR spectrum of g r i s e o f u l v i n ( F i g u r e 2) w a s o b t a i n e d i n DMSO-d s o l u t i o n (conc. w/v = 10 mg/0.40 m l ) c o n t a i n i n g TMS as k t e r n a l r e f e r e n c e u t i l i z i n g t h e V a r i a n A s s o c i a t e s CFT-20 S p e c t r o m e t e r o p e r a t i n g a t a frequency of 79.5 MHz. The chemical s h i f t s ( 6 , ppm) are w i t h r e f e r e n c e t o TMS. The e x p e r i m e n t a l c o n d i t i o n s a r e : Sweep w i d t h Pulse width Acquisition t i m e Data t a b l e
= = = =
800 Hz 6.0 1.1 sec ( 25'tip) 5.1 s e c 8K
E D W A R D R. T O W N L E Y
222
1
li
200
FIGURE 1 :
250
300
WAVELENGTH [nm]
350
Circular Dichroism Spectra of Griseofulvin
400
224
EDWARD R. T O W N L E Y
T a b l e I1 Proton
Chemical S h i f t s ( 6 , ppm)
6 '-CH3
0.82
5'-CH 6 '-CH 21
2.3-2.9
m
(3H)
2'-OCH3
3.63
8
(3H)
3.96 4.04
S
4-0CH3 } 6-OCH3
Aromatic
d ( J x 6 . 5 Hz)
(3H)
8
3 '-H 5-€I d= d o u b l e t , s= s i n g l e t , m- m u l t i p l e t . The carbon-13 NMR s p e c t r u m of g r i s e o f u l v i n ( F i g u r e 3 ) w a s o b t a i n e d a t am bi ent t e m p e r a t u r e i n DMSO-d 6 c o n t a i n i n g TMS a s i n t e r n a l r e f e r e n c e u t i l i z i n g V a r i a n A ssoci a t e s XL-100-15 s p e c t r o m e t e r equi pped w i t h F o u r i e r a c c e s s o ries. The s y s t e m was l o c k e d t o t h e d e u t e r i u m r e s o n a n c e f r e quency o f t h e s o l v e n t , and o p e r a t e d a t a f r e q u e n c y of 25.2 MHz f o r carbon-13. The chem i cal s h i f t s are r e p o r t e d ( c , ppm.) from t h e i n t e r n a l s t a n d a r d TMS.
-
Sweep w i d t h Pulse width Acquisition t i m e Acquisition delay
= 5500 Hz
15 P sec (66'
tip)
= 1.6 sec = 0.20 sec
T a b l e 111 Carbon
Chemical S h i f t (6,)
1' 2' 3'
4' 5' 6' 6' CH 4' ocd, 2' OCH3
90.11 170.22 104.60 195.45 39.49 35.52 13.77 57.54 56.97
Carbon 6 OCH3 3 3a 4 5 6 7 7a
Chemical S h i f t ( 56.52 191.12 104 04 157.59 91.27 164.44 95.24 168.57
6,)
A
I
I
I
1
I
I
I 1
I
I 1
I
m
,
I
I
I
I
I
I
I
1
I
I
I
I
I
I
I
#
I
I
I
%
m I
FIGURE 3:
I
I
I
I
I
I
1,
1
I "
' I '
I
I
I
I
I
,
I
Carbon 1 3 , Nuclear Magnetic Resonance Spectra of Griseofulvin i n DMSO d6
I
I
I
,
*,
~
226
EDWARD R. T O W N L E Y
The spectrum is in substantial agreement with the data reported by Wenkert et. al, (6). However, on the basis the proton coupled carbon 13 N M R spectra, the assignments for 6 and 7ci are reversed [Brambilla (16)] from those previously reported. The new assignments are based on long range H-C-0-C couplings. 2.03
Mass Spectrum The medium resolution, electron-impact mass spectrum of griseofulvin (Figure 4) was run on a Varian-Mat CH-5 Mass Spectrometer. Instrumental conditions were; Electron Energy 70eV; Source Temperature 25OoC; Sample Probe Temperature 14OoC. The fragmentation ions, given below, are consistent with the griseofulvin structure. Table IV Mass (amu)
Ions
Losses
352 337 321 310 284
CH30 CH3 CH CO Me6=CHCO
OCH
l+
215
138
I+
-t
k
i-
U
a
al
[I)
vl
[I)
9
.. U
F
s8
EDWARD R. TOWNLEY
228
I+ 123
2.04
U l t r a v i o l e t Spectrum The u l t r a v i o l e t spegtrum of g r i s e o f u l v i n i n anhyd r o u s methanol s o l u t i o n a t 25 C gave t h e f o l l o w i n g absorpt i v i t y values Wavelength maximum i s a t 324 nm; a = 15.5 Wavelength maximum i s a t 291 nm; a = 68.3 Wavelength maximum i s a t 235 nm; a = 64.0 The u l t r a v i o l e t spectrum i s shown i n F i g u r e 5.
2.05
I n f r a r e d Spectrum The i n f r a r e d spectrum of g r i s e o f u l v i n , o b t a i n e d as a m i n e r a l o i l m u l l , was r u n on a Perkin-Elmer Model 180 g r a t i n g Important a b s o r p t i o n assignments are I R spectrophotometer. given i n Table V. The spectrum i s g i v e n i n F i g u r e 6. Table V
-1
Wavenumber (cm
1
1703 ( s ) 1658 ( s ) 1615, 1597, 1580 ( s ) 1501 (m) 1220, 1210 ( 8 )
Assignment C=O s t r e t c h ; benzofuranone r i n g carbonyl C-0 s t r e t c h ; cyclohexenone c a r b o n y l C=C s t r e t c h , a r o m a t i c and c y c l i c unsaturation C=C s t r e t c h , a r o m a t i c C-0 s t r e t c h , a r y l methoxyl
I nt e n s i t y s
- strong
m
medium
-
2.06
X-ray D i f f r a c t i o n The X-ray d i f f r a c t i o n p a t t e r n of g r i s e o f u l v i n w a s o b t a i n e d on a P h i l l i p s ADP-3500 X-ray D i f f r a c t o m e t e r u s i n g Cu K, r a d i a t i o n (1.5405A0) and N i f i l t e r . The d a t a is g i v e n i n Table VI.
GRISEOFULVIN
2.06
229
X-Ray Powder D i f f r a c t i o n P a t t e r n of G r i s e o f u l v i n Table V I
20 4 009 4.117 10.679 13.123 13.844 14.497 16.422 17.669 19.194 19.625 20.184 21.562 21.986 22.462 23.765 24.067 24.295 25.780 26.567 28.418 29.835 31.104 31.185 31.385 32.624 32.674 34.852 34.914 35.896 36.142 36 202 36.290 37.077 37.270 38.500 38.569 38.659
d(Ao)* 22.038 21.460 8.284 6.746 6.397 6.110 5.398 5.020 4.624 4.523 4.399 4.121 4.043 3.958 3.744 3.698 3.663 3.456 3.355 3.141 2.995 2.875 2.868 2.850 2.745 2.741 2.574 2.570 2.502 2.485 2.481 2.475 2.425 2.413 2.338 2.334 2.329
I/I'** 18 14 46 48 8 59 100 7 30 16 24 34 23 45 72 10 13 26 87 57 29 20 19 24 14 14 12 11 18 14 15 14 14 13 18 18 19
*d ( i n t e r p l a n a r d i s t a n c e ) = n / 2 s i n 0 = r e l a t i v e i n t e n s i t y (based on t h e h i g h e s t i n t e n s i t y of 100)
**Ill'
230
EDWARD R. T O W N L E Y
WAVELENGTH [nm] FIGURE 5:
U l t r a v i o l e t Spectrum of G r i s e o f u l v i n Obtained i n Anhydrous Methanol Solvent
2.5
4600
FIGURE 6:
3
3500
4
3000
2500
WAVELENGTH 5 6
2000
MICRONS 8 9 10
7
1700 1400 FREQUENCY (CM’)
1100
12 14
18 22
800
500
Infrared Spectrum of Griseofulvin Obtained a s a Mineral O i l Mull.
3550
205
EDWARD R. TOWNLEY
232
2.07
Fluorescence and Luminescence Griseof u l v i n e x h i b i t s b o t h f l u o r e s c e n c e and luminescence. A r e p o r t by Neely e t al., ( 7 ) g i v e s c o r r e c t e d f l u o r e s c e n c e e x c i t a t i o n (max. 295 nm) and e m i s s i o n (max. 420 nm) s p e c t r a , v a l u e s f o r quantum e f f i c i e n c y of f l u o r e s c e n c e (0.108) c a l c u l a t e d f l u o r e s c e n c e l i f e t i m e (0.663 n s e c ) and phosphorescence decay t i m e (0.11 s e c . ) . The f l u o r e s c e n c e e x c i t a t i o n and emission s p e c t r a a r e g i v e n i n F i g u r e 7. 2.08
Photolysis There i s no change i n t h e t h i n l a y e r chromatogram (single spot) o r i n the fluorescence o r u l t r a v i o l e t spectra a f t e r i r r a d i a t i o n i n methanol w i t h a xenon lamp f o r 20 hours. It is t h e r e f o r e concluded t h a t t h e r e is no s i g n i f i c a n t photod e g r a d a t i o n of g r i s e o f u l v i n under r e a s o n a b l e c o n d i t i o n s of l i g h t exposure ( 7 ) . 2.09
O p t i c a l Rotation
Griseofulvin e x h i b i t s the following o p t i c a l r o t a t i o n when d i s s o l v e d i n t h e s e s o l v e n t s . Table V I I [a]
k7'=
+370
4
Dimethylformamide
[a]:60=
+358
17
Dioxane
[a]:60=
+302
17
S a t u r a t e d chloroform Acetone
2.10
M e l t i n g Range The D i f f e r e n t i a l Thermal Gravimetry c u r v e ( F i g u r e 9 ) demonstrates t h a t t h e g r i s e o f u l v i n m e l t i n g p o i n t t a k e s p l a c e with decomposition. The m e l t i n g range of g r i s e o f u l v i n from s e v e r a l s o u r c e s i s g i v e n i n Table VIII. Table V I I I Me1t i n g Range 0 C
-
218 t o 224 2 20 218 217-224
Reference 3 4 17 51
GRISEOFULVIN
233
8C 7c
60
50 >
I-
w 40 k
z -
30
20 10
0 200 FIGURE 7:
300
400 WAVELENGTH
500
Corrected Fluorescence and Emission Spectra of Griseofulvin: la, Excitation Spectrum with Emission at 420 nm; l b , Emission Spectrum with Excitation at 295 nm.
EDWARD R. TOWNLEY
234
2.11
D i f f e r e n t i a l Scanning C a l o r i m e t r y F i g u r e 8 shows t h e DSC thermogram of g r i s e o f u l v i n o b t a i n e d w i t h a DuPont Model 900 Thermal Analyzer. A single s h a r p m e l t i n g endokherm o c c u r s f o r t h i s s u b s t a n c e w i t h o n s e t t e m p e r a t u r e a t 216 C.
2.12
Thermogravimetry F i g u r e 9 shows t h e TG thermogram of g r i s e o f u l v i n o b t a i n e d w i t h a DuPont Model 950 Thermogravimetric Analyzer. The thermogram shows no weight l o s s from ambient t o about 2OO0C followed by weight loss due t o s u b l i m a t i o n . 2.13
Electrophoretic Properties Zeta p o t e n t i a l s of d i s p e r s e d g r i s e o f u l v i n have been s t u d i e d b o t h a l o n e , and i n t h e p r e s e n c e of s u r f a c e - a c t i v e a g e n t s , t h e l a t t e r a t a c o n t r o l l e d pH ( 8 ) . A M o b i l i t y / Z e t a P o t e n t i a l pH p l o t of = +25mV g r i s e o f u l v i n , shows a p o s i t i v e c h a r g e a t pH 1 . 5 which r a p i d l y d e c r e a s e s t o z e r o a t pH 2 . 4 . There i s t h e n r e v e r s a l of c h a r g e followed by a n i n c r e a s e o v e r t h e pH r a n g e 2 . 4 t o 7 . 0 . The z e t a p o t e n t i a l a t t h e l a t t e r pH i s -45 mV. The p o t e n t i a l t h e n s t a y s c o n s t a n t o v e r t h e pH range 7 t o 10.
2.14
Solubility The f o l l g w i n g d a t a are g i v e n f o r t h e s o l u b i l i t y of g r i s e o f u l v i n a t 25 C ; a c e t o n e 30 g/L, carbon t e t r a c h l o r i d e 2 g/L, d i c h l o r o e t h a n e 80 g/L, dimethylacetamide, 40 g/L, dioxane 30 g/L, e t h y l e t h e r 0 . 7 g/L, h e p t a n e 0.3 g/L, methanol 0 . 4 g/L; m i n e r a l o i l (0.1 g/L; propylene g l y c o l 2 g/L; Span 80 0.2 g/L, Tween 80, 7 g/L water 0 . 2 g/L ( 1 7 ) .
3.
P r o d u c t i o n and S y n t h e s i s Griseof u l v i n is b i o s y n t h e t i c a l l y manufactured by e l a b o r a t i o n w i t h P e n i c i l l i u m griseofulvum and r e l a t e d s t r a i n s of Penicillia. The b i o s y n t h e s i s h a s been t h e s u b j e c t of numerous chemical and b i o l o g i c a l s t u d i e s , t h e l a t e s t of which is g i v e n by Harris, e t . a l . ( 9 ) F i g u r e 10. Other proposed b i o s y n t h e t i c pathways a r e d i s c u s s e d . G r i s e o f u l v i n was f i r s t i s o l a t e d i n 1938 by Oxford ( 1 0 ) (1939); i t s t o t a l s y n t h e s i s was accomplished i n 1960 and f o l l o w i n g y e a r s i n s e v e r a l l a b o r a t o r i e s ( B r o s s i e t a l . , 1960 ( 1 1 ) Grove, 1963; ( 1 2 ) Mutant s t r a i n s of P. patulum are used f o r t h e commercial p r o d u c t i o n of t h e a n t i b i o t i c by f e r mentation (9).
et. al.,
4.
Impurities Some f e r m e n t e r b r o t h i m p u r i t i e s have been l i s t e d by Holbrook, B a i l e y and B a i l e y (13) and r e p e a t e d i n a d e s c r i p t i o n
FIGURE 8:
Differential Scanning Calorimetry Curve of Griseofulvin
20
0
\ 50
100 T. 'C
FIGURE 9 :
200 250 300 350 150 (CORRECTED FOR CHROMEL ALUMEL THERMOCOUPLES)
Thermogravimetry Curve of Griseofulvin
400
450
500
237
GRISEOFULVIN
acetate
-
0
0
0
0
-
CHJO
a
0
0
OH
-
FIGURE 10:
0
I CHJ
OH H,C
a
I
CHJ
A Biosynthetic Route f o r G r i s e o f ulvin.
EDWARD R. TOWNLEY
238
of e f f i c i e n t l i q u i d chromatographic s e p a r a t i o n systems by B a i l e y and B r i t t a i n ( 1 4 ) and i n a g a s chromatographic s e p a r a t i o n system by Margosis ( 1 5 ) . S t r u c t u r e s are i n F i g u r e 11. The common i m p u r i t y found i n commercial b a t c h e s of g r i s e o f u l v i n is d e c h l o r o g r i s e o f u l v i n ( 1 4 , 1 5 ) which a p p e a r s t o b e i n t h e range of 0.5 t o 3 . 5 % .
5.
Stability G r i s e o f u l v i n is a s t a b l e drug s u b s t a n c e . After 1 2 y e a r s s t o r a g e a t room t e m p e r a t u r e no decomposition was d e t e c t e d by d i f f e r e n t i a t i n g LC methods (16). There is no p h o t o d e g r a d a t i o n under r e a s o n a b l e c o n d i t i o n s of l i g h t exposure ( 7 ) . G r i s e o f u l v i n is c o n v e r t e d t o g r i s e o f u l v i c a c i d under a c i d i c c o n d i t i o n s . 6.
Drug Metabolic P r o d u c t s The major human m e t a b o l i t e of g r i s e o f u l v i n i s 6-demethylg r i s e o f u l v i n and i t s g l u c u r o n i d e ( 1 7 , l B ) which a c c o u n t f o r about 65% of t h e i n t r a v e n o u s d o s e ( 1 9 ) and 3 5 t o 65% of t h e o r a l dose ( 2 0 , 2 1 ) . The 6 - d e m e t h y l g r i s e o f u l v i n is a l s o t h e major m e t a b o l i t e i n dogs ( 2 2 ) and r a b b i t s ( 2 3 ) w h i l e b o t h 4d e m e t h y l g r i s e o f u l v i n and 6 - d e m e t h y l g r i s e o f u l v i n are major m e t a b o l i t e s i n r a t s ( 2 4 ) and mice ( 2 5 ) . These m e t a b o l i t e s can b e determined by g a s l i q u i d chromatography v i a i s o p r o poxyl d e r i v a t i v e s ( 1 8 ) o r t r i m e t h y l s i l y l e t h e r d e r i v a t i v e s ( 2 6 , 2 7 ) . The 6-demethylgriseofulvin h a s been measured i n u r i n e by h i g h performance l i q u i d chromatography ( 2 8 ) and u l t r a v i o l e t spectrophotometry ( 1 9 ) . Only t r a c e amounts of g r i s e o f u l v i n are found i n t h e u r i n e ( 2 8 ) .
7.
Methods of A n a l y s i s
7.01
Identification A wine r e d c o l o r is produced when about 5 mg of g r i s e o f u l v i n are d i s s o l v e d i n 1 m l of s u l f u r i c a c i d w i t h about 5 mg of powdered potassium dichromate ( 2 9 ) .
7.02
Elemental A n a l y s i s A n a l y s i s of g r i s e o f u l v i n , w a s determined f o r c a r b o n , hydrogen, and c h l o r i n e . The carbon, and hydrogen a n a l y s i s w a s performed on a P e r k i n . E l m e r Model 240 i n s t r u m e n t . A n a l y s i s f o r c h l o r i n e w a s performed by combustion of t h e sample and c o u l o m e t r i c t i t r a t i o n u s i n g a n American I n s t r u m e n t Co. Chloride T i t r a t o r . The r e s u l t s from t h e e l e m e n t a l a n a l y s i s are l i s t e d i n
Table I X .
239
GRISEOFULVIN
0 I1
C
0 0
CH03
0
CH 3
-- 0
Dechlorgr i seo fulvin
@i0 \ CHO
c1
0
-
cii 3 0
c1
=c
CII 3
Dihydrogr iseofulvin
CH 3
Dehydrogriseofulvin
C H 30
c1
CH 3
Tetrahydrogriseofulvin CH30
C1
CtI 3
OCR 3
Griseofulvic Acid
c1 Isogriseofulvin FIGURE 11:
Impurities Found in the Fermenter Broth
EDWARD R. TOWNLEY
240
Table I X Elemental A n a l y s i s of G r i s e o f u l v i n : Element C H
c1
Batch UGFP-1961
% Theory
% Found
57.88 4.86 10.05
57.97 4.84 9.92
7.03
Spectrophotometric Analysis Q u a n t i t a t i v e u l t r a v i o l e t a n a l y s i s of g r i s e o f u l v i n may b e performed by comparison t o a R e f e r e n c e S t a n d a r d . The u l t r a v i o l e t absorbance i s d e s c r i b e d i n S e c t i o n 2.04 and F i g u r e 5. 7.04
Spectrofluorometric Analysis Griseof u l v i n e x h i b i t s f l u o r e s c e n t p r o p e r t i e s which have been u t i l i z e d f o r h i g h l y s e n s i t i v e a n a l y s e s i n blood and serum (30-33) s k i n and sweat ( 3 4 ) . Riegelman (32) h a s combined TLC s e p a r a t i o n w i t h a f l u o r i m e t r i c d e n s i t o m e t e r r e a d o u t t o g i v e a h i g h l y s p e c i f i c and s e n s i t i v e g r i s e o f u l v i n d e t e r mination i n plasma. Other a n a l y s e s are commonly performed i n e i t h e r 1%aqueous e t h a n o l ( 3 0 ) , a c t i v a t i o n maxima 295 and 335 nm, f l u o r e s c e n c e maxima a t 450 nm o r anhydrous methanol (31) a c t i v a t i o n maxima unchanged a t 295 and 335 nm, f l u o r e s c e n c e maxima 420 nm. Values are u n c o r r e c t e d . Other a p p l i c a t i o n s t o t h e a n a l y s i s of b u l k d r u g s , dosage forms o r as a d e t e c t i o n method f o r high performance l i q u i d chromatography are f e a s i ble. 7.05
Colorimetric Analysis A c o l o r i m e t r i c a s s a y of g r i s e o f u l v i n , based on t h e yellow-orange c o l o r (Xmax=420 nm) which d e v e l o p s when g r i s e o f u l v i n is h e a t e d w i t h i s o n i c o t i n i c a c i d h y d r a z i d e i n a l k a l i n e medium h a s been d e s c r i b e d by Unterman (35) and t h e mechanism i n v e s t i g a t e d by Unterman and Duca (36). 7.06
Iodometric Analysis Iodometric a n a l y s i s has been a p p l i e d t o t h e d e t e r mination of g r i s e o f u l v i n i n s t a g e s of t h e manufacturing proc e s s (37). The mycelium i s e x t r a c t e d w i t h chloroform and t h e a n a l y s i s c a r r i e d out i n a l c o h o l i c solution. The 0.01N i o d i n e s o l u t i o n is s t a n d a r d i z e d w i t h g r i s e o f u l v i c a c i d . 7.07
Turbidimetric Analysis A t u r b i d i m e t r i c a s s a y f o r potency e v a l u a t i o n of g r i s e o f u l v i n h a s been r e p o r t e d (38). The drug i s d i s s o l v e d i n
GRISEOFULVIN
24 1
e t h y l e n e g l y c o l monomethyl e t h e r (niethyl c e l l o s o l v e ) . Polym e r i z a t i o n i s induced w i t h g l y c e r o l and guanosine-5'-triphosp h a t e (GTP). 7.08
Polarographic Analysis A s t u d y d i r e c t e d toward a comparison of t h e reduct i o n p o t e n t i a l s f o r g r i s e o f u l v i n homologs and a n a l o g s s u g g e s t s t h a t polarography i s a method of g r i s e o f u l v i n i d e n t i f i c a t i o n ( 3 9 ) . In e t h a n o l i c s o l u t i o n w i t h 0 . 2 M K C 1 s u p p o r t i n g elect r o l y t e , g r i s e o f u l v i n shows two p o l a r o g r a p h i c waves w i t h h a l f wave p o t e n t i a l s a t about -1.58 V and -1.84 V. T h i s system h a s been a p p l i e d w i t h good r e s u l t s t o t h e d e t e r m i n a t i o n of f i n i s h ed p r o d u c t s i n c l u d i n g t a b l e t s . The a c c u r a c y , p r e c i s i o n and s e l e c t i v i t y of t h e method w a s compared w i t h t h e i o d o m e t r i c method ( 4 0 ) . I s o g r i s e o f u l v i n and g r i s e o f u l v i c a c i d do n o t interfere. (41,42) 7.09
Chromatographic Analyses 7.091
P a r t i t i o n Column Chromatography G r i s e o f u l v i n maybe s e p a r a t e d from o b s e r v e d s t r u c t u r a l l y s i m i l a r i m p u r i t i e s i n t h e f e r m e n t e r b r o t h by means of p a r t i t i o n column chromatography ( 1 3 ) . A C e l i t e c o l umn packing and s o l v e n t system c o n s i s t i n g of methano1:water: hexane:chloroform ( 8 : 2 : 9 : 1 ) was used. Tetrahydrogriseofulvin, dihydrogriseofulvin, i s o g r i s e o f u l v i n , dechlorogriseofulvin are s e p a r a t e d from g r i s e o f u l v i n . The s t r u c t u r e s f o r t h e s e compounds have been g i v e n i n S e c t i o n 5. 7.092 T a b l e X.
P a p e r Chromatography A p a p e r chromatography system i s g i v e n i n
(43) Table X
S o l v e n t System Benzene :Cyclohexane; Methanol :Water (5:5:6:4) Glacial a c e t i c a c i d , 0.5%, w a s added t o t h e o r g a n i c phase of t h e s o l v e n t after equilibration. 7.093 i n T a b l e XI.
Paper
Detection
Reference
Whatman No. 1
uv
43
Thin Layer Chromatography Thin l a y e r chromatographic systems are g i v e n The d e t e c t i o n method w a s U.V.
EDWARD R. T O W N L E Y
242
Table XI Adsorbent
Tr
Reference
Methanol :n-bu tanol; 95% ethano1:conc. ammonium hydroxide (4:1:2:1, by ~01.)
Silica Gel
0.64
44
Ch1oroform:isopropanol (3:1, by vole)
Silica Gel
0.86
44
n-butano1:formic acid: Silica Gel water (77:10:13 by vol.)
0.86
44
n-Butanol:95% ethanol conc. ammonium hydroxide:water (4:1:2:1 by vole)
Silica Gel
0.64
44
Ch1oroform:acetone (93:7 by vole)
Silica Gel
0.65
45
Ch1oroform:methanol (lot1 by vole)
Silica Gel
0.82
46
-
47
Solvent System
Ch1oroform:acetic acid Silica Gel diethyl ether (17:1:3) Methanol :benzene (2:98 by vol.)
Silica Gel
0.50
48
Ethyl acetate
Silica Gel
0.50
17
7.094
Gas Chromatopraphy Successful griseofulvin analyses by gas chromatography are reported for simulated samples (49) fermentation extracts (45) and pharmaceutical bulk and dosage forms (50). Margosis (15) describes the application of gas chromatography to the purity determination of griseofulvin. Separation from the related compounds; dehydrogriseofulvin, isogriseofulvin and dechlorogriseofulvin was demonstrated. In a subsequent collaborative study (50) the accuracy and precision of the method was established. Although griseofulvin is thermally stable, the high GLC temperatures require precautions similar to those taken for steroids when preparing columns, column supports and associated equipment (45).
GRISEOFULVIN
243
The s p e c i f i c and s e n s i t i v e GLC d e t e r m i n a t i o n of g r i s e o f u l v i n i n body f l u i d s and t i s s u e s such as s k i n , sweat, u r i n e and plasma w i t h e l e c t r o n c a p t u r e d e t e c t i o n h a s been used by s e v e r a l i n v e s t i g a t o r s (34,51,52). Gas chromatographic c o n d i t i o n s are g i v e n in Table XII. Table XI1
Carrier Gas
Column
150 cm x 4 mm I.D.; Ushaped s t a i n l e s s s t e e l t u b i n g , 1.5% QF-1 on Anakrom ABS 3 f t x 4 mm I.D.; coiled g l a s s tubing, 3% OV-101 on Gas Chrom Q
N2
He2
Column Temp.
Internal Standard
230'
245'
5 f t x 4 mm I.D.; g l a s s 10% Methane column, 3% OV-17 on 90% Argon Chromosorb W. o r Gas or Chrom Q.
Reference
diphenylphthalate
tetraphenylcyclopentadienone
27OoC
diazepam
45,49
15
34,50, 51,52
N2
3 f t x 4 mm I.D.; glass coiled. % OV-17 on Gas Chrom. Q
He 2
225'
tetraphenyl15 cyc l o p e n t adienone
7.095
High Performance L i q u i d Chromatography G r i s e o f u l v i n can b e r e a d i l y chromatographed on e i t h e r normal o r r e v e r s e p h a s e columns. S e p a r a t i o n of dec h l o r o g r i s e o f u l v i n , t h e most common s y n t h e t i c i m p u r i t y i s accomplished on C / 1 8 , CN (17) o r ETH columns. (15) I s o g r i s e o f u l v i n , i s s e p a r a t e d on e i t h e r CN (17) o r ETH columns (15). L i q u i d chromatography c o n d i t i o n s are g i v e n i n T a b l e XIII.
EDWARD R. T O W N L E Y
244
Table XI11
Column PBondapak C/18 ( o c t y l d e c y l c h e m i c a l l y bonded to silica)
Reverse phase
mondapak C/18 ( o c t y l d e c y l c h e m i c a l l y bonded to silica)
II
Zorbax CN (cyanop r o p y l c h e m i c a l l y bonded to silica)
11
Mobile Phase
Internal Standard
Refer-
Methanol: water 3:2
n-butyl p-hydroxy benzoate
16
45% a c e t o - d i a z e p a n
53
ence
nitrile in 45mM KH PO4 pn = 3.6
Permaphase ETH Normal (C-7 e t h e r c h e m i c a l l y phase bonded t o p e l l i c u l a r 30-50 mesh g l a s s packing)
Methanol: water 3:2
5% c h l o r o form i n hexane
m-phenyl phenol
16
14
7.10
B i o l o g i c a l Methods o r A n a l y s i s M i c r o b i o l o g i c a l p r o c e d u r e s have been developed f o r a s s a y of g r i s e o f u l v i n and a p p l i e d t o t h e a n a l y s i s of b u l k d r u g s and dosage forms ( 1 ) . The c y l i n d e r p l a t e a g a r d i f f u s i o n method is t h e o f f i c i a l m i c r o b i o l o g i c a l method of d e t e r m i n a t i o n ( 5 5 ) . Microsporum gypseum (ATCC 14683) i s t h e t e s t organism. 8.
I d e n t i f i c a t i o n and D e t e r m i n a t i o n i n Body F l u i d s and T i s s u e G r i s e o f u l v i n h a s u s u a l l y been determined i n body f l u i d s and t i s s u e s by s p e c t r o f l u o r i m e t r i c (30-34) o r g a s chromatograp h i c methods (45,46,48). More r e c e n t l y g r i s e o f u l v i n h a s been determined i n plasma by h i g h performance l i q u i d chromatography (53,541. A n a l y s i s of Dosage forms Usual dosage forms of g r i s e o f u l v i n are c a p s u l e s , t a b l e t s and b o l u s e s . These may b e p r e p a r e d f o r a n a l y s i s by s i m p l e l i q u i d s o l i d e x t r a c t i o n of drug s u b s t a n c e . Margosis (15,50) used chloroform as an e x t r a c t i n g s o l v e n t w i t h g e n t l e h e a t . A compendia procedure d e s c r i b e s t h e e x t r a c t i o n of g r i s e o f u l v i n from t a b l e t s w i t h b o i l i n g a l c o h o l . The a n a l y s i s f o r e x t r a c t e d drug s u b s t a n c e has been performed by s e v e r a l methods. Most common is a simple u l t r a v i o l e t a n a l y s i s ( 2 , 3 , 5 5 ) . Polarography u t i l i z i n g t h e system g i v e n i n S e c t i o n 7.08 h a s been used (39). Thin-layer, g a s and l i q u i d chromagraphy may a l s o be 9.
G R I S EO F U LV I N
245
used u t i l i z i n g systems d e s c r i b e d i n S e c t i o n s 7.093, 7.094, and 7.095 r e s p e c t i v e l y . These l a t t e r methods are v a l u a b l e because of t h e i r s p e c i f i c i t y . I n t h e United S t a t e s , g r i s e o f u l v i n drug s u b s t a n c e and dosage forms must conform t o t h e r e g u l a t i o n s of t h e F e d e r a l Food and Drug A d m i n i s t r a t i o n concerning a n t i b i o t i c d r u g s (55, 5 6 ) . M i c r o b i o l o g i c a l a s s a y r e s u l t s o b t a i n e d by a n a l y t i c a l methods d e s c r i b e d i n t h e s e compendia a r e c o n c l u s i v e . 10.
Acknowledgements The a u t h o r wishes t o thank D r . M. D. Yudis and D r . H. Suprenant f o r t h e i r encouragement f o r t h i s work and t o acknowledge t h e v a l u a b l e a s s i s t a n c e of members of t h e S c h e r i n g C o r p o r a t i o n , P h y s i c a l Organic Research S e c t i o n : D r . R. B r a m b i l l a , M r . P. B a r t n e r , M r . C. Eckhart and M r . R. F o e s t e r f o r t h e a c q u i s i t i o n and i n t e r p r e t a t i o n of t h e p h y s i c a l d a t a , and t o t h e S c h e r i n g l i b r a r y s t a f f p a r t i c u l a r l y M s . J . Nocka, f o r t h e l i t e r a t u r e s e a r c h e s and S c h e r i n g General O f f i c e S t a f f f o r t h e c a r e f u l t y p i n g of t h i s monograph.
EDWARD R. T O W N L E Y
246
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28.
15,
E. Papp, K. Magyar and H. J. Schwartz, J. Pharm. Sci., 65, 441 (1976).
29
H. Auterhoff and M. Kliem, Arch der Pharmazie, 309, 326 (1976)
30
C. Bedford, K.J. Child and E.G. Tomich, Nature, 2,364 (1959)
31.
M. Kraml, J. Dubuc and D. Dvornik, J. Pharm. Sci., 5 4 , 655 (1965).
32.
L.J. Fisher and S . Riegelman, J. Chromatogr.,.u, 268 (1966)
EDWARD R. TOWNLEY
248
19, ( 6 )
33.
K. E i s e n b r a n d t , Pharmazie,
406 ( 1 9 6 4 ) .
34.
V. P Shah, S. Riegelman and W. L. E p s t e i n , J. Pharm. S c i . , 6 l , 634 ( 1 9 7 2 ) .
35.
H.W.
36
H.W. Unterman and A l . Duca, Rev. Roum Chim. (1971).
37.
H.W. Unterman and A l . Duca,. Chim. Anal. 196 ( 1 9 7 2 ) .
38
J. Hoebeke and G. Van V i j e n , L i f e S c i . , l7, 5 9 1 ( 1 9 7 5 ) .
39.
H.W. Unterman and A l . Duca, Isr. J. Chem., l2, ( 5 ) 985 (1974).
40.
J. Kadar-Pauncz, Acta Pharm Hung., 3 5 , 297 ( 1 9 6 3 ) .
41.
H.W. Unterman and A l . Duca, Rev. Chim. ( B u c h a r e s t ) ( 1 9 7 1 ) ; 2, 188 ( 1 9 7 2 ) .
42
H.W. Unterman, and A l . Duca, Chim. Anal. 1 ( 2 ) , 97 ( 1 9 7 1 ) .
43.
S. Symchowicz and K.K.
Unterman, Rev. Chim. ( B u c u r e s t i )
16,( 5 )
286 ( 1 9 6 5 ) .
16,1077
(Bucharest) 2 ( 3 )
1,97
(Bucharest)
Wong, Biochem. Pharmacol, l5,
1595 ( 1 9 6 6 ) . 44.
W.A. Creasey, K.G. Bensch and S.E. Pharmacol., 20, 1579 ( 1 9 7 1 ) .
45.
R.J. Cole, J . W . K i r k s e y and C.E. b i o l . 9 l9, 1 0 6 , ( 1 9 7 0 ) .
46.
C. L i n , R. Chang, C . Casmer, and S. Metab. Dispos., 1,6 1 1 ( 1 9 7 3 ) .
47.
2 . Durackova, V.
Malawista, Biochem.
Holaday, Appl. Micro-
Symchowicz, Drug
B e t i n a , P. Nemec, J. Chromatog.,
116,
141 ( 1 9 7 6 ) . 48
49.
I s s a q , E.W. Barr, T. Wei, C. Meyers, A. A s z a l o s , J. Chromatog., 133, 291 ( 1 9 7 7 ) .
H.J.
S. I g u c h i , M. Yamamoto and T. Goromaru, J. Chromatogr.,
24,
182 ( 1 9 6 6 ) .
GRISEOFULVIN
249
64,
50.
M. M a r g o s i s , J. Pharm. S c i . ,
51.
H . J . S c h w a r t z , B.A. Waldman, and V. Madrid, J. Pharm. S c i . , 65, 370 (1976).
52.
V.P.
Shah, S . Riegelman and W.L.
1020 ( 1 9 7 5 ) .
E p s t e i n , J. Pharm. S c i . ,
6 1 , 634 (1972).
155, 206
53.
L.P. Hackett and L . J . (1978).
54.
R.L. N a t i o n , G.W. Peng, V. Smith and W.L. Pharm. S c i . , 67, 805, 1978.
55.
US Code of F e d e r a l R e g u l a t i o n s (1976) Food and DruRs, T i t l e 21, p a r t 436.105, Washington, D.C., US Government
D u s i , J. Chromatog.,
Chiou, J.
printing office. 56.
E.M. Oden, G.H. Wagman, and M . J . W e i n s t e i n , A n a l y t i c a l M i c r o b i o l o g y , Vol. 11, Academic P r e s s , 1972, p 385.
Analytical Profiles of Drug Substances, 8
HALCINONIDE Joel Kirschbaum I.
2.
3.
4.
5. 6.
7.
History, Description, Precautions, Synthesis 1 . 1 History I . 2 Name, Formula, Molecular Weight I . 3 Appearance, Color. Odor I .4 Precautions I .5 Synthesis Physical Properties 2.01 Single Crystal X-RayDiffraction 2.02 Mass Spectrometry 2.03 Nuclear Magnetic Resonance Spectrometry (NMR) 2.031 'H-NMR 2.032 IT-NMR 2.04 Infrared Spectrometry 2.05 X-Ray Powder Diffraction 2.06 Ultraviolet Spectrometry 2.07 Optical Rotation 2.08 Fluorescence Spectrometry 2.09 Melting Range 2.10 Differential Thermal Analysis 2. I I Thermal Gravimetric Analysis 2.12 Microscopy and Crystal Size 2. I3 Particle Size 2.14 Surface Area 2. I5 Polymorphism 2.16 Hydration Solution Properties 3 . 1 Intrinsic Dissolution Rate 3 . 2 Solubilities in Aqueous and Nonaqueous Solvents 3.3 Partition Coefficients Methods of Analysis 4. I Elemental and Inorganic Analyses 4.2 Identification, Ultraviolet and Colorimetric Analyses 4.3 Chromatographic Analyses 4.3 I High Pressure Liquid Chromatography (HPLC) 4.32 Thin-Layer Chromatography (TLC) 4.33 Column Chromatography 4.34 Paper Chromatography 4.4 Polarographic Analysis 4.5 Halcinonide in Tissues and Body Fluids Stability Acknowledgments References 25 I
Copyright @ 1979 by Academic Press, Inc. All rights of reproduction in any form reserved.
ISBN 0-12-260808-9
JOEL KIRSCHBAUM
252
1 History, Description, Precautions and Synthesis
1.1 History Halcinonide is a topical antiinflammatory agent. 192 Introduction of a 9a-fluoro group3 to the hydrocortisone molecule resulted in an eight-fold increase in antiinflammatory activity. Such other groups as 16a-hydroxy, 16a-methyl, 168methyl, 16,17-acetonide and 6a-methyl moieties have been found to diminish or eliminate mineralocorticoid activity resulting from the 9a-fluoro substituent, while retaining he enhanced antiinflammatory activity of the halo derivative Halcinonide lipophilicity is increased by masking the 16,17-hydroxyl groups as the acetonide, which increases the availability of the steroid at the site of action in the skin. The 21-chloro group also increased antiinflammatory properties. Halcinonide has systemic3 as well as topical activity.
E.
1.2 Names, Formula and Molecular Weight Halcinonide is the United States adopted name5 (USAN). The preferred chemical names6 are 21-chloro-9-fluoro-11Bhydroxy-l6a, 17-[(l-methylethylidene)bis(oxy)]pregn-4-ene-3, 20-dione, and 21-chloro-9a-fluoro-ll~-l6a,l7-trihydroxypregn-4 -ene-3,20-dione cyclic 16,17-acetal with acetone. Other chemical names are 21-chloro-9-fluoro-ll~-hydroxy-l6~,l7a-isopropylidenedioxy-4-pregnene-3,2O-dione, 9a-fluoro-21-chloro-llf3, 16a, 17a-trihydroxypregn-4-ene-3, 20-dione 16,17 acetonide and 21chloro-9-fluoro-118,16~,l7-trihydroxypregn-4-ene-3,2O-dione cyclic 16,17-acetal with acetone. 21
12
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2qH 32 5 454.97 Daltons
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Halcinonide has also been called Halog and Squibb SQ 18,566. The Chemical Abstracts systematic number is CAS-3093-35-4.
HALCINONIDE
1.3
253
Appearance, Color and Odor
Halcinonide is a white or practically white, odorless powder consisting of free flowing crystals. 1.4
Precautions
Since halcinonide is a corticosteroid, large doses of unformulated steroid are needed systemically before the unwanted side effects appear. Halcinonide is usually formulated at concentrations of 0 . 1 % , or less. Normal handling precautions are adequate.
1.5
Synthesis
The of halcinonide is summarized in Figure 1, starting with 16a-hydroxy-9a-fluorohydrocortisone (A4-pregnene-9a-f luoro-11@, 16a,1 7 a , 21-tetrol-3,20-dione; dihydrotriamcinolone, I), which is available c ~ m m e r c i a l l y . l ~ - ~ ~ This tetrahydroxy steroid is slurried in acetone, and then 70% perchloric acid is added slowly. The acetonide, I1 (9a-fluoro11~,16a,l7,21-tetrahydroxypregn-4-ene-3,2O-dioney cyclic 16,17acetal with acetone; d i h y d r o t r i a m c i n o l o n e - a c e t o n i d e ) precipitates spontaneously from solution. Mesyl chloride is added to the acetonide in pyridine to give the 21-mesylate derivative (dihydrotriamcinolone acetonide-21-mesylate, 111). Compound I11 is dissolved in dimethylformamide, lithium chloride is added and the mixture is refluxed to produce halcinonide (IV), which is recrystallized from a solution of n-propanol in water. 2.
Physical Properties
2.01 Single Crystal X-Ray Diffraction
14
The three dimensional structure was obtained by means of single crystal X-ray diffraction. CuKa radiation, a graphite monochromator, and a photomultiplier tube were used to collect 1825 total reflections on an automated diffractometer. Of these, 1162 were used for the analysis. Figure 2 shows a computer generated drawing of halcinonide. The position of the chlorine atom was not clear from the Patterson map, but the direct method program "MLJLTAN" gave its position. Least squares refinement of coordinates together with anisotropic temperature factors, in the final stages, gave an R factor of 0.11.
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JOEL KIRSCHBAUM
256
2.02 Mass S p e c t r o m e t r y F i g u r e . 3 i s t h e p l o t t e d low r e s o l u t i o n mass s p e c t r u m of h a l c i n o n i d e found u s i n g a n A E I S c i e n t i f i c Apparat u s L t d , Model 902 mass s p e c t r o m e t e r . S p e c t r a were c o l l e c t ed on f r e q u e n c y modulated a n a l o g t a p e and p r o c e s s e d on a D i g i t a l Equipment C o r p . , P D P - l l . The t a b l e 1 5 below summarizes h i g h r e s o l u t i o n d a t a from m/z 39 t o t h e p r o m i n e n t m o l e c u l a r i o n a t 454.1922, which c o r r e s p o n d s t o C24H3205FC1. Each f r a g m e n t i o n c o n t a i n i n g c h l o r i n e a p p e a r s as a d o u b l e t p e a k b e c a u s e c h l o r i n e is a m i x t u r e of two i s o t o p e s ( 3 5 C l and 3 7 C l > . T h e s e p e a k s a r e two mass u n i t s a p a r t w i t h a n i n t e n s i t y r a t i o of 3 t o 1. Fragmentation proceeds a l o n g s e v e r a l pathways, a s shown below.
439 419 396?)m/z
361
377
m/z 2 6 4
m/z
278
These s t r u c t u r e s do n o t n e c e s s a r i l y r e p r e s e n t the a c t u a l i o n i c s t r u c t u r e b u t o n l y t h e o r i g i n of t h e f r a g m e n t .
C H
The weak i o n s a t m/z 121, 122 and 1 2 3 (CgHgO, 0) a r e c h a r a c t e r i s t i c of A4-3-one s t e r o i d s . 8 11
0 and C H
8 10
Figure 3 Low Resolution Mass Spectrum of Halcinonide. See text for details. 5433 S Q 1 8 , 5 6 6 BFI NN009NFl 175 DEG
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High-Resolution Massa Spectrum of H a l c i n o n i d e Found Mass
Calc. Mass
454.1925 439.1680 419.2252 396.1501 377.2147 361.1838 319.1665 278.1695 264.1524 246.1422 135.0808 123.0769 122.0729 121.0683 76.9790 43.0184
454.1922 439.1687 419.2233 396.1503 37 7.2128 361.1815 319.1709 278.1682 264.1525 246.1420 135.0810 123.0810 122.0732 121.0653 76.9794 43.0184
a
Unsat.
bO/EC
8. 0 8. 5 8.5 8. 0 7.5 8.5 7.5 6.0 6.0 7.0 4.5 3.5 4.0 4.5 1.5 1.5
24 23 24 21 22 21 19 17 16 16 9 8 8
32 29 32 26 30 26 24 23 21 19 11 11 10
8
9
2 2
3
2
- 0
F -
5 5 5 4 4 4 3 2 2 1 1 1 1 1 1 1
Only t h o s e peaks c o n s i d e r e d t o b e s i g n i f i c a n t t o t h e d i s c u s s i o n are l i s t e d . element map c a n b e o b t a i n e d on r e q u e s t .
bNumber of double bonds and r i n g s . C
0 E E 0 E E E 0 0 0 E E 0 E E E
c H
0-odd e l e c t r o n i o n ; E-even e l e c t r o n i o n .
1 1 1 1 1 1 1 1 1 1 0 0 0 0 0 0
c1 1 1 0
1 0 0 0 0 0 0 0 0 0 0
1 0
A complete
HALCINONIDE
259
2 . 0 3 Nuclear Magnetic Resonance Spectrometry
2.031
(NMR)
'H-NMR
Figure 4 is the 100 MHz NMR Spectrum of halcinonide in deuterochloroform containing tetramethylsilane as internal reference at 0 Hz. The instrument used is a Varian Associates, Inc., Model XL-100 NMR spectrometer. Below is an interpretation of the various resonances. 'H-NMR
Proton at Carbon
Assignments
Chemical Shift
Peak Appearance S = singlet D = doublet B = broad
c-4
5.78
S
c-11
4.58
B
C-16
5.05
D J15,16= 4 . 0 Hz
C-18
0.87
S
c-19
1.51
S
c-21
4.19 4.57
AB quartet
8-Acetonide, methyl
1.15
a-Acetonide, methyl
1.44
These data agree with the published results of the 21hydroxy-A' analog, triamcinolone acetonide.l 7
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HALClNONlDE
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26 1
13C-NMR
The 13C-NMR spectrum of halcinonide, Figure 5, was obtained18 using a Jeol FX-60Q NMR spectrometer operating in the Fourier transform mode at 15 MHz. Numbers on the vario u s peaks refer to the assignments in the table below. These assignments were made by comparison of chemical shifts and 3C-19F coupling constants to those assigned to such related steroids as 9a-fluorocortisol (9a-fluoro-llf3,17,21-trihydroxypregn-4-ene-3,20-dione). Four pairs of closely related peaks show chemical shift differences small enough to lead to possible reversals o f their tentative assignments. These pairs are the peaks assigned to the acetonide methyl groups (6 = 28.6 and 6 = 25.1 ppm), the two carbonyl peaks (6 = 202.1 and 199.1 ppm), the methylene carbons assigned to C-1 and C-7 (6 = 26.2 and 28.5 ppm), and the methylene carbons assigned to C-2 and C-15 (6 = 33.2 and 33.7 ppm). These assignments must be verified by additional experimentation. 'C-NMR Assignments Carbon
1 2 3
4
5 6 7 8 9 10 11 12 13 14 15 16 17 18 19 20 21 22 23 24
Chemical Shift 6 (ppm>a 26.2 33.7 199.1 124.7 169.0 30.7 28.5 33.1 99.0 43.7 70.2 37.3
(28.5) (33.2) (202.1)
(26.2)
44.8
43.4 33.2 81.9 98.1 17.0 21.9 202.1 47.1 111.5 28.6 25.1
C-F Coupling Constant (Hz) 3
3 19 175 21
2 (33.7)
6 (199.1) (25.1) (28.6)
a Referenced from center peak of deuterochloroform = 77.0 pprn from tetramethyl silane. Numbers in parentheses refer to alternative assignments (see text for details).
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2.04
I n f r a r e d Spectrometry
F i g u r e 6 shows t h e i n f r a r e d s p e c t r u m of h a l c i n o n i d e r u n as a p o t a s s i u m bromide p e l l e t , u s i n g a Perkin-Elmer Model 6 2 1 i n f r a r e d s p e c t r o m e t e r . Below a r e t h e i n t e r p r e t a t i o n s of v a r i o u s a b s o r b a n c e s . l 9
1
Frequency (cm )
2.05
Interpretation
3450
-OH S t r e t c h
2950
-OH S t r e t c h
17 3 0
C z 0 Keto
1660
C3
Keto
1620
A4
C=C
X-ray Powder D i f f r a c t i o n
F i g u r e 7 is t h e powder X-ray d i f f r a c t i o n p a t t e r n of h a l c i n o n i d e a s o b t a i n e d on a P h i l i p s gowder Using a d i f f r a c t i o n u n i t e m i t t i n g CuKa r a d i a t i o n a t 1.54A. s c i n t i l l a t i o n c o u n t e r d e t e c t o r , t h e sample w a s scanned and r e c o r d e d from a p p r o x i m a t e 1 2 t o 4 0 d e g r e e s ( 2 0 ) . The t a b l e below i s t h e s o r t e d d a t a . 21;
20 (Degrees)
' d ' (Angstrom) 1
14.80 12.53 18.49 17.94 19.82 29.31 18.10 11.67 32.14 39.59 25.86 21.47 26.80 25.24 15.67 40.37 22.33 33.08 25.47 34.02 'Interplanar
5.99 7.06 4.80 4.94 4.48 3.05 4.90 7.58 2.78 2.28 3.45 4.14 3.33 3.53 5.66 2.23 3.98 2.71 3.50 2.64
Relative Area
2
1.000 0.866 0.738 0.526 0.422 0.266 0.246 0.225 0.195 0.171 0.165 0.142 0.135 0.135 0.131 0.124 0.117 0.114 0.053 0.052
distance
2 R e l a t i v e a r e a , o r i n t e n s i t y , i s based on h i g h e s t i n t e n s i t y of 1.00 u s i n g CuKa r a d i a t i o n .
Figure 6 I n f r a r e d Spectrum of H a l c i n o n i d e , Potassium Bromide P e l l e t . See t e x t € o r d e t a i l s .
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JOEL KIRSCHBAUM
2.06
U l t r a v i o l e t Spectrometry
U l t r a v i o l e t s p e c t r a 2 ' of h a l c i n o n i d e w e r e r e c o r d e d on a Beckman Acta C I I I s p e c t r o p h o t o m e t e r . The s p e c t r a i n m e t h a n o l , 0.M m e t h a n o l i c h y d r o c h l o r i c a c i d and 0 . W m e t h a n o l i c sodium h y d r o x i d e show p e a k maxima a t 238 nm, and r e m a i n unchanged a f t e r 24 h o u r s . Absorbances are t a b u notation. l a t e d below u s i n g t r a d i t i o n a l E 1l % cm
1% Elcm So l v e n t
Initial
3 Hours
24 Hours
Me t h a n o 1
379
374
373
0.M Methanolic
370
372
370
380
382
380
H y d r o c h l o r i c Acid 0 . IM M e t h a n o l i c
Sodium Hydroxide The s p e c t r u m i n 95% e t h a n o l a l s o h a s a peak maximum a t 238 nm and a p p e a r s s t a b l e f o r a t l e a s t 3 h o u r s . I n a c e t o n i t r i l e and e t h y l e t h e r t h e maximum i s s h i f t e d t o 234 nm and 229 nm, r e s p e c t i v e l y . 2.07
Optical Rotation
were
The s p e c i f i c r o t a t i o n s i n d e t e r m i n e d 2 3 t o b e as f o l l o w s ,
Wavelength (nm)
2.08
Specific Rotation
589
+156
578
+164
546
+188
436
+348
305
+436
F l u o r e s c e n c e Spectrometry
Using a Perkin-Elme54Model 204 f l u o r e s c e n c e s p e c t r o p h o t o m e t e r , no f l u o r e s c e n c e w a s found a t e i t h e r 1 o r 1000 ug h a l c i n o n i d e p e r mL o f m e t h a n o l . No f l u o r e s c e n c e w a s induced i n 0 . U h y d r o c h l o r i c a c i d o r 0 . U sodium h y d r o x i d e .
267
HALCINONIDE
2.09
Melting Range
Following the USP procedure25 for class lA compounds, the melting range.of halcinonide is 270-272" (reference 21). This is in excellent agreement with the results of differential thermal analysis, below, as well as hot stage microscopy, section 2.12. 2.10
Differential Thermal Analysis
A duPont Model 900 Differential Thermal Analyzer shows halcinonide to have one endothermZ6 at 269". Decomposition on melting precludes differential scanning colorimetry studies for purity.
2.11
Thermal Gravimetric Analysis
Using a Perkin-Elmer Model TGS-2 Thermogravimetric Analyzer, halcinonide was found26 to lose 0.3% total volatile material at 70". No further l o s s was found up to 150". The heating rate was 20"/minute under a nitrogen atmosphere. 2.12 the method to 4, 5 to three lots (acicular)
Microscopy and Crystal Type
Microscopically, the crystal type depends on of preparation of halcinonide. Slabs, either 2 10, or 10 to 15 microns square, were found in of halcinonide, intermingled with needle-like crystals 5 to 10microns 10ng.27
14 Single crystal x-ray diffraction studies showed that the crystals of halcinonide recrystallized from n-propyl alcohol-water azeotrope (79:22) are orthorhombic and belong to the gpace group P2 2 2 , with unit sell constants 1 of a = 10.007 A , b = 11.875 an& c = 19.460 A. Density is 1.330 gm/cm3, as measured by flotation in a hexane-carbon tetrachloride gradient. The molecular weight calculated from the unit cell volume and density is 461 daltons (theoretical is 455 daltons).
A
Hot stage microscopy26 was performed using a Mettler FP52 temperature controller at a rate o f 3"/minute. Melting began at 268.2", and by 271.4" all crystals were melted. The yellow melt slowly turned orange-brown. Cooling showed no recrystallization at ambient temperature.
JOEL KIRSCHBAUM
268
2.13
Particle
Size
By l i g h t s c a t t e r i n g u s i n g a Royco i n s t r u m e n t , a l l p a r t i c l e s are below 20 microns.27 C o u l t e r Counter ana l y s i s of ground h a l c i n o n i d e suspended i n a sodium c h l o r i d e s o l u t i o n shows 100% t o be <10.2p (p = m i c r o n ) , 98.2% <6.4p, 95.3% <5.1p, 52.0% <2.6p and 19.9% <1.6p.
2.14
S u r f a c e Area
A s measured by g a s a d ~ o r p t i o n ,t h~e~ s u r f a c e areas of t h r e e l o t s of ground h a l c i n o n i d e a r e 2.61, 3.85 and 4.08 m2/g. 2.15
Polymorphism
There i s no evidence € o r polymorphism from i n f r a r e d s p e c t r o s c o p y and d i f f e r e n t i a l t h e r m a l a n a l y s i s , and o n l y i n c o n c l u s i v e d a t a from x-ray d i f f r a c t i o n and microscopy studies
.
2.16
Hydration
The c r y s t a l s of h a l c i n o n i d e are n o t s o l v a t e d w i t h water, based on a t o t a l v o l a t i l e c o n t e n t of 0.3% o b t a i n ed by t h e r m a l g r a v i m e t r i c a n a l y s i s , a c o r r e c t e l e m e n t a l a n a l y s i s , and a loss-on-drying v a l u e of 0.6% (cf. s e c t i o n 4 . 1 , Elemental and I n o r g a n i c A n a l y s e s ) . 3.
Solution Properties 3.1
I n t r i n s i c D i s s o l u t i o n Rate
The i n t r i n s i c d i s s o l u t i o n r a t e w a s determined a f t e r compressing powder under 2000 p . s . i . g . p r e s s u r e u s i n g 318" d i a m e t e r disc-shaped d i e s . I n one l i t e r of 0 . M hydroc h l o r i c a c i d a t 37", a g i t a t e d a t a r a t e of 50 r.p.m., t h e i n t r i n s i c d i s s o l u t i o n rate of h a l c i n o n i d e i s 8.33 x loW3 mg min.-l cm-' computed from d a t a o b t a i n e d by u l t r a v i o l e t s p e c t r o m e t r y . 28 3.2
S o l u b i l i t i e s i n Aqueous and Nonaqueous S o l v e n t s
S o l u b i l i t i e s of h a l c i n o n i d e were determined i n v a r i o u s s o l v e n t s . 2 9 R e s u l t s a r e r e p o r t e d u s i n g t h e U.S.P. d e f i n i t i o n s . 30
269
HALCINONIDE
Solvent
Water H y d r o c h l o r i c a c i d , 0.W Sodium h y d r o x i d e , 0.N Acetone Ace t o n i t r i l e Acetonitrile-water Benzene Chloroform Castor o i l Dimethylsulf o x i d e Ethanol Ethyl e t h e r G l y c e r y l monooleate Hexanes Isopropyl myristate Methanol n-Oc t a n o l P o l y e t h y l e n e g l y c o l 200 P o l y e t h y l e n e g l y c o l 400 Polypropylene g l y c o l Propylene g l y c o l
Solubility
Insoluble Insoluble Insoluble Soluble Sparingly soluble Slightly soluble Slightly soluble Freely soluble Slightly soluble Freely soluble Slightly soluble Slightly soluble Slightly soluble I n so l u b l e Slightly soluble Slightly soluble Slightly soluble Slightly soluble Slightly soluble Slightly soluble Very s l i g h t l y s o l u b l e
270
JOEL K I R S C H B A U M
3.3
Partition Coefficients
H a l c i n o n i d e was p a r t i t i o n e d 3 ' between h e x a n e s and m e t h a n o l , and between h e x a n e s and a q u e o u s a c e t o n i t r i l e a t a p p a r e n t pH v a l u e s of 2 , 4 , 6 ( u n a d j u s t e d ) , and 10. A f t e r one h o u r of m i x i n g , t h e s t e r o i d c o n t e n t w a s d e t e r m i n e d by u l t r a v i o l e t s p e c t r o m e t r y of b o t h p h a s e s . I n a l l cases, a b s o r b a n c e a t t h e p e a k maximum of 239 nm was d e t e c t e d o n l y i n t h e a c e t o n i t r i l e - w a t e r o r m e t h a n o l l a y e r . The aqueous a c e t o n i t r i l e (pH 6) r e s u l t was v e r i f i e d 3 2 u s i n g 1 4 C - h a l c i n o n i d e l a b e l e d a t t h e 2- c a r b o n of t h e a c e t o n i d e m o i e t y . Thus, t h e halcinonide i s completely r e t a i n e d i n e i t h e r the a c e t o n i t r i l e water o r m e t h a n o l l a y e r s , i n d i c a t i n g t h e u t i l i t y of t h e s e s o l v e n t s y s t e m s f o r e x t r a c t i n g t h e s t e r o i d from f o r m u l a t i o n s . Another s t u d y 3 3 i n v o l v e d i s o p r o p y l m y r i s t a t e and aqueous p r o p y l e n e g l y c o l . A f t e r e u i l i b r a t i o n f o r two weeks a t 3 7 " , t h e l a y e r s were s e p a r a t e d 3 2 and t h e aqueous g l y c o l a s s a y e d f o r s t e r o i d u s i n g h i g h - p r e s s u r e l i q u i d chromatog r a p h y (cf. s e c t i o n 4 . 3 1 ) . The i s o p r o p y l m y r i s t a t e / a q u e o u s propylene g l y c o l p a r t i t i o n c o e f f i c i e n t s are as follows: p r o p y l e n e g l y c o l - w a t e r (4:l); 1 4 4 ; p r o p y l e n e g l y c o l - w a t e r ( 2 : 3 ) , 44.4; p r o p y l e n e g l y c o l - w a t e r ( 3 : 2 ) , 8.14, and propyl e n e g l y c o l - w a t e r ( 9 : 1 ) , 0.82. 4.
Methods of A n a l y s i s
4.1
E l e m e n t a l and I n o r g a n i c A n a l y s e s
The e l e m e n t a l a n a l y s i s 3 5 of h a l c i n o n i d e i s c a r b o n 63.38% (63.35%, t h e o r e t i c a l ) ; hydrogen 7.39% ( 7 . 1 0 % , t h e o r e t i c a l ) ; c h l o r i n e , 7.89 ( 7 . 7 9 % , t h e o r e t i c a l ) , and f l u o r i n e , 4.30% ( 4 . 1 7 % , t h e o r e t i c a l ) . Emission s p e c t r o c h e m i c a l a n a l y s i s f o r metals w a s performed u s i n g a Spec I n d u s t r i e s c a r b o n a r c A . C . u n i t w i t h a Bausch and Lomb d u a l g r a t i n g s p e c t r o g r a p h . Data were r e c o r d e d on g l a s s p l a t e s and i n t e r p r e t e d by means of a m i c r o p h o t o m e t e r . H a l c i n o n i d e c o n t a i n e d t r a c e amounts (% 60 pg/g t o t a l ) of t h e f o l l o w i n g m e t a l l i c i m p ~ r i t i e s ~i r~o ;n , manganese, c o p p e r , n i c k e l , l e a d , z i n c , aluminum, sodium, c a l c i u m , and magnesium. R e s i d ~ e - o n - i g n i t i o n ~of~ t h e same l o t 3 8 i s less t h a n 0.1%. Heavy metals c o n t e n t ( r e f e r e n c e 39, method 11) i s less t h a n 0.003%.38 A f t e r 3 h o u r s a t 100" i n vacuum, t h e l o ~ s - o n - d r y i n g ~v ~a l u e 3 8 i s 0 . 6 % . Four l o t s of h a l c i n o n i d e were a n a l y z e d f o r r e s i d u a l s o l v e n t s by d i s s o l v i n g p o r t i o n s i n p y r i d i n e . A f t e r r e t e n t i o n on a precolumn, water c o n t e n t w a s d e t e r m i n e d by
H ALCINON I DE
27 I
v a p o r p h a s e ( g a s ) chromatography u s i n g a n a u t h e n t i c s t a n d a r d b e f o r e and a f t e r e a c h i n j e c t i o n . Water c o n t e n t s of 0 . 6 % , o r l e s s , were found by c o m p a r i s o n w i t h a u t h e n t i c s t a n d a r d s . n-Propanol h a s o c c a s i o n a l l y b e e n found t o b e present. 4.2
I d e n t i f i c a t i o n , U l t r a v i o l e t and C o l o r i m e t r i c Analyses P r o p o s e d compendia1 i d e n t i f i c a t i o n tests f o r t h e
United States Pharmacopeia i n v o l v e comparing e i t h e r t h e i n f r a r e d o r u l t r a v i o l e t a b s o r p t i o n s p e c t r u m of s a m p l e h a l c i n n o n i d e w i t h t h a t o f a n a u t h e n t i c sample4'. To t n i s a u t h o r , a c h r o m a t o g r a p h i c method i s s u p e r i o r s i n c e e l u t i o n t i m e u s u a l l y d e p e n d s on much o f t h e m o l e c u l e i n t e r a c t i n g w i t h t h e s o l i d and m o b i l e p h a s e s v i a weak bonding f o r c e s . U l t r a v i o l e t a b s o r p t i o n d e p e n d s p r i n c i p a l l y on t h e 3-one-4-eneY A and B r i n g region being i n t a c t . H a l c i n o n i d e h a s b e e n q u a n t i t a t e d i n v a r i o u s formul a t i o n s o r a s b u l k powder by a d i f f e r e n t i a l u l t r a v i o l e t , b o r o h y d r i d e r e d u c t i o n a s ~ a y . ~ 2T h i s d i f f e r e n t i a l a s s a y inv o l v e s m e a s u r i n g t h e u l t r a v i o l e t a b s o r b a n c e of a n a l i q u o t of m e t h a n o l i c s t e r o i d s o l u t i o n c o n t a i n i n g sodium b o r o h y d r i d e decomposed p r i o r t o t h e a d d i t i o n of s t e r o i d . Its absorbance i s d e t e r m i n e d a g a i n s t a m e t h a n o l i c r e f e r e n c e s o l u t i o n of s t e r o i d r e d u c e d by sodium b o r o h y d r i d e t o d e s t r o y t h e 3-one4-ene chromophore. The u t i l i t y of t h i s p r o c e d u r e i s t h a t many i n t e r f e r e n c e s from e x c i p i e n t s and o t h e r , u n c o n j u g a t e d , s t e r o i d s can b e e l i m i n a t e d i n t h e a s s a y of a f o r m u l a t i o n . The a d d i t i o n of h a l c i n o n i d e t o v a r i o u s c o l o r i m e t r i c r e a g e n t s i v e s r e s u l t s t y p i c a l of s t e r o i d s w i t h i t s s u b s t i t ~ e n t s . ~ q - 4 5 A s t e s t e d i n o u r labor at or^,^^ h a l c i n o 47 , nide r e a c t s with a c i d i c ethanolic 4-nitrophenylhydrazine a f t e r h e a t i n g , c o o l i n g and t h e a d d i t i o n of sodium h y d r o x i d e , t o g i v e a r i l l i a n t p u r p l e "plum" c o l o r . With m e t h a n o l i c isoniazid4', halcinonide g i v e s a b r i g h t yellow c o l o r , w i t h no n o t i c e a b l e f a d i n g a f t e r two h o u r s . H a l c i n o n i d e added t o 4 - a m i n o a n t i ~ y r i n e ~i n~ m e t h a n o l i c h y d r o c h l o r i c a c i d g i v e s a p a l e g r e e n c o l o r . H a l c i n o n i d e added t o e t h a n o l i c t e t r a methylammonium hydroxide5', and h e a t e d , g i v e s a c l o u d y amber If c o l o r . T h i s c a n b e t h e b a s i s of a q u a n t i t a t i v e a say.51 added t o e t h a n o l i c tetramethylammonium hydroxide5' and p i c r i c a c i d , a n orange-red ( t e a c o l o r e d ) s o l u t i o n r e s u l t s with halcinonide. I n concentrated s u l f u r i c acid,53 halcinon i d e g i v e s a d e e p y e l l o w c o l o r . Adding water s l o w l y c a u s e s a v i o l e t c o l o r t o a p p e a r a t t h e i n t e r f a c e . Halc' o n i d e g i v e s a r o y a l p u r p l e c o l o r w i t h b l u e t e t r a z o l i u m 3 ' and a yellow-brown c o l o r w i t h aluminum c h l o r i d e i n n i t r o m e t h a n e .
JOEL KIRSCHBAUM
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4.3
Chromatographic Analyses 4.31 High-pressure Liquid Chromatography (HPLC)
Reverse phase high-pressure liquid chromatography is used to separate and quantitate bulk and formulated h a l ~ i n o n i d e . ~Commercially ~ available, prepacked octadecylsilane columns, 10 pm in particle size, United S t a t e s Phamacopeia designation L-1 (such as Partisil, MicroPak or UBondapak), are used. The mobile phase is aqueous acetonitrile (1:l to 1:3) with a flow rate of 0.3 to 1.0 mL/min. Detection is at 254 nm. Figure 7 shows the elution of halcinonide and progesterone internal standard. Using a precision loop injector, repetitive injections gave a relative standard deviation of 0.6%. Without the progesterone internal standard, the relative standard deviation is 0.8%. Formulated halcinonide, in concentrations of 1 to 0.25 mg steroidlg, is either diluted with mobile phase, extracted into methanol, or partitioned into aqueous acetonitrile from h e ~ a n e 9s56. ~ ~ Halcinonide can be separated from kenalogl’ (triamcinolone acetonide) by HPLC.57 Intermediates in the synthesis of halcinonide (cf. section 1.5) have the following relative retention times; Dihydrotriamcinolone, RRT = 0.18;dihydrotriamcinolone acetonide, RRT = 0.32, and dihydrotriamcinolone acetonide-21~ purity . mesylate, RRT = 0.72 (Halcinonide, RRT = ~ 0 0 ) ~The of dihydrotriamcinolone can be determined by HPLC using the same reverse phase column and a mobile phase consisting of 0.8% ammonium nitrate, 0.23% monobasic ammonium phosphate, 32.5% methanol, 8% tetrahydrofuran and water.58 Cortisone acetate is used as an internal standard.59 Impurities are determined at a higher concentration.
HALCINONIDE
273
Halcinonide
Progesterone
+r Figure 8 R e v e r s e P h a s e H i g h - p r e s s u r e L i q u i d Chromatography of H a l c i n o n i d e . P r o g e s t e r o n e i s u s e d as i n t e r n a l s t a n d a r d . See t e x t f o r d e t a i l s .
JOEL KIRSCHBAUM
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4.32
Thin Layer Chromatography (TLC)
TLC, using silica gel GF 254 plates, can separate halcinonide from its synthetic precursors (cf. section 1.5). Using a developing solvent of chloroform60 ethyl acetate (5:1), the following Rf values were found : Dihydrotriamcinolone, Rf = 0.0; dihydrotriamcinolone acetonide, Rf = 0.08; dihydrotriamcinolone acetonide-21-mesylate, Rf = 0.18 and halcinonide, Rf = 0.36. Continuous TLC development gives respective relative Rf values of 0.02, 0.02, 0.48 and 1.0. With benzene (CAUTION)-acetone-water (70:30:07) the respective Rf values are 0.12, 0.42, 0.66 and 0.81. Traces of these intermediates have been found in some lots of halcinonide, as has dihydrotriamcinolone-2l-acetate, an impurity occasionally found in some preparations of dihydrotriamcinolone. Elution from the TLC plate with ethanol permits quantitation of bulk halcinonide and halcinonide extracted from formulations. ‘C-Halcinonide (labelled at the acetonide carbon) was examined for impurities using silica gel TLC plates and chloroform-ethyl acetate (5 :1)61 mobile phase. The Rf value of halcinonide is 0.5. 4.33
Column Chromatography
A diatomaceous earth column was used to separate halcinonide from excipients62 The formulation is mixed with column packing material and then is transferred to the top of the column. Steroidal material is eluted with benzene (CAUTION) under a well-ventilated hood and then quantitated using thin layer chromatography60 or tetramethylammonium hydroxide51 colorimetry
.
.
4.34 Paper Chromatography Paper chromatography using Whatman No. 1 paper was once used to determine the homogeneity of halcinonide.60 Twenty percent formamide in methanol comprises one stationary phase and methylisobutyl ketone-formamide ( 2 0 : l ) is the mobile phase. A second solvent system uses 25% propylene glycol-chloroform as the stationary phase and toluene saturated with propylene glycol as the mobile phase.
4.4 Polarographic Analysis In dimethylformamide, halcinonide is reduced in two steps.63 The 2la-chloroketo group exhibits a halfwave reduction potential of -1.17 volts U S Hg. This is easily distinguished from the half-wave potential of -1.62 volts 2)s Hg of the A4-3-keto group. Thus, halcinonide can be
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a s s a y e d i n t h e p r e s e n c e o f o t h e r 4-ene-3-keto steroids that l a c k t h e 21-chloro group. This response r e q u i r e s a concentrat i o n between 0.5 and 2.0 d of s t e r o i d p e r l i t e r . The more s e n s i t v e t e c h n i q u e of d i f f e r e n t i a l p u l s e p ~ l a r o g r a p h y ~ ~ should a l s o b e a p p l i c a b l e t o halcinonide. 4.5
Halcinonide
&-I T i s s u e s
and Body F l u i d s
The a n t i i n f l a m m a t o r y p r o p e r t i e s of s u c h t o p i c a a g e n t s a s h a l c i n o n i d e are u s u a l l y d e t e r m i n e d by a vasoconstrictor assay. Topically applied corticosteroids c a u s e a b l a n c h i n g a t t h e s i t e o f a p p l i c a t i o n , which c a n b e t h e forearm65 o r t h e u p p e r back of h e a l t h y a d u l t s where s t r a t u m corneum i s removed w i t h c e l l o p h a n e t a p e . 6 6 The t e s t a r e a s , c o n t a i n i n g v a r i o u s c o n c e n t r a t i o n s of h a l c i n o n i d e , are o c c l u d e d w i t h p l a s t i c wrap and are e v a l u a t e d on a n a l l - o r P e r c u t a n e o u s a b s o r p t i o n s t u d i e s 6 7 w i t h 0.1% none b a s i s . 1 4 C - h a l c i n o n i d e cream, 1 g cream p e r dog o r r a b b i t , showed t h a t t h e s t e r o i d i s absorbed through intact o r abraded s k i n . I n d o g s , 0 . 4 t o 0.5% i s e s t i m a t e d t o b e a b s o r b e d t h r o u g h In rabbits, 6 t o i n t a c t and 4 t o 10%t h r o u g h a b r a d e d s k i n . 16% of t h e 4 C - h a l c i n o n i d e w a s a b s o r b e d t h r o u g h i n t a c t and 1 4 t o 23% t h r o u g h a b r a d e d s k i n . Metabolism68 w a s s t u d i e d w i t h h a l c i n o n i d e l a b e l l e d w i t h carbon-14 i n t h e 2 - p o s i t i o n of t h e a c e t o n i d e It w a s a d m i n i s t e r e d i n t r a v e n o u s l y t o dogs a t a d o s e group. The m a j o r p o r t i o n o f t h e r a d i o a c t i v i t y w a s o f 5 mg/kg. excreted i n b i l e . Radio-autography of b i l e showed a t l e a s t 10 d i s t i n c t m e t a b o l i t e s t o be p r e s e n t . Four of t h e metabol i t e s were i d e n t i f i e d . The two most a b u n d a n t m e t a b o l i t e s , t h a t were i d e n t i f i e d , a c c o u n t e d f o r 43% ( F i g u r e 8 , M1) and 30%(M2) o f t h e r a d i o a c t i v i t y . The two minor m e t a b o l i t e s (M3 and M4) a c c o u n t e d f o r 2% e a c h . I n dog u r i n e , t h e s e f o u r m e t a b o l i t e s (Ml-4) a c c o u n t e d f o r 1 0 , 1 5 , 5 and 18% o f t h e radioactivity, respectively. I n dog b l o o d , unchanged h a l c i n o n i d e and m e t a b o l i t e s M3 and M4 e a c h a c c o u n t e d f o r a b o u t M 1 and M2 w e r e n o t d e t e c t e d . 15% of t h e r a d i o a c t i v i t y . These f o u r m e t a b o l i t e s , none of which c o n t a i n e d c h l o r i n e , were i d e n t i f i e d by comparing t h e i r u l t r a v i o l e t , n u c l e a r m a g n e t i c r e s o n a n c e o r mass s p e c t r a , and t h e i r t h i n - l a y e r c h r o m a t o g r a p h i c b e h a v i o r ( e i t h e r u n d e r i v a t i z e d , o r as a s u i t a b l e d e r i v a t i v e ) w i t h similar d a t a obtained f o r authent i c r e f e r e n c e s a m p l e s . M 1 w a s i d e n t i f i e d as t h e 21-carboxy d e r i v a t i v e of h a l c i n o n i d e (-CH2C1 + -C02H), M2 i s t h e 6Bhydroxy d e r i v a t i v e , M3 i s t h e 21-hydroxy d e r i v a t i v e (-CH2C1 -CH20H) and M4 i s t h e 66-hydroxy d e r i v a t i v e of M3. Figure 9 shows t h e p r o p o s e d pathway. M 3 i s t h e a c e t o n i d e d e r i v a -f
Figure 9 Proposed M e t a b o l i c Pathways f o r H a l c i n o n i d e i n t h e Dog.
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t i v e i n t h e s y n t h e s i s of h a l c i n o n i d e (cf. F i g . 2) and i t i s a l s o found a s a d e g r a d a t i o n p r o d u c t i n in vitro s t u d i e s summarized below. T h i s compound, d i h y d r o t r i a m c i n o l o n e a c e t o n i d e , p o s s e s s e s t o p i c a l and s y s t e m i c a n t i i n f l a m m a t o r y a c t i v i t y . 69
5.
Stability:
Halcinonide d i s s o l v e d i n e i t h e r methanol, deuterom e t h a n o l , a q u e o u s ammonia-methanol, o r d e u t e r i u m o x i d e d e u t e r a t e d ammonia-methanol s o l v e n t s a p p e a r s s t a b l e a f t e r s t o r a g e f o r s i x d a y s a t 50", u s i n g n u c l e a r m a g n e t i c r e s o n a n c e and mass s p e c t r o m e t r y . 70 Using t h i n l a y e r chromatography (cf. s e c t i o n 4 . 3 2 , f i r s t s y s t e m ) 6 0 no change w a s f o u n d i n two l o t s of h a l c i n o n i d e a f t e r But t h e s t o r a g e a t 50" f o r s i x months i n brown g l a s s b o t t l e s . d i r e c t e x p o s u r e t o 900 f o o t - c a n d l e s of l i g h t f o r one month c a u s e d a n i n c r e a s e i n i m p u r i t i e s of two l o t s from 0.5% t o 3.9% o r 4.9%. P h o t o l y t i c d e g r a d a t i o n of t h e A-ring i s e x p e c t e d s i n c e h y d r o c o r t i s o n e and p r e d n i s o l o n e u n d e r g o r e a r r a n g e m e n t s when s o l u t i o n s of t h e s e s t e r o i d s i n a l c o h o l a r e exposed t o u l t r a v i o l e t r a d i a t i o n o r o r d i n a r y f l u o r e s c e n t l i g h t i n g . 71-73 F o r m u l a t e d h a l c i n o n i d e , a t a c o n c e n t r a t i o n of 0.1% i n e i t h e r a cream b a s e o r p o l y e t h y l e n e g l y c o l - w a t e r l o t i o n , a f t e r s t o r a g e a t a p p r o x i m a t e l y 23" f o r 3 y e a r s , showed no l o s s o n h a l c i n o n i d e c o n t e n t , u s i n g h i g h p r e s s u r e l i q u i d chromatography. 4 6 The c o n t e n t s remained unchanged w i t h i n 2% of l a b e l e d concentration. One t r i a l f o r m u l a t i o n , s t o r e d a t 60" f o r 7 months showed d e g r a d a t i o n . 7 4 The one i m p u r i t y t h a t w a s i s o l a t e d and i d e n t i f i e d ( w i t h t h e a i d of mass s p e c t r o m e t r y ) i s d i h y d r o t r i a m c i n o l o n e a c e t o n i d e ( F i g u r e l), a n i n t e r m e d i a t e i n t h e s y n t h e s i s of halcinonide. T h i s compound a l s o p o s s e s s e s t o p i c a l a n t i i n f l a m matory a c t i v i t y . 69 6.
Acknowledgements
The a u t h o r g r a t e f u l l y acknowledges t h e c o u r t e o u s assist a n c e of t h e many c o n t r i b u t o r s c i t e d a s " p e r s o n a l communication." Some of t h e i n f o r m a t i o n c i t e d i n t h i s manner w a s e s p e c i a l l y obtained f o r t h i s analytical profile. Unless o t h e r w i s e i d e n t i f i e d , t h e work w a s done a t E. R . S q u i b b & S o n s , I n c . Much c r e d i t f o r t h i s p r o f i l e b e l o n g s t o D r . K l a u s F l o r e y , who wrote t h e o r i g i n a l one f o r u s e a t Squibb. S p e c i a l t h a n k s go to R . P o e t , G . B r e w e r , K . F l o r e y and S . Perlman f o r t h e i r c r i t i c a l r e a d i n g of t h i s MS, t o C . Pope f o r t y p i n g i t and t o my i a m i l y , f o r t h e i r p a t i e n c e d u r i n g t h e c o m p i l i n g of t h i s a n a l y tical profile.
JOEL KIRSCHBAUM
278
7.
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F. Bagatell and M. Augustine, Curr. Ther. Res., 26, 7 4 8 (1974).
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J. Fried and E. Sabo, J . Amer. Chem Soc., 75, 2273 (1953).
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R. C. Millonig and E. Yiacas i n "Pharmacological and Biochemical Properties of Drug Substances,'' M.E. Goldberg, editor, American Pharmaceutical Association, Washington, D.C., 1 9 7 7 , p. 215.
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Patent 3 , 0 4 8 , 5 8 1 , August 7 , 1 9 6 2 , to E. R. Squibb.
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Patent 3 , 8 9 2 , 8 5 7 ,
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U.S. Patent, 3 , 1 1 6 , 2 1 9 , Cyanamid.
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S. Bernstein, R. Lenhard, W. Allen, M. Heller, R. Littell, S. Stolar, L. Feldman, and R. Blank, J . h e r . Chem. SOC, 78, 5693 ( 1 9 5 6 ) .
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J.Z.
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P.T. Funke and A.I. Cohen, Personal Communication.
16.
M. Puar and A . I . Cohen, Personal Communication.
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HALCINONIDE
ProfiZes, 2, 397 ( 1 9 7 2 ) .
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K. F l o r e y , Ann.
18.
M.
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P . Grabowich, Personal communication.
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P. Valatin, Personal communication.
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united S t a t e s Pharmacopeia, 19, 6 5 1 ( 1 9 7 5 ) .
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H. Jacobson and V. Valenti, Personal communication.
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A. Dhruv, Personal communication.
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M. Augustine, J.M. Battaglia, C.G. Hughes and S. Perlman, Personal communications.
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N. Trandifir, Personal communication.
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A . Niedermayer,
Porubcan, Personal communication.
29, 6 ( 1 9 7 5 ) .
Perlman, Personal communication.
Personal communication.
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J. Bartos and M. Pesez, i n "Colorimetric and Fluorimetric Analysis of Steroids," Academic Press, New York, 1 9 7 6 .
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M. Pesez and J. Bartos i n "Colorimetric and Fluori-
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A.A. Forist and J.L. Johnson in "Pharmaceutical Analysis," T. Higuchi and E. Brochmann-Hanssen, Editors, Interscience Publishers (J. Wiley), New York, 1 9 6 1 , p.
67, 275 ( 1 9 7 8 ) .
metric Analysis of Organic Compounds and Drugs," Marcel Dekker, New York, 1 9 7 4 .
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L. Kerr and J. Kirschbaum, Personal communication.
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M. Kimura, T. Nishina, and T. Sakamoto, Chem. Pharm. B u l l . (Tokyo), l 5 , 4 5 4 ( 1 9 6 2 ) .
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E.P. Schulz, M. Diaz, G. Lopez, L. Guerrero, H. Barrera, A Pereda, and A. Aquilera, A n a l . Chem., 36, 1 6 2 4 (1964).
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E. Ivashkiv, Personal Communication.
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M. Pesez and J. Bartos in "Colorimetric and Fluorimetric Analysis of Organic Compounds and Drugs," Marcel Dekker, New York, 1 9 7 4 , p. 4 8 1 .
53.
S.
Berstein and R. Lenhard, J . Org. Chem., Z8,
1146
(1953). 54.
S. Gijr'cig and Gy. Szdsz in "Analysis of Steroid Hormone Drugs," Akadgmiai Kiadb, Budapest, 1 9 7 8 .
55.
J. Kirschbaum, R. Poet, K. Bush and G. Petrie, Personal communication.
HALCINON IDE
28 1
56.
J.E. Fairbrother i n "Assay of Drugs and Other Trace Compounds in Biological Fluids, Ed. by E. Reid, "Methodological Developments in Biochemistry, Vol. 5, Longman Group, London, 1976, p. 14 1.
57.
G. Gordon and P.R. Wood. (1977).
58.
W. Beyer, The Upjohn Company, Personal communication.
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J . Kirschbaum, Personal communication.
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H. Roberts, Personal communication.
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P. Egli, Personal communication.
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E. Ivashkiv and R. Poet, Personal communication.
63.
0. Kocy and C. Smith, Personal communication.
64.
R.N. Yadav and F.W. Teare, J . Pharm. Sci. 67, 436 (1978).
65.
A. McKenzie and R. Stoughton, A r c h . Derm., 86, 608
A n a l . Div. C h e m . SOC. 14, 30
(1962).
Brit. J . Derm., 6 9 , 11 (1957).
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G . Wells,
67.
A. Heald and C. Ita, Personal communication.
68.
K. Kripalani, A. El-Abdin, A . Dean and A. Cohen, Pharmacologist 29, 168 (1977) [Abs. No. 2401.
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L. Lerner, Personal communication.
70.
P. Funke and M. Puar, Personal communication.
71.
D. Barton and W. Taylor, J . C h e m . Soc. 2958, 2500.
72.
Ibid. J . Arner. C h e m . Soc., 8 0 , 244 1958.
73.
W. Hamlin, T. Chulski, P. Johnson and J . Wagner, J . h e r . Pharm. Assoc. ( S c i . Ed.! 4 9 , 253 (1963).
74.
K. Bush and G. Petrie, Personal communication. Literature reviewed to January 1, 1979.
Analytical Profiles of Drug Substances, 8
HYDRALAZINE HYDROCHLORIDE Chester E . Orzech, Norris G . Nash, and Raymond D. Daley
3. 4. 5. 6.
7. 8.
Description 1 . 1 Name, Formula, Molecular Weight I .2 Appearance, Color, Odor 1.3 History Physical Properties 2.1 Infrared Spectra 2 . 2 Ultraviolet Spectra 2.3 Mass Spectrum 2.4 Nuclear Magnetic Resonance Spectra 2.5 Differential Thermal Analysis (DTA) 2 . 6 Crystal Properties 2.7 Microchemical Characterization 2.8 Solubility 2 . 9 Dissociation Constants 2.10 Melting Points Synthesis Stability-Degradation Metabolism Methods of Analysis 6. I Identification Tests 6.2 Elemental Analysis 6 . 3 Spectrophotometric Methods 6 . 4 Fluorescence 6.5 Titration Methods 6.6 Gasometric Methods 6 . 7 Polarography 6.8 Paper chromatography 6 . 9 Thin-Layer Chromatography 6.10 High Pressure Liquid Chromatography 6.1 I Gas Chromatography Acknowledgments References
283
Copyright @ I979 by Academic Press. Inc. All rights of reproduction in any form reserved.
ISBN 0-12-260808-9
CHESTER E. ORZECH ET AL.
284
1.
DESCRIPTION
N a m e , Formula, Molecular Weight The Chemical A b s t r a c t s name f o r h y d r a l a z i n e hydroc h l o r i d e i s 1( 2H)-phthalazinone hydrazone monohydrochloride, s t a r t i n g w i t h volume 80; p r e v i o u s l y t h e name l-hydrazinop h t h a l a z i n e monohydrochloride w a s used. The CAS R e g i s t r y No. i s [304-20-1] f o r t h e h y d r o c h l o r i d e s a l t , [86-54-4] f o r t h e base. 1.1
NHNH2
I
C8H8N4OHC1
Molecular Weight:
196.64
Appearance, C o l o r , Odor Hydralazine h y d r o c h l o r i d e i s a white t o o f f - w h i t e o d o r l e s s c r y s t a l l i n e powder. 1.2
1.3
History The a b i l i t y of h y d r a l a z i n e and similar hydrazino compounds t o reduce blood p r e s s u r e w a s r e p o r t e d by Gross e t a1 ( 1 ) i n 1950. Methods of s y n t h e s i s were p u b l i s h e d by Druey and R i n g i e r ( 2 ) i n 1951, along w i t h t y p i c a l r e a c t i o n s d i s p l a y e d by t h e compound , i n c l u d i n g s e v e r a l r e a c t i o n s which l a t e r became t h e b a s e s f o r a n a l y s i s of h y d r a l a z i n e and i t s m e t a b o l i t e s . The drug h a s been widely used f o r t r e a t m e n t of h y p e r t e n s i o n , and p a p e r s on i t s p r o p e r t i e s and methods f o r i t s d e t e r m i n a t i o n have been p u b l i s h e d i n many languages. Hydralazine i s u s u a l l y used i n combination w i t h o t h e r drugs. In r e c e n t y e a r s , it h a s been found t o b e e s p e c i a l l y u s e f u l when used with b e t a - a d r e n e r g i c b l o c k i n g a g e n t s and d i u r e t i c s (3,4). 2.
PHYSICAL PROPERTIES 2.1
Infrared Spectra
The i n f r a r e d spectrum of h y d r a l a z i n e h y d r o c h l o r i d e (Figure I > w a s o b t a i n e d w i t h a Beckman IR-12 spectrophotometer. A mineral o i l d i s p e r s i o n between potassium bromide p l a t e s w a s scanned from 423 t o 4000 cm-1, and a t h i c k e r l a y e r of t h e d i s p e r s i o n , supported on p o l y e t h y l e n e f i l m ,
HYDRALAZINE HYDROCHLORIDE
was scanned from 200 t o 530 cm-’. bands can b e a s s i g n e d as f o l l o w s : Frequency, cm
-1
285
Some of t h e a b s o r p t i o n
Assignment ( 5 )
3220
N-H s t r e t c h
92.5
Aromatic C-H s t r e t c h
2800-3000
Mineral o i l C-H stretch
1590- 1600
C=C s t r e t c h
1460
Mineral o i l C-H band
785
Out of p l a n e bending,
4 adjacent
H atoms on an aromatic r i n g The m i n e r a l o i l a b s o r p t i o n a t 2800 t o 3000 cm-I and at 1460 cm- o b s c u r e s a b s o r p t i o n bands of h y d r a l a z i n e h y d r o c h l o r i d e at 2810, 2320, and 2970 cm-1 (N-H’ s t r e t c h ) and a w e a k s h a r p band a t 1470 cm-l; t h e s e bands can be observed i n potassium bromide d i s p e r s i o n s p e c t r a . The bands a t 1070 and 1082 cm-1 tend t o merge i n t o a s i n g l e band i n potassium bromide dispersion spectra. The i n f r a r e d spectrum of h y d r a l a z i n e h y d r o c h l o r i d e b a s e i n a potassium bromide d i s p e r s i o n ( F i g u r e 2 ) w a s recorded from 400 t o 4000 cm-1 , and t h e 200 t o 550 cm-1 region w a s o b t a i n e d from a m i n e r a l o i l d i s p e r s i o n s u p p o r t e d on p o l y e t h y l e n e f i l m . The s p e c t r a o f potassium bromide d i s p e r s i o n s of t h e b a s e a r e q u a l i t a t i v e l y i d e n t i c a l t o t h o s e of m i n e r a l o i l d i s p e r s i o n s . The assignment of a b s o r p t i o n bands i n t h e spectrum of t h e b a s e i s s i m i l a r + t o t h a t of t h e h y d r o c h l o r i d e except € o r t h e p r e s e n c e of N-H stretch a b s o r p t i o n i n t h e l a t t e r . A spectrum of t h e b a s e h a s been published ( 6 ) . 2.2
Ultraviolet Spectra F i g u r e 3 is t h e u l t r a v i o l e t a b s o r p t i o n spectrum of h y d r a l a z i n e h y d r o c h l o r i d e i n water s o l u t i o n , run on a Cary Model 14 spectrophotometer. The s o l u t i o n contained 9.9 mg of h y d r a l a z i n e h y d r o c h l o r i d e p e r l i t e r , and w a s run a g a i n s t water ( 1 cm c e l l s ) . The d i s c o n t i n u i t y i n t h e spectrum a t 219 nm i s a change of a b s o r p t i o n s c a l e ; t h e absorbance s c a l e range i s 0.0 t o 1.0 f o r t h e wavelength range 350 t o
rl rl
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.
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CHESTER E. ORZECH ET A L .
288
219 nm, and 1.0 t o 2.0 f o r t h e wavelength range 219 t o 200 nm. A scan of water a g a i n s t water i s a l s o recorded on t h e c h a r t . The spectrum e x h i b i t s m a x i m a a t 315, 303, 260, 239, and 211 nm, w i t h r e s p e c t i v e a b s o r p t i v i t i e s as f o l l o w s : 4,200; 5,200; 10,600; 11,000; 33,800 l./mole cm. Druey and Tripod ( 3 ) , Kuhnert-Brandstbtter e t al (71, Sharkey e t al ( 8 ) , and Solomonova e t al ( 9 ) r e p o r t e d similar m a x i m a and a b s o r p t i v i t i e s , except t h a t t h e y d i d Clarke (6) g i v e s d a t a not r e p o r t t h e 211 nm m a x i m u m . similar t o t h a t o f t h e above i n v e s t i g a t o r s . Sunshine ( 1 0 ) g i v e s t h e spectrum i n 0.1N h y d r o c h l o r i c a c i d , w i t h m a x i m a at 312, 302, 259, and 233 nm, and t h e spectrum i n 0.1N sodium hydroxide, w i t h m a x i m a at 304, 27.1, and 262 nm. Naik e t al (11) gave p a r t i a l u l t r a v i o l e t s p e c t r a of t h e b a s e , t h e monohydrochloride, and t h e d i h y d r o c h l o r i d e : ( a ) t h e b a s e e x h i b i t e d m a x i m a a t 305 and 273 nm, w i t h a t h i r d maximum n e a r 262 nm; ( b ) t h e monohydrochloride e x h i b i t e d m a x i m a a t 315, 302, 2'30, and 260 nm; ( c ) t h e d i h y d r o c h l o r i d e e x h i b i t e d a m a x i m u m a t 318 nm w i t h a broad The Merck Index (12) l i s t s s h o u l d e r a t about 300 nm. m a x i m a at 315, 304, 260, 240, and 211 nm f o r t h e aqueous s o l u t i o n of t h e hydrochloride. 2.3
Mass Spectrum F i g u r e 4 shows t h e low r e s o l u t i o n mass spectrum of h y d r a l a z i n e hydrochloride. The d a t a were o b t a i n e d with an LKB 9000s mass s p e c t r o m e t e r , w i t h an i o n i z a t i o n voltage of 70 eV, s o u r c e temperature z O o C . Some of t h e peaks m a y b e a s s i g n e d as f o l l o w s ( 1 3 ) :
Mass Charge R a t i o
Assignment
160
M+
129
M
+-
.NH-NH,
103
t
76
C6H4
51
C4H3
36/38
HC1'
+
! -I f :.I-:
. .
.
.
.
,
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.-
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. . .
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.
. .
..
. . . . . . .
# -;
.
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. . . . . .
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.
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I
A l I S N 3 1 N I 3A11Vl31J
0
a,
a
0
k
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0
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d
k a
HYDRALAZIN E HYDROCHLORIDE
29 I
2.4
Nuclear Magnetic Resonance S p e c t r a The NMR spectrum shown i n F i g u r e 5 w a s o b t a i n e d by d i s s o l v i n g h y d r a l a z i n e h y d r o c h l o r i d e i n deuterium oxide c o n t a i n i n g 3- ( t r i m e t h y l s i l y 1 ) - I-propane-sulfonic a c i d sodium s a l t ( E X ) . The s e r i e s of p e a k s a t 0 , 0.6, 1.8, and 3 ppm are all due t o t h e WS. The peak a t 4.8 pprn i s due t o HDO which forms on exchange w i t h t h e s o l v e n t and t h e p e a k s at 8.01 and 8.61 ppm a r e due t o t h e a r o m a t i c p r o t o n s . The N M R spectrum of t h e b a s e ( F i g u r e 6 ) w a s o b t a i n e d i n a 1 :1 mixture of dirnethylsulfoxide-d :deuterochloroform. The p e a k s a t 2.53 ppm a r e due t o t 8 e s o l v e n t . The N-H p r o t o n s a r e a t 4.1 pprn and t h e aromatic p r o t o n s a r e a t 7.6 and 8 ppm. The s p e c t r a were produced u s i n g a Varian EM-360 NMR s p e c t r o m e t e r .
2.5
D i f f e r e n t i a l Thermal A n a l y s i s (IYTA) The DTA c u r v e s i n F i g u r e s 7 and 8 were o b t a i n e d with a W o n t Model 900 instrument. F i g u r e 8 shows t h a t t h e b a s e m e l t s s h a r p l y and F i g u r e 7 shows t h a t t h e hydroc h l o r i d e melts w i t h decomposition. V i s u a l l y t h e hydroc h l o r i d e melts at 274"C, b u t decomposition t a k e s p l a c e o v e r a l a r g e t e m p e r a t u r e range ( F i g u r e 7).
2.6
Crystal Properties Chojnacki e t a1 ( 1 4 ) i n v e s t i g a t e d t h e c r y s t a l p r o p e r t i e s of h y d r a l a z i n e hydrochloride. Recrystallized from water, t h e c r y s t a l s were found t o be monoglinic, w i t h t h e u n i t c e l l a = 9.408, b = 14.529, c = 6.643A, p = 103.59", Z = 4. The c a l c u l a t e d d e n s i t y w a s 1.486, t h e measured d e n s i t y 1.479 g p e r cm3. The s p a c e group w a s P21/c. Powder d i f f r a c t i o n d a t a , g e n e r a l l y similar t o t h a t of Table 1, i s a l s o given. X-ray powder d i f f r a c t i o n d a t a f o r h y d r a l a z i n e h y d r o c h l o r i d e and h y d r a l a z i n e b a s e are g i v e n i n Table 1. These d a t a were o b t a i n e d with a Norelco d i f f r a c t o m e t e r u s i n g n i c k e l - f i l t e r e d copper Ka r a d i a t i o n . 2.7
Microchemical C h a r a c t e r i z a t i o n S a n d r i (15) r e p o r t e d t h e formation of c h a r a c t e r i s t i c c r y s t a l s w i t h cadmium bromide-hydrobromic a c i d , bismuth iodide-potassium i o d i d e , and bismuth bromide-hydrobrornic a c i d , with compositions CdBr -HBr*C H N - 4 H 2 0 , ~ i I q - c 8 H ~ N 4and , HEiiBr - C H N r e s2p e c t i v e8l y8. 4 u h n e r t - B r a n d s4t s*t e r e al ( 7 ) r e p o r t e d t h e micros c o p i c h o t - s t a g e c h a r a c t e r i z a t i o n of h y d r a l a z i n e hydroc h l o r i d e . Above 21OoC, small r o d s , g r a n u l e s , and p r i s m s sublime. The m e l t i n g p o i n t i s 268-a5"C. G a s bubbles are evolved as m e l t i n g b e g i n s , and m e l t i n g p r o c e e d s w i t h
9 41
CHESTER E. ORZECH ET A L .
292
TABLE 1 X-RAY POWDER DIFFRACTION PATTERNS OF HYDRALAZINE HYDROCHLORIDE AND HYDRALAZINE BASE Hydrochloride Base 0
0
7.74 7-25 5-92 5-54 4.82 4.62 4.37 3.99 3.87 3-63 3.39 3-38 3-32 3 - 29
3.22 3-15 3-05 2-99 2-95 2-93 2.85 2-77 2.72 2.64 2.58 2.44 2.41 2-39 2.34 2.24 2.22
2.18 2.16 2.10
2.06 2.02
1.99 1-97 I .94 1.89
-
d(A)
d(A)
100
93 9 2 2
18 47 15
12
54 9 11
31 65 92 7 9 4 2 2
6
22 2 2
4 7
2 1
16
2 2 2 2
3
2 1 2
4 4
2
7.37 5-87 5.62 5.04 4.86 4.48 3.98 3.74 3.66 3.47 3.28 3.24 3-12 2.96 2.80 2.7 1 2.67 2.60 2.49 2.44 2.38 2-30
2.28 2.25 2.18
2.12
2-07 2.04 1-99 1.95 1.87 I .85 1.83 1-79 I .78 1.76 1.72 1.67 1.62
100
11
49 11
17 18
2
10
2
15
100
17
11 2
7
1 2 2 2 2 1 2 1 2 1
3
2
3
1 2 2 1 1 1 1 1
3 1
1
293
HYDRALAZINE HYDROCHLORIDE
1
I
1
10
8
9
Figure
5.
1
1
7
6
1
1
1
1
5 4 PPY (61
2
3
I
Nuclear Magnetic Resonance Spectrum of Hydralazine
Hydrochloride.
1
1
1
1
I
I
I
1
I
1
1
10
9
0
7
6
5
4
3
2
I
0
PPY 16)
Figure
6.
Nuclear Magnetic Resonance Spectrum of Hydralazine Base.
h)
P
Figure 7.
D i f f e r e n t i a l Thermal Analysis Curve of Hydralazine Hydrochloride.
Figure 8.
D i f f e r e n t i a l Thermal Analysis Curve of Hydralazine Base.
CHESTER E. ORZECH ET A L .
296
t h e separation of high melting (over 300°C) needles and bushlike aggregates. The e u t e c t i c temperature with p-acetamidophenyl s a l i c y l a t e was 181 "C, with dicyandiami.de 162°C. The p i c r a t e salt forms from aqueous s o l u t i o n as long needles and columns t h a t melt a t 210 t o 212°C with decomposition. The styphnate forms needles and r o s e t t e s with a melting point of 200 t o 203°C. Sunshine (10) and Clarke ( 6 ) give two microc r y s t a l t e s t s , both from aqueous s o l u t i o n : ( a ) l e a d iodide-potassium a c e t a t e reagent forms dense r o s e t t e s ; (b) iodine-potassium i o d i d e ( 1 :5O) reagent forms c l u s t e r s or masses of needles.
2.8
Solubility The Merck Index (12) g i v e s t h e s o l u b i l i t y i n water as 9 . 1 mg p e r m l at 15"C, and 44.2 mg p e r m l a t 25°C. In 95% ethanol, t h e s o l u b i l i t y i s given as 2 mg p e r ml. These a r e consistent with t h e following approximate s o l u b i l i t y d a t a , determined at room temperature: Solvent Water
Approximate S o l u b i l i t y , mg/ml
39
Methanol
6 -7
Ethanol (95%)
1-9
2-Propanol
0.1
Chloroform
< 0.1
Ethyl e t h e r (anhydrous)
< 0.1
Ethyl a c e t a t e
< 0.1
Acet oni t r i l e
< 0.1
2.9
Dissociation Constants Evstratova and Ivanova (16) reported a pKa of 7.1. Evstratova e t a1 (17) reported a pK of 7.1 i n water, a a pK of 4.7 i n aqueous 90 percent acetone, and a p\ of 15.6 inathe l a t t e r solvent. N a i k e t a1 (11) reported a pK of 6.9 for t h e d i s s o c i a t i o n of t h e monohydrochloride anda0.5 f o r d i s s o c i a t i o n of t h e dihydrochloride, determined absorptiometrically. Artamanov et al reported a pKa of 7.2 (18).
HYDRALAZINE HYDROCHLORIDE
297
2.10 Melting P o i n t s The m e l t i n g p o i n t of h y d r a l a z i n e h y d r o c h l o r i d e i s n e a r n3"C, t h a t of t h e b a s e i s n e a r 173°C. Melting p o i n t s r e p o r t e d i n t h e l i t e r a t u r e a r e as f o l l o w s : Melting P o i n t of Hydrochloride ( a ) ,
no -
OC
280
(3,191
,
273 271
( 2 , s 21 ,22,23 )
-
272
(24)
(25)
265
273
Reference
-
(26)
274
( a ) The h y d r o c h l o r i d e m e l t s w i t h decomposition. Melting P o i n t of Base, 172
173
Reference (2,21,22)
165 - 172
(24)
172
(25)
173
3.
-
OC
-
175
(27)
SYNTHESIS
Hydralazine has been p r e p a r e d by v a r i o u s p r o c e d u r e s from I - c h l o r o p h t h a l a z i n e ( 2 , 2 1 , 2 2 , 2 4 , 2 8 ) , p h t h a l a z i n e - l t h i o n e (20,23,25), 1 , 4 - d i c h l o r o p h t h a l a z i n e (29,30,31), I-(methylsulfony1)-phthalazine (271, o r 1-cyano-2-benzal a c e t a t e (26). Phthalazone, used t o p r e p a r e l-chlorop h t h a l a z i n e , h a s been p r e p a r e d from naphthalene (3,281 o r from p h t h a l i c anhydride ( 3 ) . A comprehensive survey on h y d r a z i n o p h t h a l a z i n e s and r e l a t e d compounds h a s been p u b l i s h e d by Druey and Tripod ( 3 ) . Some of t h e s e p r o c e d u r e s a r e o u t l i n e d i n F i g u r e s 9 and 10.
4.
STABILITY
-
DEGRADATION
Hydralazine h y d r o c h l o r i d e i s q u i t e s t a b l e as t h e c r y s t a l l i n e s o l i d . A t room t e m p e r a t u r e , it i s s t a b l e i n In aqueous d i s t i l l e d water s o l u t i o n f o r weeks (32).
ri V
&Jo
298
-1
E XN
O&7
0 V
0 X
0
(H
aCN H( OAC 1
I
HNNH
Figure 10.
-
c1 Several Syntheses f o r Hydralazine.
ci
CHESTER E. ORZECH E7 A L .
300
s o l u t i o n w i t h a pH g r e a t e r t h a n 7 , h y d r a l a z i n e decomposes, forming p h t h a l a z i n e ; t h e r a t e of decomposition depends on pH, t e m p e r a t u r e , and t h e k i n d and c o n c e n t r a t i o n of anion p r e s e n t (33). I n b i o l o g i c a l samples t h e drug d i s a p p e a r s r a p i d l y a t room temperature, a p p a r e n t l y by enzymatic r e a c t i o n s . The hydrazino group i s h i g h l y r e a c t i v e , forming It i s a l s o a hydrazones w i t h aldehydes and ketones. reducing a g e n t , and i t forms complexes w i t h many metal i o n s (34). A t 275 t o 280°C i t decomposes t o h y d r a z i n e , ammonia, n i t r o g e n , and 1 , k d i h y d r o - l , 1 ' - b i p h t h a l a z i n e (35).
5.
METABOLISM
Hydralazine h y d r o c h l o r i d e i s r a p i d l y metabolized and excreted. Experiments w i t h carbon-14 l a b e l e d drug i n humans i n d i c a t e d t h a t l e s s t h a n 10 p e r c e n t of t h e i n t a c t drug was e x c r e t e d (36). Within 5 days a f t e r a dose, 83 t o 89 p e r c e n t was e x c r e t e d i n t h e u r i n e and 9 t o 12 p e r c e n t i n t h e f e c e s . Of t h e m a t e r i a l e x c r e t e d i n t h e u r i n e , 96 p e r c e n t w a s recovered i n t h e first 24 hours. Individuals who are slow a c e t y l a t o r s e x h i b i t h i g h e r h y d r a l a z i n e blood l e v e l s t h a n f a s t a c e t y l a t o r s , f o r t h e same dose (37). Reported metabolic p r o d u c t s of h y d r a l a z i n e i n v a r i o u s s p e c i e s are as follows: Metabolite
I.
3-Methyl-s-triazolo !3,I t d p h t h a l a z i n e
Species Man
Rat
11.
111. IV.
Reference (36,37,38,39, 40,41,42,43,44) (3,39,43,45,
46 1
Guinea p i g Rabbit Pigeon
(45) (38 1
N- ( I-Phthalaziny1)hydrazone of p y r u v i c acid
Man
(36,38,47,85 ) (38,46) (38)
N- ( 1-Phthalaziny1)hydrazone of acetone
Man Rat
(47) (44,461
N- ( 1-Phthalaziny1)hydrazone of aketoglutaric acid
Man
(47)
Rat Rabb i t
(45)
HYDRALAZINE HYDROCHLORIDE
30 I
s-Triazolo[3,4al phthalazine
Man
VI.
1(2H)-Phthalazinone
Man Rat
VII.
Phthalazine
Man
(37)
Rat
(46)
4- ( 2-Acetylhydrazino )phthalazinone Man
(36)
9-Hydroxy-3-methyl-striazol0[3,4a! phthalazine Man
(36)
V.
VIII.
IX.
X.
3-Hydroxymethyl-striazolot3,4a! phthalazine
Rat
Man Rat
In c a s e s where t h e m e t a b o l i t e s above p o s s e s s s u i t a b l e f u n c t i o n a l g r o u p s , t h e y a r e u s u a l l y e x c r e t e d as g l u c u r o n i d e s or s u l f a t e s . F i g u r e 11 i s a scheme i l l u s t r a t i n g t h e metabolism of h y d r a l a z i n e , based p r i m a r i l y on t h o s e proposed by Haegele e t al ( 4 6 ) and Wagner e t a1 (36).
6.
METHODS OF ANALYSIS
6.1
Identification Tests Hydralazine h y d r o c h l o r i d e can be e a s i l y i d e n t i f i e d by t h e p h y s i c a l p r o p e r t i e s d e s c r i b e d i n S e c t i o n 2 above. Where i d e n t i f i c a t i o n o f h y d r a l a z i n e i n f o r m u l a t i o n s i s n e c e s s a r y , t h e f o l l o w i n g t e s t s may b e u s e f u l . Cooper ( 4 9 ) used s p o t t e s t s on p a p e r , r e a c t i n g f e r r i c i o n or dirnethylarninobenzaldehyde w i t h t h e unknown. The i r o n r e a g e n t y i e l d s a b l u e c o l o r , and dimethylaminobenzaldehyde an orange c o l o r . The r e s u l t s o b t a i n e d w i t h 95 o t h e r d r u g s a r e given. Belikov e t a1 (50)d e s c r i b e d t h r e e r e a c t i o n s t o i d e n t i f y hydralazine. Sodium n i t r o p r u s s i . d e r e a c t s w i t h an a l k a l i n e aqueous s o l u t i o n of h y d r a l a z i n e t o y i e l d a r e d c o l o r ; when t h e m i x t u r e c o n t a i n s m i n e r a l a c i d s , a g r e e n p r e c i p i t a t e i s formed, b u t w i t h a c e t i c a c i d , a r e d p r e c i p i t a t e i s formed. Cinnamaldehyde r e a c t s w i t h a h y d r o c h l o r i c a c i d s o l u t i o n of h y d r a l a z i n e t o g i v e a y e l l o w p r e c i p i t a t e , m.p. 197-200"C. p-Nitrobenzaldehyde r e a c t s w i t h a n
/
z-2 EN'
K)
X
vb-=
w
3
w
&L 8 );i
V X
1:
2 - 2 4
302
'H 0
O t
2-2
1
m
R-R?
P
H H
gg 303
CHESTER E. ORZECH ET AL.
304
aqueous s o l u t i o n of h y d r a l a z i n e t o g i v e an orange p r e c i p i t a t e , m.p. 260-26I0C. Modras ( 5 1 ) r e p o r t e d s p o t t e s t r e a c t i o n s t o d i f f e r e n t i a t e h y d r a l a z i n e from c l o s e l y r e l a t e d drugs. Reagents used were aqueous copper (I) c h l o r i d e , aqueous ammonium molybdate, i o d i n e i n potassium i o d i d e s o l u t i o n , aqueous c o b a l t (11) n i t r a t e , a l c o h o l i c n i n h y d r i n , and a l c o h o l i c bromophenol b l u e . The t e s t s were performed on paper o r on S i l i c a G e l G. Roshchenko e t al ( 5 2 ) r e a c t e d h y d r a l a z i n e w i t h p ,p'-dichlorobenzene sulfonamidate sodium i n water at 80 t o 90°C t o produce a c r y s t a l l i n e p r e c i p i t a t e C H 0 N S C 1 20.17452 2 with a m e l t i n g p o i n t of 196-197"C. I n t h e USP ( 1 9 ) method f o r i d e n t i f y i n g h y d r a l a z i n e i n t a b l e t s and i n j e c t i o n s , o-nitrobenzaldehyde i s added t o form an orange p r e c i p i t a t e . S t o h s and S c r a t c h l e y ( 5 3 ) used t h i n l a y e r chromatography t o i d e n t i f y h y d r a l a z i n e i n dosage forms and b i o l o g i c a l f l u i d s ( s e e S e c t i o n 6.8). 6.2
Elemental Analyses The elemental compositions of h y d r a l a z i n e hydroc h l o r i d e and h y d r a l a z i n e b a s e are as f o l l o w s :
Element
Hydrochloride Calculated Found(2)
Base Calculated Found( 2)
48.87
48 -99
59.99
---
Hydrogen
4.61
4.83
5 -03
---
Nitrogen
28.49
28-39
34.98
35 -09
Chlorine
18.03
18.17
---
---
Carbon
Spe ct rop ho t omet r i c Methods Solomonova e t al ( 9 ) determined h y d r a l a z i n e i n t a b l e t s by a d i r e c t u l t r a v i o l e t a b s o r p t i o n method. Although t h e compound can b e e x t r a c t e d from f o r m u l a t i o n s with a l c o h o l o r w a t e r , o t h e r components of t h e m i x t u r e may i n t e r f e r e w i t h d i r e c t u l t r a v i o l e t a b s o r p t i o n measurement by c o n t r i b u t i n g t o t h e observed a b s o r p t i o n . The s o l u t i o n s u s u a l l y cannot be cleaned up by e x t r a c t i o n t e c h n i q u e s because h y d r a l a z i n e decomposes i n a l k a l i n e s o l u t i o n . However, t h e r e a r e many r e a c t i o n s t h a t g i v e r i s e t o n e a r u l t r a v i o l e t o r v i s i b l e a b s o r p t i o n bands s u i t a b l e f o r quant i t a t i on.
6.3
305
HYDRALAZINE HYDROCHLORIDE
A f r e q u e n t l y r e p o r t ed s p e ct ropho t omet r i c t e c h i que f o r t h e d e t e r m i n a t i o n of h y d r a l a z i n e i s based on r e a c t i o n s with a r o m a t i c aldehydes t o form hydrazones w i t h a b s o r p t i o n i n t h e v i s i b l e region. Luk'yanchikova e t al ( 5 4 ) used p-nitrobenzaldehyde; Wesley-Hadzi j a and Abaffy (55) and Ruggieri (56 ) used p-dimethylaminobenzaldehyde; Luk'yanchikova (57,581 used cinnamaldehyde; S c h u l e r t (33) used p-hydroxybenzaldehyde; and Zak e t al ( 5 9 ) used p-methoqbenzaldehyde, a f t e r t e s t i n g cinnamaldehyde, s a l i c y l a l d e h y d e , 3,4,5- t r i m e t h o q b e n z a l d e h y d e , and I-napht haldehyde P e r r y (32), and Grabowicz and B r u l i n s k a (60)used n i n h y d r i n t o o b t a i n a s o l u t i o n w i t h an a b s o r p t i o n maximum n e a r 450 nm. E l l e r t and Modras (61 ) t r e a t e d h y d r a l a z i n e w i t h f e r r o u s i o n i n a l k a l i n e s o l u t i o n , and measured t h e c o l o r produced a t 540 nm. Ruggieri (56) r e p o r t e d a c o l o r i m e t r i c t e s t u s i n g 2-naphthoquinonesulfonate sodium t o form a r o s e - v i o l e t color. Urbanyi and O'Connell (62,63)developed an automated c o l o r i m e t r i c method u s i n g b l u e t e t r a z o l i u m f o r t h e a n a l y s i s of h y d r a l a z i n e i n t h e p r e s e n c e of r e s e r p i n e and hydrochlorothiazide.
.
6.4
Fluorescence N a i k e t al (11) e x t r a c t e d h y d r a l a z i n e hydroc h l o r i d e from t a b l e t s w i t h 50 p e r c e n t aqueous methanol and mixed a p o r t i o n of t h e e x t r a c t w i t h 99 volumes of concent r a t e d s u l f u r i c a c i d t o o b t a i n f l u o r e s c e n c e a t 353 nm w i t h e x c i t a t i o n a t 323 nm. The f l u o r e s c e n c e i n t e n s i t y v a r i e d l i n e a r l y w i t h c o n c e n t r a t i o n i n t h e range 2 t o 8 pg hydralazine hydrochloride p e r m l . I n j e c t i o n s were analyzed similarly.
6.5
T i t r a t i o n Methods Ruggieri (56) r e p o r t e d t i t r a t i n g h y d r a l a z i n e w i t h p e r c h l or i c a c i d Ruzhentseva e t a1 ( 6 4 ) converted h y d r a l a z i n e t o ammonia by h e a t i n g with z i n c i n s u l f u r i c a c i d , forming 3 moles of ammonia p e r mole of h y d r a l a z i n e . The m i x t u r e w a s made a l k a l i n e and t h e ammonia w a s d i s t i l l e d i n t o b o r i c a c i d s o l u t i o n , which w a s t h e n t i t r a t e d . S a n d r i ( 1 5 ) t e s t e d t h r e e t i t r a t i o n methods w i t h good r e s u l t s . One was t i t r a t i o n w i t h potassium bromate i n t h e p r e s e n c e of potassium bromide and h y d r o c h l o r i c a c i d , u s i n g a s t a r c h - i o d i n e end-point. Another w a s a d d i t i o n of e x c e s s p e r i o d i c acid-potassium i o d i d e with sodium
.
306
CHESTER E. ORZECH ET AL.
thiosulfate back-titration. The t h i r d w a s a d d i t i o n of sodium hydroxide and a c o n c e n t r a t e d s o l u t i o n of potassium f e r r o c y a n i d e , then a c i d i f y i n g and t i t r a t i n g with potassium permanganat e s o l u t i o n . P e r e l 'man and Evst rat ova (65 ) t i t r a t e d h y d r a l a z i n e h y d r o c h l o r i d e i n dimethylformamide s o l u t i o n t o a p o t e n t i o m e t r i c end-point w i t h sodium methoxide s o l u t i o n . Artamanov e t a1 (18) determined h y d r a l a z i n e h y d r o c h l o r i d e by conductometric t i t r a t i o n with sodium hydroxide s o l u t i o n . Goryacheva and Prikhodkina ( 6 6 ) t i t r a t e d hydralaz i n e from t a b l e t s w i t h N-bromosuccinimide s o l u t i o n . One mole of h y d r a l a z i n e h y d r o c h l o r i d e w a s e q u i v a l e n t t o 2 moles of N-bromosuccinimide. Methyl r e d was used as t h e indicator. Soliman and B e l a l i n v e s t i g a t e d a r g e n t i m e t r i c (67,681 and m e r c u r i m e t r i c (69) methods. Hydralazine p r e c i p i t a t e s s i l v e r from ammoniacal s i l v e r n i t r a t e s o l u t i o n . The s i l v e r i s d i s s o l v e d w i t h h o t n i t r i c a c i d and t i t r a t e d w i t h ammonium t h i o c y a n a t e s o l u t i o n . A l t e r n a t i v e l y , mercury i s p r e c i p i t a t e d from a l k a l i n e potassium mercuric i o d i d e s o l u t i o n . The p r e c i p i t a t e d mercury i s d i s s o l v e d by adding e x c e s s s t a n d a r d i o d i n e s o l u t i o n . The excess i o d i n e i s b a c k - t i t r a t e d w i t h sodium t h i o s u l f a t e solution a f t e r acidifying with a c e t i c acid. USP X I X d i r e c t s t h a t h y d r a l a z i n e b e determined i n t h e raw material, t a b l e t s , and i n j e c t i o n s by potassium i o d a t e t i t r a t i o n i n s t r o n g l y a c i d s o l u t i o n , u s i n g chloroform t o d e t e c t t h e p r e s e n c e of i o d i n e (19).
6.6
Gasometric Methods McKennis and Yard (70) s t u d i e d t h e n i t r o g e n e v o l u t i o n from a s e r i e s of hydrazino compounds when t r e a t e d w i t h 0.0% K I O i n 0.z H 04 i n a Warburg a p p a r a t u s at 37OC. I n an aqueous 3 s o l u i o n , h y d r a l a z i n e r e l e a s e d 102 p e r c e n t of t h e t h e o r e t i c a l amount of n i t r o g e n i n I5 minutes. Viala (71) determined h y d r a l a z i n e i n s o l u t i o n s o r t a b l e t s by measuring t h e n i t r o g e n f r e e d from t h e hydrazine group, u s i n g potassium permanganate i n s u l f u r i c a c i d , o r i o d i n e i n sodium b i c a r b o n a t e s o l u t i o n .
B
6.7
Polarographx P o l a r o g r a p h i c s t u d i e s o f h y d r a l a z i n e and r e l a t e d compounds were r e p o r t e d by Giovanoli-Jakubezak e t a1 (72) and by Modras ( 7 3 ) . The r e d u c t i o n p r o c e e d s i n two 2-electron s t a g e s w i t h t h e formation of t h e t e t r a h y d r o d e r i v a t i v e . Hydralazine could b e determined i n t h e
HYDRALAZINE HYDROCHLORIDE
307
p r e s e n c e of decomposition p r o d u c t s , at a c o n c e n t r a t i o n of about 0.0OlM i n 12 h y d r o c h l o r i c a c i d c o n t a i n i n g a s m a l l amount of g e l a t i n . The half-wave p o t e n t i a l s of t h e two waves were -0.7 and -0.95 V a g a i n s t a s a t u r a t e d calomel electrode
.
6.8
Paper Chromatography Ruggieri (56) and McIsaac and Kanda (38) d e s c r i b e chromatography on Whatman No. 1 p a p e r w i t h b u t a n o l / a c e t i c acid/water (4:1:5) as t h e s o l v e n t . Detection w a s by quenching of t h e background f l u o r e s c e n c e of t h e p a p e r under u l t r a v i o l e t l i g h t or by ammoniacal s i l v e r n i t r a t e . The Rf v a l u e f o r h y d r a l a z i n e w a s 0.90. S e v e r a l i n v e s t i g a t o r s (41,45,74)have used a l k a l i n e systems f o r p a p e r chromatography of h y d r a l a z i n e and i t s m e t a b o l i t e s , b u t Lesser e t al (75) suggest t h a t a l k a l i n e chromatography systems may n o t be s u i t a b l e f o r h y d r a l a z i n e i t s e l f .
6.9
Thin Layer Chromatography S t o h s and S c r a t c h l e y (53) i n v e s t i g a t e d s e v e r a l t h i n l a y e r chromatography systems f o r thiazi.de d i u r e t i c s and a n t i h y p e r t e n s i v e d r u g s , u s i n g s i l i c a g e l G and a v a r i e t y of d e t e c t i o n r e a g e n t s . Hydralazine R
Solvent System Methyl e t h y l ketone/n-hexane
( 1 :1)
0.72
Methyl e t h y l ketone/n-hexane
( 2 : 1)
0.62
Methyl e t h y l ketone/n-hexane
(3:1 )
0.oo
Chl oro fo rm/ac e t on e/t r i et hanol amin e
(50:50:1.5)
f
0.68
Reagents f o r d e t e c t i n g h y d r a l a z i n e were D r a g e n d o r f f ' s r e a g e n t , a l k a l i n e dimethylaminobenzaldehyde, a n i s a l d e h y d e , and Bratton-Marshall r e a g e n t . Z a k e t a1 (59) used 3g h y d r o c h l o r i c acid/methanol a s c o r b i c a c i d (44:6:1) on s i l i c a g e l and found an R v a l u e f o f 0.53 f o r h y d r a l a z i n e . Lesser e t a1 (75) used c e l l u l o s e s h e e t s w i t h f l u o r e s c e n t i n d i c a t o r , a c e t i c acid/0.0 1% aqueous disodium e d e t a t e (3:97), and observed an Rf v a l u e of 0.78 for hydralazine. On s i l i c a g e l w i t h f l u o r e s c e n t i n d i c a t o r , t h e Rf v a l u e w a s l e s s t h a n 0.05 w i t h ( a ) chloroform/n-heptane/ a c e t i c a c i d (6:4:I), and ( b ) cyclohexane/chloroform/ a c e t o n i t r i l e ( I :2:I ).
CHESTER E. ORZECH ET A L
308
6.10
High P r e s s u r e Liquid Chromatography Smith e t al (76,771 analyzed h y d r a l a z i n e i n a drug mixture c o n t a i n i n g h y d r a l a z i n e h y d r o c h l o r i d e , hydrochlorot h i a z i d e , and an i m p u r i t y d e r i v e d from t h e l a t t e r . The column w a s 1 m x 2.1 mm (ID) s t a i n l e s s s t e e l , packed w i t h a s t r o n g anion exchanger on 3 pin Zipax@. The mobile phase was pH 9.2 b o r a t e b u f f e r c o n t a i n i n g 0.005z sodium s u l f a t e (5%methanol), a t 1.7 m l p e r minute. Detection w a s by u l t r a v i o l e t a b s o r p t i o n a t 254 nm. Honigberg e t a1 ( 7 8 ) t e s t e d reversed-phase chromatography f o r s e p a r a t i o n of a number of d r u g s , i n c l u d i n g hydralazine. The columns contained e i t h e r octadecyltrichlorosilane o r d i p h e n y l d i c h l o r o s i l a n e , bonded Of t h e numerous t o 37 t o 50 p n p e l l i c u l a r s i l i c a packing. mobile p h a s e s t e s t e d , t h e b e s t f o r s e p a r a t i n g h y d r a l a z i n e , h y d r o c h l o r o t h i a z i d e , and r e s e r p i n e w a s a c e t o n i t r i l e / O . 1% ammonium a c e t a t e (20:80), pH 7.35. The columns were 1.22 m x 2.3 mm (ID) and t h e flow rate w a s 1.4 m l p e r minute. Detection w a s by u l t r a v i o l e t a b s o r p t i o n at 254 nm. 6.11 G a s Chromatography Jack e t al ( 7 9 ) determined h y d r a l a z i n e i n plasma. The sample w a s t r e a t e d w i t h n i t r o u s a c i d , which r e a c t s with h y d r a l a z i n e t o form t e t r a z o l o [ 1,5a]phthalazine (2). The d e r i v a t i v e was e x t r a c t e d with benzene and determined by g a s chromatography. I-Hydrazino-4-methylphthalzine w a s used as an i n t e r n a l s t a n d a r d . The same p r o c e d u r e , or m o d i f i c a t i o n s o f i t , was used by Zak e t a1 (801, T a l s e t h ( 4 2 , 8 2 , 8 2 , 8 3 ) , and Haegele e t a1 ( 4 6 ) f o r m e t a b o l i c s t u d i e s . Zak e t a1 (80) p o i n t o u t t h a t h y d r o l y s i s of c o n j u g a t e s of t h e drug m a y cause a n a l y t i c a l r e s u l t s on b i o l o g i c a l samples t o be v a r i a b l e , depending on t h e a c i d c o n c e n t r a t i o n d u r i n g d e r i v a t i z a t i o n , and t h a t s e l e c t i v e a n a l y s i s f o r unchanged h y d r a l a z i n e and a c i d - l a b i l e m e t a b o l i t e s can be c a r r i e d o u t by s u i t a b l e adjustment of t h e a c i d c o n c e n t r a t i o n . Smith e t a1 (84) determined h y d r a l a z i n e i n t a b l e t s . An aqueous e x t r a c t of t h e t a b l e t s w a s t r e a t e d with 2,4-pentanedione, forming 1- (3,5-dimethylpyrazole) phthalazine. The method w a s a p p l i e d t o s t a b i l i t y s t u d i e s of t a b l e t s s u b j e c t e d t o e l e v a t e d t e m p e r a t u r e s , where t a b l e t s could not b e analyzed by t h e USP method.
7.
ACKNOWLFEMENTS
The w r i t e r s wish t o thank D r . B. T. Kho f o r h i s review of t h e manuscript, Dr. G. S c h i l l i n g of Ayerst Research L a b o r a t o r i e s f o r h i s mass s p e c t r a l d a t a and
Table 2 GAS CHROMATOGRAPHY SYSTEMS USED FOR DERIVATIZED HYDRALAZINE DETERMINATIONS Reference Number
Column
(79)
1.5 m x 2 mm I D , g l a s s , packed w i t h 3% OV-225 on 80-100 mesh Chromosorb W-m
(80)
1.2 m x 2 mm I D , glass, packed w i t h 3% OV-225 on Gas-Chrom Q
(46)
1 m x 4 mm I D , g l a s s , packed with 3% OV-I7 on 80-100 mesh Chromosorb W
(84)
1.8 m x 4 mm I D , g l a s s , packed w i t h 70% S E - 3 on 80-100 mesh G a s Chrom Q
Carrier G a s
N2' ml/min.
He 7
40 ml/min.
N
55
2' ml/min.
Column Temp.,
OC
Detector
220 O C
Pulsed electron capture (Ni-63, 10 mCi )
220 O C
Electron capture
Programmed, a t 4"/min., 170- 240 O C
200 O C
Mass spectrometer
Flame ionization
3 10
CHESTER E. ORZECH ET AL.
i n t e r p r e t a t i o n , t h e l i b r a r y s t a f f (Ms. J. Mcbnough and M s . G. Smith) f o r t h e l i t e r a t u r e s e a r c h , and Mrs. S. W i l l e t t e f o r t y p i n g t h e p r o f i l e .
8.
RFFERENCES F. Gross, J. Druey, and R. Meier, E x p e r e n t i a 6, 19 (1950). 2. J. Druey and B. H. R i n g i e r , Helv. Chim. Acta 195-210 (1951); C.A. 10248f. 3. J. Druey and J. Tripod, Med. Chem. (New York) 2, 223-62 (1967); C.A. 70, 77829e. 4. J. Koch-Weser, N. Engl. J. Med. 295, 320-3 (1976); C.A. 85, 103541rn. 5. L. J . B e l l a m y , "The I n f r a - r e d S p e c t r a of Complex Molecules", 3 r d . ed., John Wiley & Sons, New York, N.Y., 1975. 6. E. G. C. C l a r k e , e d i t o r , " I s o l a t i o n and I d e n t i f i c a t i o n of Drugs", The Pharmaceutical P r e s s , London, England, 1969. 7. M. Kuhnert-BrandstBtter, A. K o f l e r , R. Hoffmann, and H.-C. Rhi, S c i . Pharrn. 33, 205-30 (1965); C.A. 64, 7966g. 8. M. F . S h a r k e y , C. N. Andres, S. W. Snow, A. Major, T. K r a m , V. Warner, and T. G. Alexander, J. A s s . Offic. Anal. Chem. 2, 1124-54 (1968). 9. S. G. Solomonova, N. M. Turkevich, and N. V. Kurinnaya, Farm. Zh. (Kiev) 28, 42-4 (1973); C.A. 78, 140445j. 10. I. S u n h i n e , e d i t o r , ffHandbook of A n a l y t i c a l Toxicology", The Chemical Rubber Co., Cleveland, Ohio, 1969. 11. D. V. Naik, B. R. Davis, K. M. Minnet, and S. G. Schulman, J. Pharm. S c i . 65, 8 4 - 6 (1976); C.A. 126826b. 12. "The Merck Index", 9 t h ed., Merck & Co., Inc., Rahway, N.J., 1976. 13- G. S c h i l l i n g , Ayerst Research L a b o r a t o r i e s , P e r s o n a l Communication. 14. J. Chojnacki, L. Lebioda, and K. S t a d n i c k a , Rocz. Chem. 49, 1163-6 (1975); C.A. &, 106677e. G. C. L d r i , B o l l . chim. farm. 431-6 (1957); 15 C.A. 52, 4109g. 16. K. I. E v s t r a t o v a and A. I. Ivanova, Farmatsiya (Moscow) 1 7 ( 2 ) , 41-5 ( 1 9 6 8 ) ; C.A. 46128a. K. I. E v s G a t o v a , N. A. Goncharova, and V. Ya. I7 Solomko, Farmatsiya (Moscow) 1 7 ( 4 ) , 33-6 ( 1 9 6 8 ) ; C.A. 99338a. 1.
3,
5,
84,
96,
69,
-
69,
31 I
HYDRALAZINE HYDROCHLORIDE
18.
19
20. 21. 22. 23 24.
25.
26.
n. 28.
33.
34
35.
37.
B. P. Artamanov, T. Ya. Konenkova, and S. L. M a i o f i s , Med. Prom. SSSR 1 9 ( 9 ) , 57-9 (1965); C.A. 63, 17800f. " U n i t z S t a t e s Pharmacopeia XIX" , Mack P u b l i s h i n g CO., Easton, Pa., 1975. K. F u j i i and S. S a t o , Ann. Rept. G. Tanabe Co. L t d . 1 , 1-3 (1956); C.A. 51, 6650~. U.S. P a t e n t 2,484,029; C.A. 44, 4046b. B r i t . P a t e n t 629,177; C.A. 4 q 4516i. Japan. P a t e n t 5526 ( ' 5 4 ) ; CX. 49, 1598221. S. B i n i e c k i and B. Gutkowska, Axa Pol. Pharm. 3, 3 - 3 0 ( 1 9 5 5 ) ; C.A. 50, 1206211. B r i t . P a t e n t 735,899; C.A. 50, 1080ii. B r i t . P a t e n t 719,183; C.A. 3, 15982i. E. O i s h i , Yakugaku Zasshi 959-71 ( 1969 1; C.A. 7 2 , 3 4 5 0 ~ . T. P . S y c h e v a , T. P. Kuz'micheva, A. T. Chernyaeva, T. Kh. Trupp, and M. N. Shchukina, Med. Prom. SSSR 1 4 ( 2 ) , 13-17 ( 1 9 6 0 ) ; C.A. 54, 22669g. Fr. P a t e n t 2,193,824; C.A.-82, 73014k. Ger. P a t e n t 2,311,510; C.A.30, 1 0 8 5 6 0 ~ . Can. P a t e n t 992,082; C.A. 86743728m. H. M. P e r r y , J. Lab. Clin.Med. 41, 566-73 ( 1 9 5 3 ) ; C.A. 47, 1060ii. A. R . S c h u l e r t , Arch. i n t e r n . pharmacodynamie B, 1-15 (1961); C.A. 55, 2 2 4 7 1 ~ . S. F a l l a b , Helv. C z m . Acta 45, 1957-65 ( 1 9 6 2 ) ; C.A. 5242~. S. B i n i e c k i , M. M o l l , K. Niewiadomski, a n d M. Rzewuski, Acta P o l . Pharm. 33, 425-7 ( 1 9 7 6 ) ; C.A. 86, 161223r. J. Wagner, J. W. F a i g l e , P. Imhof, and G. L i e h r , Arzneim.-Forsch. 8 , 2388-95 (1977); C.A. 88, 13066111. M. M. Reidenberg, D. Drayer, A. L. DeMarco, and C. T. B e l l o , C l i n . Pharmacol. Ther. 970-7 (1973); C.A. 449. W. M. McIsaac and M. Kanda, J. Pharmacol. Exptl. Therap. 7-13 (1964); C.A. &, 11233bH. Zimmer, J: McManus, T. Novinson, E. V. Hess, and A. H. L i t w i n , Arzneim.-Forsch. 20, 1586-7 ( 1 9 7 0 ) ; C.A. 40761h. H. Zimmer, J. Kokosa, and D. A. G a r t e i z , Arzneim.Forsch. 23, 1028-9 ( 1 9 7 3 ) ; C.A. @, 22460d. A. L i t w i n , L. E. Adams, E. V. Hess, J. McManus, and H. Zimmer, A r t h r i t i s Rheum. 5, 217-23 ( 1 9 7 3 ) ; C.A. 80, 43862b.
&,
-
2,
-
9,
x,
38 39
9
40. 41.
2,
2,
312
CHESTER E. ORZECH ET A L .
42.
43.
44.
T. T a l s e t h , Eur. J. Clin. Pharmacol. 2, 395-401 (1976); C.A. 100742n. H. Zimmer, R. Glaser, J. Kokosa, D. A. G a r t e i z , E. V. Hess, and A. L i t w i n , J. Med. Chem. 18, 188169~. 1031-3 (1975); C.A. A. J. McLean, K. D. Haegele, P. DuSouich, and J. L = McNay , Eur. J. Drug Metab. Pharmacokinet 1 1, 17-20 (1977); C.A. 9911011. C. D. Douglass and R. Hogan, Proc. SOC. Exptl. 100, 446-8 (1959); C.A. 53, 14319f. Biol. Med. K. Haegele, H. B. S k r d l a n t , N. W. R x i e , D. Lalka, and J. L. McNay, J. Chromatogr. 517-34 (1976); C.A. 86, 25798e. K. D.Haegele, A. J. McLean, P. DuSouich, H. B. S k r d l a n t , B. Werckle, and J. L. McNay, Clin. Res. 25, 46OA (1977). S. B. Zak, T. G. G i l l e r a n , J. K a r l i n e r , G. Lukas, J. Med. Chem. 17, 381-2 ( 1 9 7 4 ) ; C.A. 8 1 , 45171~. P. Cooper, P h a x . J. 177, 495-6 ( 1 9 5 6 7 C.A. 2, 6945g V. G. Belikov, G. I. Luk'yanchikova, V. N. Bern12, 60-2 s h t e i n , and I. Ya. Kul, Aptechn. Delo ( 1 9 6 3 ) ; C.A. 9357b. Z. Modras, Farm. Pol. 3, 347-8 (1969); C.A. 71,
86,
5,
. z(
88,
45 46. 47
48. 49
9
50
126,
-
-
61,
51-
84594~. 52.
53
54
A. I. Roshchenko, E. G. Rezchik, and T. V. Gorenko , Farmat s i y a (Moscow) &(5 ) , 76-8 ( 1975 ) ; C.A. 84, 35406~. S. J . S t o h s and G. A. S c r a t c h l e y , J. Chromatogr. 114, 329-33 ( 1 9 7 5 ) ; C.A. 65305g. G. I. Luk'yanchikova, E. N. Vergeichik, A. N. Baranova, A. S. Davydenko, E. N. Pelekhova, 0. I. Turubarova, G. V. Alfimova, and S. G. T i r a s p o l l skaya, Aktual. Vop. Farm. 71-5; C.A. 76, 90123k. B. Wesley-Hadzija and F. Abaffy, Croat. Chem. Acta 30, 15-19 (1958); C.A. 54, 2661i. R. Ruggieri, Farmaco ( P G i a ) Ed. p r a t . 2, 571-6 (1956); C.A. 53, 14421a. U.S.S.R. P a t e n t 148,956; C.A. 58, 1311h. G. I. Luk'yanchikova, Med. P r o z SSSR 1 6 ( 9 ) , 46-8 (1962); C.A. 5454h. S . B. Z a k , M. F. B a r t l e t t , W. E. Wagner, T. G. G i l l e r a n , and G. Lukas, J. Pharm. S c i . 225-9 (1974); C.A. 140963t. W. Grabowicz and J. B r u l i n s k a , Farm. Pol. 29, 805-7 (1973); C.A. 112718~.
84,
9
m,
55 56
57 58. 59
-
58,
a,
80,
60.
80,
313
HY DRALAZINE HYDROCHLORIDE
61. 62.
6364.
-
65
66. 67
68. 69 70.
7172-
a,
H. E l l e r t a n d Z. Modras, Farm. Pol. 511-15 ( 1 9 7 1 ) ; C.A. 6766v. T. Urbanyi and A. O'Connell, Anal. Cheni. 44, 565-70 ( 1 9 7 2 ) ; C.A. 76, 90100d. T. Urbanyi and A. W. O'Connell, Adv. Autorn. Anal., Technicon I n t . Congr. 2, 15-21 (1972); C.A. 82, 116 154a. A. K. Ruzhentseva, I. S. Tubina, and L. N. Bragina, Med. Prom. SSSR 1 4 ( 1 1 ) , 34-6 ( 1 9 6 0 ) ; C.A. 55, 9789g. Ya. M. Perel'man and K. I. E v s t r a t o v a , Aptechn. Delo 1 2 ( 1 ) , 45-9 (1963); C.A. 6 1 , 9360h. N. S.Goryacheva and L. N. P r f l o d k i n a , Farmatsiya 61575n. (Moscow) 17(3), 69-72 (1968); C.A. R. Solirnan and S. A. B e l a l , Pharmazie 3, 204 ( 1 9 7 4 ) ; C.A. 8 1 , 111504j. R. Solirnan a n T S . A. B e l a l , J. Drug Res. 7-11 (1974); C.A. 84918e. S. B e l a l and R. Soliman, Pharmazie 59-60 (1975); C.A. &, 1 5 7 1 2 ~ . H. McKennis and A. S. Yard, U.S. Dept. Corn., O f f i c e Tech. Serv., PB Rept. 143,914 ( 1 9 5 7 ) ; C.A. 55, 17375i. A. Viala, Trav. soc. pharm. M o n t p e l l i e r 18, 96-100 (1958); C.A. 53, 8534g. T. Giovanoli-Jakubezak, J. Chodkowski, and D. Gralewska, Rocz. Chem. 45, 1315-28 (1971); C.A. 76, 30113a. Z. Modras, Chern. Anal. (Warsaw) 1349-53 (1973); C.A. 78, 128457g. H. ZiKer, R. G l a s e r , J. Kokosa, D. A. G a r t e i z , E. V. Hess, and A. L i t w i n , J. Med. Chem. 18, 1031-33 ( 1 9 7 5 ) ; C.A. 188169~. J. M. L e s s e r , Z. H. Israili, D. C. Davis, and P. G. Dayton, Drug Metab. Dispos. 2, 351-60 (1974); C.A. 8 2 , 64s. J. B . S m i t h , J. A. M o l l i c a , H. K. Govan, and I. M. Nunes, Amer. Lab. 4 ( 5 ) , 13-17, 19 (1972); C.A.
76,
69,
6,
83,
2,
-
73.
74.
17,
83,
75
76
-
77,
39 28%.
77.
78 79
-
M o l l i c a , H. K. Govan, and I. M. Nunes, I n t . Lab. 1972 (July-Aug.), 15-16, 19-20, 22-23; C.A. 83, 4 m g . I. L. Honigberg, J. T. S t e w a r t , A. P. Smith, and D. W. H e s t e r , J. Pharm. S c i . 64, 1201-4 ( 1 9 7 5 ) ; C.A. Q, 103357s. D. B. J a c k , S. Brechb'ihler, P. H. Degen, P. Zbinden, and W. R i e s s , J. Chrornatogr. 115,87-92 ( 1 9 7 5 ) ; C.A. 38500k.
J. B. Smith, J. A.
84,
CHESTER E. ORZECH ET AL.
3 14
80. 81. 82.
83. 84.
85.
S. B. Zak, G. L u k a s , and T. G. G i l l e r a n , Drug Metab. Dispos. 2, 116-21 (1977); C.A. 95267a. T. T a l s e t h , Eur. J. Clin. P h a m a c o l . 2, 183-7 (1976); C.A. 1864599. T. T a l s e t h , Clin. Pharmacol. Ther. 3, 715-23 (1977); Index Medicus (Sept. 1, 362-3. T. T a l s e t h , Clin. Pharmacokinet. 2, 317-19 (1977); Index Medicus (Feb.), 363. K. M. Smith, R. N. Johnson, and B. T. Kho, J. Chromatogr. 137,431-7 (1977); C.A. 73417~. P. A. Reece, P. E. S t a n l e y , and R. Z a c e s t , J. Pharm. S c i . 1150-3 (1978).
87,
5,
1977
1978
87,
67,
L i t e r a t u r e surveyed through 1977.
Analytical Profiles of Drug Substances, 8
CALCIUM LEUCOVORIN Leslie 0.Pont, Andrew P . K . Cheung, and Peter Lirn I.
2.
3. 4.
5. 6.
7. 8.
Description 1 . 1 Name, Structure, Empirical Formula, Molecular Weight 1.2 Appearance, Odor, Color 1.3 Isomeric Forms Physical Properties 2. I Infrared Spectrum 2.2 Proton Magnetic Resonance Spectrum 2.3 Carbon- 13 Magnetic Resonance Spectrum 2.4 Ultraviolet Spectrum 2.5 Mass Spectrum 2.6 X-Ray Crystallographic Data 2.7 Optical Rotation 2.8 Circular Dichroism 2.9 Dissociation Constants 2.10 Solubility Synthesis Stability 4.1 Bulk 4 . 2 Solution Metabolism Methods of Analysis 6.1 Elemental Analysis 6 . 2 Equivalent Weight Determination 6.3 Biological Assay 6.3.I Microbiological Assay 6.3.2 Enzyme Assay 6.4 Polarographic Assay 6.5 Spectrophotometric Analysis 6.5. I Fluorimetric Analysis 6 . 5 . 2 Ult ravioletlvisible Analysis 6 . 6 Chromatography 6.6. I Paper Chromatography 6.6.2 Thin-Layer Chromatography 6.6.3 Column Chromatography 6.6.4 High Pressure Liquid Chromatography 6.6.5 Affinity Chromatography 6 . 7 Radioassay Acknowledgments References
3 15
Copyright @ 1979 by Academic Press, Inc. All rights of reproduction in any form reserved. ISBN 0-12-260808-9
LESLIE 0 . PONT ET A L .
316
1.
Description
1.1 Name, Structure, Empirical Formula, and Molecular Weight Citrivorum factor (CF), folinic acid, and leucovorin are all N-[4[[(2-amino-5-formyl-l,4,5,6,7,8-hexahydro4-oxo-6-pteridinyl)methyl]-amino]benzoyl]glutamic acid, I, the Leuconostoc citrovorum 8081* growth factor first reported by Sauberlich and Baumann. Leucovorin refers to the chemically synthesized material that contains both dL and 1L diastereomers; "citrovorum factor" and "folinic acid" generally apply to the biologically synthesized 1L isomer. Much of the data reported here was obtained on calcium leucovorin, the stable, isolatable, biologically compatible salt. __ Name
Empirical Formula
Molecular Weight
Leucovorin
C20Hz3N707
473.449
Calcium leucovorin
CZ0H2,N707Ca
511.513
Calcium leucovorin is also identified by the National Cancer Institute number: NSC 3590.
H
I Citrovorum f a c t o r CF, f o l i n i c a c i d , l e u c o v o r i n , 5fHbF
CALCIUM LEUCOVORIN
317
R, C-NH-CH
I
CH 2 I CH z I COOH I1 IIa
R 1 = OH
IIb
R 1 = NH2 R 2 = CH3
Methotrexate, amethopterin, MTX
IIc
R1
10 formylfolic acid, lOfFA
=
OH
R2
=
H
R 2 = CHO
Folic acid, FA
COOH I11 IIIa
R1
=
H
Rz = H
Tetrahydrofolic acid, H4F
IIIb
R1
= CH3
Rz = H
IIIc
R1 = H
5-methyltetrahydrofolic acid, 5mH F 10-formyltetrahydrofolic acid, 10fH4F
R2 = CHO
+ c1-
IV N 5 , N 1O-methenyltetrahydrofolic acid , anhydroleucovorin, 5,lO-methenylH4F
LESLIE 0. PONT ET AL.
3 18
I
CH z I
CH z I COOH
v N',N'o-methylenetetrahydrofolic
1.2
acid , 5 ,lo-methylene H4F
Appearance, Odor, C o l o r
Calcium l e u c o v o r i n o c c u r s a s a n amorphous, odorless powder t h a t i s o f f - w h i t e t o l i g h t b e i g e i n c o l o r . The s a l t is n o t i s o l a t e d i n a n anhydrous form, b u t g e n e r a l l y c o n t a i n s 10-15% w a t e r (3-5 m o l e c u l e s o f h y d r a t i o n ) .
1.3
I s o m e r i c Forms
Two a s y m m e t r i c c a r b o n a t o m s , t h e a c a r b o n i n t h e g l u t a m i c a c i d p o r t i o n o f t h e m o l e c u l e and t h e C 6 c a r b o n i n the tetrahydropteridine r i n g , allow four p o s s i b l e isomers. S i n c e s y n t h e t i c p r o c e d u r e s would u n d o u b t e d l y s t a r t w i t h L-glutamic a c i d , t h e i s o m e r i c p o s s i b i l i t i e s a r e r e d u c e d t o t h e dL a n d 1 L d i a s t e r e o m e r s . Of t h e s e , t h e b i o l o g i c a l l y more a c t i v e form i s t h e 1 L ; s e p a r a t i o n o f t h e d i a s t e r e o m e r s i s e f f e c t e d by s o l u b i l i t y d i f f e r e n c e s o f t h e c a l c i u m s a l t s . ' x
R e c l a s s i f i e d as P e d i c o c c u s c e r e v i s i a e .
CALCIUM LEUCOVORIN
3 19
Although a p u r e dL sample had n o t been o b t a i n e d , a sample p o s s e s s i n g a h i g h p o s i t i v e r o t a t i o n and lower b i o l o g i c a l a c t i v i t y had been i s o l a t e d . '
2.
Physical Properties 2.1
I n f r a r e d Spectrum
F i g u r e 1 i s t h e i n f r a r e d spectrum t a k e n from a m i n e r a l o i l s u s p e n s i o n of a r e p r e s e n t a t i v e sample o f calcium l e u c o v o r i n . A common f e a t u r e of f o l a t e d e r i v a t i v e i r s p e c t r a o b t a i n e d i n t h i s l a b o r a t o r y i s t h e a b s e n c e of s h a r p a b s o r p t i o n b a n d s , which i s u s u a l l y a t t r i b u t e d t o l a c k of c r y s t a l l i n i t y . Below a r e l i s t e d t h e major a b s o r p t i o n assignments:
Ir a b s o r p t i o n ( p ) 'L
'L
Assignment
3.0
H Z O , N-H(2)
6.0-6.7
H'O, amide I , a r y l s y s t e m s , CO,-,
7.1
c0'-
(tentative)
1.1.9
2.2
amide I1
P r o t o n Magnetic Resonance Spectrum Due t o t h e i o n i c n a t u r e of c a l c i u m l e u c o v o r i n , a n
'H nmr s p e c t r u m c o u l d n o t b e o b t a i n e d i n a n a p r o t i c s o l v e n t ; t h e r e f o r e , t h e s p e c t r u m was o b t a i n e d from a d e u t e r a t e d aqueous s o l u t i o n . The f o l l o w i n g a s s i g n m e n t s h a v e b e e n made r e l a t i v e t o TMS = 0 . 0 0 ppm from a 100-MHz V a r i a n XL100 s p e c trum ( F i g u r e 2 ) : Assignment
Chemical S h i f t (ppm)
Multiplicity
H 8, Y
1.70-2.60
m
H 7, 9
2.95-3.80
m
H a
4.00-4.60
( o b s c u r e d by HOD)
q
J (Hz)
z
0
t"??
0 0 0 0 0 0 0 0 0
0
i-9
0
r"
0
3 3 ~ w a osaw tl 320
7
0
g
m
m
z LT
>
0
w
8 3 5
-I
2
a
2 u U
0
I 13
$
LT I-
n
n
0
2
w LT
U
z
W
LT 13
c7
U
32 I
E
8 7
vl i
Q
P
LESLIE 0.PONT ET A L .
322
Assignment
Chemical S h i f t (ppm)
Multiplicity
J (Hz)
H 3 ' , 5'
6.64
d
8
H 2'c 6'
7.60
d
8
8.59
S
7.89
S
4.8
m (broad)
0 II
H-C-,
5
unknown H, 6
+
The above a s s i g n m e n t s a r e i n g e n e r a l a g r e e m e n t w i t h t h o s e of Pastore3 for folates. The C, p r o t o n i s o b s c u r e d by t h e l a r g e HOD p e a k , and i t s l o c a t i o n was c o n f i r m e d by s h i f t i n g t h e HOD a b s o r b a n c e a t 8 0 " C. The p e a k a t + 7.9 ppm d u e t o a n unknown s p e c i e s h a s b e e n p r e s e n t i n a l l c a l c i u m l e u c o v o r i n samples. The i d e n t i t y o f t h e s p e c i e s r e s p o n s i b l e f o r t h i s s i n g l e t r e m a i n s unknown, b u t a t t h e p r e s e n t t i m e t h e s e a u t h o r s h y p o t h e s i z e t h a t t h e dL d i a s t e r e o m e r ' s f o r m y l g r o u p c o n t r i b u t e s t h i s peak. Since chemically prepared calcium l e u c o v o r i n i s a s s a y e d a t t h i s l a b o r a t o r y , a n 'H nmr s p e c trum h a s n o t been o b t a i n e d on a b i o l o g i c a l l y o r enzymatic a l l y p r e p a r e d m a t e r i a l . E i t h e r s h o u l d b e f o l i n i c a c i d and t h e r e f o r e have t h e 1 L c o n f i g u r a t i o n . Investigations t o r e s o l v e t h i s problem a r e c o n t i n u i n g . 2.3
Carbon-13 Magnetic Resonance Spectrum
The 1 3 C nmr s p e c t r u m r e p r o d u c e d i n F i g u r e 3 w a s o b t a i n e d from a D,O/NaOD s o l u t i o n of c a l c i u m l e u c o v o r i n on a V a r i a n X L l O O S p e c t r o m e t e r . The a s s i g n m e n t s on t h e TMS s c a l e a n d r e f e r e n c e d t o d i o x a n e are l i s t e d below: Assignment
Chemical S h i f t (ppm)
c- 2 c- 4
93.7 102.0 0.0
C- 6
c- 7
-
23.3
0
I1
- C-H
c- 9
98.2
- 25.0
I
I
I
I
1
I
1
I
I
1
1
1
I
I
I
I
I
I
I
D IOXAN E
c PPm FIGURE 3
13C NMR OF CALCIUM LEUCOVORIN
LSJ-57
LESLIE 0 . PONT ET A L .
324
A s s i gnmen t
Chemical S h i f t (ppm)
C-4a o r C-8a
25.2
C-8a o r C-4a
86.5
c-1'
54.7
C-2
I ,
C-3',
C-6'
62.4
c-5'
45.7
c-4 c-7
84.8
'
C-Ci
C- B C-Y
102.8
-
10.8 37.9 32.3
a- coo-
112.6
y-coo-
115.6
The above a s s i g n m e n t s a r e i n r e a s o n a b l e agreement w i t h t h o s e previously reported f o r p t e r i d i n e s . 2.4
U l t r a v i o l e t Spectrum
F i g u r e 4 r e p r e s e n t s t h e uv s p e c t r u m of c a l c i u m l e u c o v o r i n i n pH 7.0 p h o s p h a t e b u f f e r (0.10 M ) , A,, = 286 nm, Amin = 243 nm, and i n 0.10N NaOH (pH 1 3 ) , A,, = 282 nm, A m i n = 242 nm. These s p e c t r a l f e a t u r e s a r e s i m i l a r t o t h o s e r e p o r t e d i n t h e l i t e r a t u r e . 5-12 The most commonly r e p o r t e d a b s o r p t i v i t i e s f o r l e u c o v o r i n o r f o l i n i c a c i d were o b t a i n e d from s o l u t i o n s prepa:ed i n 0.1N NaOH; t h e s e v a l u e s v a r y from 2.7 x lo4 M-' cm-' t o 3 . 2 6 x 10' M-' crn-l'l. Robinson" r e p o r t s E~~~ a p p r o x i m a t e l y 5% lower ( a t pH 8 . 4 ) t h a n t h o s e i n b a s i c s o l u t i o n . The s i n g l e a b s o r p t i o n i s due t o c o n t r i b u t i o n s from p-amino-benzoylglutamate and t h e u n s a t u r a t e d p o r t i o n of t h e p t e r i d i n e r i n g . Loss of a b s o r b a n c e a t s h o r t e r and l o n g e r w a v e l e n g t h s i n b a s i c s o l u t i o n (256 nm and 368 nm) i s c h a r a c t e r i s t i c o f r e d u c e d f o l a t e s . Spectral d a t a o b t a i n e d from s o l u t i o n s p r e p a r e d i n a c i d s do n o t r e f l e c t l e u c o v o r i n a b s o r b a n c e s b e c a u s e t h e compound i s n o t s t a b l e . Leucovorin d e h y d r a t e s under a c i d i c c o n d i t i o n s t o produce anhydroleucovorin, N5 ,N"-methenyltetrahydrofolic acid, IV. T h i s compound h a s been i s o l a t e d i n more t h a n o n e form, d e p e n d i n g on pH. l 3 Q
CALCIUM LEUCOVORIN
325
1.0
0.9 0.8
0.7 w
0
z a
2
0.6 0.5 0.4
0.3
0.2 0.1
0 200
250
nm
350
300
LSJ-58
FIGURE 4
ULTRAVIOLET SPECTRUM OF CALCIUM LEUCOVORIN 0.1N NaOH pH 7 Phosphate buffer -~
LESLIE 0. PONT ET A L .
326
2.5
Mass Spectrum-
An e l e c t r o n impact mass s p e c t r u m of c a l c i u m l e u c o v o r i n h a s n o t b e e n o b t a i n e d b e c a u s e t h e compound i s n o t s u f ficiently volatile. I t would b e d i f f i c u l t t o i s o l a t e t h e f r e e a c i d w i t h o u t f i r s t d e h y d r a t i n g t h e compound. Due t o i t s i o n i c n a t u r e , calcium leucovorin w i l l n o t d i s s o l v e i n common s i l y l a t i n g r e a g e n t s . F i e l d d e s o r p t i o n , a n o t h e r mass s p e c t r a l t e c h n i q u e , g e n e r a l l y l e n d s i t s e l f more t o compounds l i k e leucovorin. I n d e e d , t h i s t e c h n i q u e h a s been a p p l i e d s u c c e s s f u l l y t o m e t h o t r e x a t e and o t h e r f o l i c a c i d a n a l o g s . l 4
2.6
X-ray C r y s t a l l o g r a p h i c Data
C r y s t a l l o g r a p h i c d a t a have n o t been p u b l i s h e d f o r c a l c i u m l e u c o v o r i n , b u t l i t e r a t u r e v a l u e s do e x i s t f o r t h e D i f f r a c t i o n p a t t e r n s could n o t be obtained barium s a l t . ' on a l l s a m p l e s a l t h o u g h t h e y had b e e n r e c r y s t a l l i z e d s e v eral t i m e s . I n t e r p l a n a r s p a c i n g s a r e l i s t e d , b u t t h e s e numb e r s a p p e a r t o change w i t h t h e amount o f m o i s t u r e p r e s e n t i n t h e sample. 2.7
Optical Rotation 21
0
a]
= 5 8 9
21
a]
0.3
14.3 k 0.4"
(c1, N/10
NaOH)
1 7 . 9 k 0.4'
(c 1, N/10
NaOH)
0
546 21
+
=
0
=
+
14.9 ? 0.4"
(C 1, H20)
=
+
18.8 t 0.4"
(c1, H z O )
5 8 9
21
a] 5 4 6
The above v a l u e s were o b t a i n e d on a n a v e r a g e l o t o f c a l c i u m l e u c o v o r i n examined in t h i s l a b o r a t o r y . C o r r e c t i o n s were made f o r water c o n t e n t . D i f f e r e n c e s i n r o t a t i o n v a l u e s may p a r t l y r e f l e c t s o l u b i l i t y i n t h e two s o l v e n t s ; t h e compound w a s more d i f f i c u l t t o d i s s o l v e i n N / 1 0 NaOH. The H 2 0 r o t a tion is c l o s e t o t h e l i t e r a t u r e value: (rID = 1 4 . 2 6 " 3.42 H,O).'
+
(c,
CALCIUM LEUCOVORIN
2.8
327
C i r c u l a r Dichroism
The f o l l o w i n g d a t a were o b t a i n e d on an a v e r a g e sample of c a l c i u m l e u c o v o r i n : Solvent
&
(nm)
[ e l (deg
M-lcm-')
0.1N NaOH
282
3.89
H20
287
3.47 x lo3
103
The molar e l l i p t i c i t i e s a r e c a l c u l a t e d f o r l e u c o v o r i n f r e e a c i d and have been c o r r e c t e d f o r water c o n t e n t . These v a l u e s may b e q u i t e d i f f e r e n t from t h o s e of f o l i n i c a c i d , Although a s i n g l e v a l u e i s r e p o r t e d f o r each s o l v e n t , b o t h s p e c t r a c o n t a i n more t h a n one a b s o r p t i o n band. Whether t h e e x t r a n e o u s a b s o r p t i o n s a r e due t o i m p u r i t i e s o r a r e a c t u a l l y due t o l e u c o v o r i n ' s a b s o r p t i o n b e h a v i o r i s n o t known at this time.
2.9
Dissociation Constants
Three pKa v a l u e s have been r e p o r t e d f o r l e u c o v o r i n ( f r e e a c i d ) ; t h e y a r e 3 . 1 , 4 . 8 , and 1 0 . 4 , as d e t e r mined by e l e c t r o m e t r i c t i t r a t i o n . 6 The f i r s t two v a l u e s a r e a t t r i b u t e d t o t h e g l u t a m y l c a r b o x y l s , and 10.4 is a s s i g n e d t o t h e h y d r o x y l group a t t h e 4 p o s i t i o n , ' by comparison t o model compounds.
2.10 S o l u b i l i t y The i o n i c n a t u r e o f c a l c i u m l e u c o v o r i n s e v e r e l y r e s t r i c t s i t s s o l u b i l i t y i n common o r g a n i c s o l v e n t s ( s o l I n water, t h e s o l u b i l i t y is u b i l i t y i n DMSO << 1 mg/ml). l a r g e (% 100 mg/ml), b u t i n 0.1N NaOH i t d r o p s s i g n i f i c a n t l y ( < 20 mg/ml). Acid s o l u b i l i t y i s d i f f i c u l t t o i n t e r p r e t s i n c e t h e s o l u t e may no l o n g e r b e l e u c o v o r i n .
3.
Synthesis
With s l i g h t m o d i f i c a t i o n s i n p r o c e d u r e , one b a s i c synt h e s i s of l e u c o v o r i n and t h e s u b s e q u e n t i s o l a t i o n of i t s s a l t s have remained unchanged f o r n e a r l y t h i r t y y e a r s . The method i n v o l v e s h y d r o g e n a t i o n of f o l i c a c i d ( p t e r o y l g l u tamic a c i d ) i n t h e p r e s e n c e of a p l a t i n u m o r p a l l a d i u m c a t a l y s t , as f i r s t d e s c r i b e d by O ' D e l l e t a l . 1 5 T h i s
LESLIE 0. PONT ET A L .
328
r e d u c t i o n s t e p i s c a r r i e d on c o n c u r r e n t l y . o r a f t e r 1 6 - 1 9 i n i t i a l f o r m y l a t i o n of f o l i c a c i d i n f o r m i c a c i d . The pH of t h e r e a c t i o n mixture i s a d j u s t e d w i t h base i n t h e presence of a n a n t i o x i d a n t and h e a t e d ( i n c u b a t e d 50-150" C P u r i f i c a t i o n by column w i t h o r w i t h o u t reduced p r e s s u r e ) . chromatography i s f o l l o w e d by p r e c i p i t a t i o n o f t h e d e s i r e d s a l t by a d d i t i o n of t h e a p p r o p r i a t e c a t i o n and o r g a n i c s o l vent. The c a l c i u m s a l t i s p r e c i p i t a t e d from a n aqueous s o l u t i o n by a d d i t i o n o f C a C l z f o l l o w e d by e t h a n o l . * '
IV
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329
NaHCO, or NaOH or both (antioxidant)
cm
IIIC
I
CaC1. or Ca(OH), Ethanol
Calcium lcucovorio
Early syntheses' ' ' employed ascorbic acid as the antioxidant to protect the newly formed tetrahydro ring. But Roth et ala9 found that ascorbic acid had no effect on leucovorin yield (40-50%) as long as incubation was performed under anaerobic conditions. More recent syntheses have used Z-mer~aptoethanol~~ or a stream of nitrogenz2 to to protect the tetrahydro system. Isolation of the active component is carried out chromatographically. Roth et al. used a magnesol (magnesium silicate) column to absorb colored impurities, followed by a Darco G 6 0 activated carbon column to eliminate sodium formate and inorganics. Elution with an alcohol/ammonia solvent was followed by rechromatographing in magnesol.
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Flynn et a1.6 used a potato starch column, elution with n-butanol/water/ethanolfglacial acetic acid, 100/50/40/ 0 . 4 , followed by a Florisil column, treated with pH 5.5
acetate buffer, CaC12 and ascorbic acid and elution with distilled water. Subsequent recrystallizations were made from water. Other authors prefer ion-exchange cellulose chromatography. Zakrzewski and Sanson' use DEAE cellulose in the O H form, eluting with a 2-mercaptoethanol/ ammonia gradient. Beavon and Blair ' recommend 1-mm cellulose plates developed in n-propanol/NH40H/Hz0, 200/1/99. The chemical synthetic methods of obtaining leucovorin or its salts are discussed above, but of course the originally identified material came from biological synthesis of citrovorum factor in animal liver.' Early isolation techniques included electrolysis of liver concentrates in the presence of acetic acid.23 Folinic acid synthesis has been reported in a variety of biological systems, including rat liver," avian liver homogenates,25"6 microorganisms, (i. e. , bacteria' " '' and virus3') and plants. 3 1 Factors affecting synthesis (e.g. , temperature, pH, antioxidants) are discussed in several of these papers. In living systems, folinic acid can be synthesized ultimately from folic acid by reduction to tetrahydrofolic acid followed by addition of a 1-carbon fragment to the molecule (N5,N1O-methylenetetrahydrofolate, V) After a 2-step oxidation, the formyl group resides either at the N5 or NIO position or as an equilibrium mixture. The essential reactions are summarized below: 3 2
.
H Folic acid + dihydrofolate
-
H dihydrofolate' reductase
N5 ,N1O-methenyltetrahydrofolate-
M
N 5-formyltetrahydrofolate
lt
NADP'
I
t et rahydrofolate
+
serine
N 5 , N -methylenetetrahydrofolate + glycine NADPH "active formaldehyde''
N 1 O - formyltet rahydrofo late
lr
NADH NAD+ N5-methyltetrahydrofolate
CALCIUM LEUCOVORIN
R e c e n t l y , t h e enzymatic f o r m a t i o n of r o l i n i c a c i d h a s been u t i l i z e d t o s y n t h e s i z e r a d i o a c t i v e l y l a b e l e d prod u c t s . 3 4 The p r e p a r a t i o n of 5-formyl t e t r a h y d r o f o l a t o , 9 , 3 ' ,5'-3H and 5 - f 0 m y l - ~ ~ C - t e t r a h y d r o f o l a t e s t a r t s w i t h t r i t i a t e d f o l i c a c i d , which is reduced t o d i h y d r o f o l a t e , i n c u b a t e d i n t h e p r e s e n c e of formaldehyde, d i h y d r o f o l a t e r e d u c t a s e , and NADPH, and f i n a l l y i n c u b a t e d w i t h 5,lOmethylenetetrahydrofolate d i h y d r o g e n a s e . The p r o d u c t , N 5 ,N1'-methenyltetrahydrofolate (with ascorbic a c i d ) w a s a d j u s t e d t o n e u t r a l pH, a u t o c l a v e d , and s t o r e d a t -20" C p r i o r t o column p u r i f i c a t i o n on DEAE and G-15 Sephadex. These l a b e l e d p r o d u c t s are t h e b i o l o g i c a l l y a c t i v e d i a s t e r e o m e r s , and t h e y a r e used t o s t u d y t h e metabolism of f o l i n i c a c i d i n c e l l s , t i s s u e s , and a n i m a l s .
4.
Stability
4.1
Bulk
Calcium l e u c o v o r i n i s s t a b l e i n b u l k form a f t e r f o u r weeks' s t o r a g e a t 6 0 " C. The s t a b i l i t y w a s m o n i t o r e d by HPLC i n t h i s l a b o r a t o r y , u s i n g t h e c o n d i t i o n s d i s cussed i n S e c t i o n 6.6.4.
4.2
Solution
Citrovorum f a c t o r h a s been r e p o r t e d t o b e s t a b l e under s e v e r e a l k a l i n e c o n d i t i o n s by B r o q u i s t e t a1.35 and e a r l i e r by Lyman and P r e s c o t t . 3 6 Steam-heating f o r 30 m i n u t e s i n 0.2" NaOH d i d n o t decompose t h e compound. A l k a l i n e s t a b i l i t y i s n o t s u r p r i s i n g when one c o n s i d e r s t h a t many o f t h e s y n t h e t i c p r o c e d u r e s r e q u i r e a u t o c l a v i n g a t h i g h pH as a f i n a l s t e p i n c o n v e r t i n g anhydroleucovorin. I n v e s t i g a t i o n s conducted i n t h i s l a b o r a t o r y i n 0.1N N a O H (pH % 1 3 ) and i n d e i o n i z e d w a t e r (pH % 6 show l e u c o v o r i n t o b e s t a b l e a t room t e m p e r a t u r e and under l a b o r a t o r y i l l u m i n a t i o n € o r a t l e a s t 24 h o u r s ( c o n c e n t r a t i o n 1 mg/ml). S t a b i l i t y w a s m o n i t o r e d by h i g h - p r e s s u r e l i q u i d chromatography u s i n g c o n d i t i o n s found i n S e c t i o n 6.6.4. As s t a t e d previously, leucovorin is not s t a b l e under a c i d i c c o n d i t i o n s . l 3 Depending on t h e pH, d i f f e r e n t forms o f a n h y d r o l e u c o v o r i n have been i s o l a t e d : pH 5 1 . 3 i s o l e u c o v o r i n c h l o r i d e ; pH = 2 a n h y d r o l e u c o v o r i n A; p H = 4 ( h o t ) a n h y d r o l e u c o v o r i n B. A l l t h r e e forms c o n v e r t back t o l e u c o v o r i n when d i s s o l v e d i n NaOH under a n a e r o b i c c o n d i t i o n s
33 I
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5.
Metabolism
Citrovorum f a c t o r f u n c t i o n s ( p r i m a r i l y ) as a 1-carbon donor i n t h e s y n t h e s i s of s e r i n e from g l y c i n e . 3 7 - 4 0 The N S formyl group i s i n c o r p o r a t e d from t h e 5 , l O methylene comSilverman e t a 1 . 4 1 have shown t h a t t h e c i t r o pound. 3 3 y vorum f a c t o r , when i n t h e p r e s e n c e of a l a r g e e x c e s s of g l u t a m i c a c i d and a hog l i v e r enzyme, l o s e s i t s formyl group t o form t h e N-formylglutamic a c i d and t e t r a h y d r o f o l i c a c i d . These a u t h o r s d i s m i s s t h e p o s s i b l e f o r m a t i o n of 10fH4F o r 5,lO-methenyl H4F i n t h e i r r e a c t i o n s . Howe v e r , Peters and Greenberg4’ r e p o r t e d s e p a r a t i n g a n enzyme from s h e e p l i v e r , c i t r o v o r u m f a c t o r c y c l o h y d r a s e , which c o n v e r t e d 5fH4F t o a compound much l i k e , b u t n o t i d e n t i c a l t o , 5,lO-methenyl H4F. Anhydroleucovorin, t h e 5,lOmethenyl H4F compound, e x i s t s i n e q u i l i b r i u m w i t h t h e 5 and 1 0 formyl compounds ( s e e b i o s y n t h e t i c scheme). The l a t t e r , 10fH4F, h a s been r e p o r t e d t o d o n a t e i t s formyl group t o m e t h i o n i n e , which i s a s s o c i a t e d w i t h a n e s t e r i f i e d s p e c i e s A t r a n s f e r RNA, which i n t u r n c o n t i n u e s i n t h e s y n t h e s i s of p r o t e i n s . 4 3 I n t h e p r e s e n c e of appropr i a t e enzymes, f o r m y l t e t r a h y d r o f o l a t e s d o n a t e formyl groups f o r p u r i n e s y n t h e s i s 4 4 :
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E q u a t i o n 1 i s c a t a l y z e d b y g l y c i n a m i d e r i b o t i d e (GAR) t r a n s f o r m y l a s e and E q u a t i o n 2 i s c a t a l y z e d b y a m i n o i m i d a z o l e carboxamide r i b o t i d e (AICAR) t r a n s f o r m y l a s e .
I n humans and r a t s , e a r l y i n v e s t i g a t i o n s showed t h a t l a r g- e d o s e s o f f o l i c a c i d r e s u l t e d i n i n c r e a s e d e x c r e t i o n of a s u b s t a n c e t h a t s t i m u l a t e d t h e growth o f P. c e r e v i s i a e and t h a t w a s presumed t o b e c i t r o v o r u m This r e s p o n s e i s now a l s o a s s o c i a t e d w i t h o t h e r r e d u c e d f o l a t e s . R e c e n t l y a g r e a t d e a l of e f f o r t h a s b e e n s p e n t i n s t u d y i n g t h e metabolism of leucovorin i n vivo. This emphasis was prompted by t h e c h e m i c a l s t a b i l i t y of t h i s f o l a t e and by t h e o b s e r v a t i o n o f a r e d u c t i o n i n t o x i c i t y o f m e t h o t r e x a t e when i t w a s g i v e n i n c o n j u n c t i o n w i t h l e u c o v o r i n . Foli n i c a c i d i s found i n human l i v e r , b u t i t i s n o t t h e m a j o r c i r c u l a t i n g f o l a t e , which i s 5-methyltetrahydrofolate. Most of t h e f o l a t e s t h a t o c c u r n a t u r a l l y i n man a r e polyglutamates, a l t h o u g h t h e y a r e t r a n s p o r t e d as monoglutamates. S e v e r a l g r o u p s i n v e s t i g a t i n g human m e t a b o l i s m o f f o l i n i c a c i d have used a d i f f e r e n t i a l m i c r o b i o l o g i c a l method f o r d e t e r m i n i n g f o l a t e s i n b i l e , serum, and u r i n e . 4 7 ’ 4 9 Using t h r e e m i c r o o r g a n i s m s t h a t r e s p o n d t o d i f f e r e n t f o l a t e s , t h e y deduced t h e i d e n t i t y o f some metab o l i c products. Generally, c a s e i r e s p o n d s t o a l l monoglutamates, f a e c a l i s a l s o m e a s u r e s monoglutamates e x c e p t 5mH4F, and p. c e r e v i s i a e growth q u a n t i t a t e s t e t r a h y d r o f o l a t e s , a g a i n e x c l u d i n g 5mH4F. P r a t t and Cooper4’ casei r e s p o n s e and a l e s s showed a l a r g e i n c r e a s e i n pronounced i n c r e a s e i n 2. f a e c a l i s growth i n b i l e and plasma a f t e r o r a l a d m i n i s t r a t i o n of l e u c o v o r i n t o p a t i e n t s . L i t t l e , i f a n y , i n c r e a s e w a s n o t i c e d i n p. c e r e v i s i a e . From t h e s e o b s e r v a t i o n s t h e y c o n c l u d e d t h a t 5fH,F i s r a p i d l y m e t a b o l i z e d t o 5mH4F, a l t h o u g h a v e r y s m a l l amount may b e a b s o r b e d as t h e i n t a c t 5-formyl compound. P e r r y and C h a n a r i n 4 ’ found s i m i l a r r e s u l t s i n u r i n e s a m p l e s . With t h e s y n t h e s i s o f t h e doubly l a b e l e d r a d i o a c t i v e compound, 5-formyl-’ 4 C - t e t r a h y d r o f o l a t e - 3 H , i n v e s t i g a t o r s have been a b l e t o t r a c e t h e m e t a b o l i c p r o d u c t s when t h e drug is administered o r a l l y o r i n t r a v e n o u s l y .
s.
L.
L.
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LESLIE 0.PONT ET AL.
Nixon and B e r t i n o have done a n e x t e n s i v e s t u d y o f f o l i n i c a c i d metabolism i n human s u b j e c t s g i v e n t h e d r u g b o t h ways. When g i v e n o r a l l y , a f t e r 75 m i n u t e s t h e majori t y (90%) of 3H i n serum w a s found i n 5mH4F, w i t h 20% o f 1 4 C a s s o c i a t e d w i t h t h e same compound; 8 t o 9% of e a c h l a b e l w a s found a s 10fH4F o r 5,lO-methenyl H4F. Due t o t h e l a b i l e n a t u r e of t h e formyl group, 70% of t h e 1 4 C was n o t absorbed on Sephadex as f o l a t e under t h e chromatog r a p h i c c o n d i t i o n s u s e d , and t h e a u t h o r s presumed t h a t r a d i o a c t i v i t y had been i n c o r p o r a t e d i n t o amino a c i d s . V i r t u a l l y no r a d i o a c t i v e 5fH4F was found. However, t h e r a d i o a c t i v i t y a s s o c i a t e d w i t h u r i n e (0-1 hour a f t e r admini s t r a t i o n ) was % 40% 3H-labeled 5fH4F. Less t h a n 20% of t h e remaining 3H w a s i d e n t i f i e d as 5mH4F o r p-aminobenz o y l g l u t a m a t e , less t h a n 40% as 10fH4F o r 5,lO-methenyl H4F. The 1 4 C w a s e x c r e t e d as a m i x t u r e of t h e t h r e e f o l a t e s . A t longer t i m e i n t e r v a l s , t h e s e proportions v a r i e d . Ninety minutes a f t e r i n j e c t i o n , 60% 3H w a s found as 5mH4F, 40% of r a d i o a c t i v i t y as 5fH4F, and 40% 1 4 C w a s no l o n g e r a s s o c i a t e d w i t h serum f o l a t e . U r i n e showed most r a d i o a c t i v i t y a s 5fH4F i n i t i a l l y , and s e v e r a l h o u r s l a t e r a r i s e w a s s e e n i n l a b e l e d 10fH4F a n d / o r 5,10-methenyl H4F. From t h i s s e r i e s of s t u d i e s , t h e a u t h o r s concluded t h a t most 1 4 C w a s removed from c i r c u l a t i n g f o l a t e s , most of t h e 3H w a s a s s o c i a t e d w i t h 5mH4F, most of t h e drug w a s a b s o r b e d by t i s s u e s , and t h e m a j o r i t y of 5fH4F w a s c o n v e r t e d t o 5mH4F. E q u a l l y i m p o r t a n t w a s t h e s i t e o f metabolism. S i n c e t h e 5f -+ 5m c o n v e r s i o n w a s more r a p i d i n p a t i e n t s r e c e i v i n g o r a l admini s t r a t i o n , t h e authors f e l t t h a t t h e r e a c t i o n took place The i n t h e i n t e s t i n e , a view s u p p o r t e d by o t h e r s . ’ l voided f o l a t e s seemed t o b e 10fH4F o r 5,lO-methenyl H4F. Another i n t e r e s t i n g s u g g e s t i o n was t h a t 5mH4F w a s cons e r v e d o v e r 5fH4F by t h e k i d n e y s . Although l e u c o v o r i n i s r a p i d l y a b s o r b e d and metabol i z e d i n t h e i n t e s t i n e , i t s m e t a b o l i c p r o d u c t , 5mH4F, i s c o n c e n t r a t e d i n c e r e b r o s p i n a l f l u i d (CSF). I n a s t u d y w i t h dogs, L e v i t t e t a1.” found t h a t i n j e c t e d l a b e l e d f o l a t e s d i s a p p e a r e d from serum and a p p e a r e d as 5mHbF i n CSF f o l l o w i n g f i r s t - o r d e r k i n e t i c s . With doubly l a b e l e d 5fH4F, t h e a u t h o r s were a b l e t o trace t h e 1 4 C formyl moiety t o s e r i n e o r m e t h i o n i n e and t h e 3H p o r t i o n t o 5mH4F. The u p t a k e o f d r u g o c c u r r e d i n two s t e p s : a ) e q u i l i b r a t i o n i n e x t r a c e l l u l a r f l u i d with nonlabeled
CALCIUM LEUCOVORIN
compound,53 followed by b ) c e l l u l a r uptake and metabolism. E a r l y p a p e r s r e p o r t e d a n a t u r a l c o n c e n t r a t i o n of f o l a t e i n CSF t h a t w a s t h r e e t i m e s t h e e q u i l i b r i u m c o n c e n t r a t i o n i n serum. T h i s c o u l d i n d i c a t e t h e importance of f o l a t e s i n n e u r a l metabolism, and t h e r e have been some r e p o r t s regardi n g t h e t h e r a p e u t i c t r e a t m e n t of n e u r o p s y c h i a t r i c d i s o r d e r s with f o l a t e s . The r e c e n t i n t e r e s t i n l e u c o v o r i n i s due t o i t s a b i l i t y t o r e d u c e m e t h o t r e x a t e (MTX) t o x i c i t y when b o t h a r e admini s t e r e d t o c a n c e r p a t i e n t s . E a r l y s t u d i e s s 4 i n mice showed t h a t most b e n e f i t o c c u r r e d when l e u c o v o r i n w a s g i v e n 12-24 h o u r s a f t e r MTX i n f u s i o n . The d e l a y i n a d m i n i s t e r i n g l e u c o v o r i n reduced t h e t o x i c e f f e c t s of MTX w i t h o u t r e d u c i n g the l a t t e r ’ s antitumor a c t i v i t y . T h e r e f o r e , an enhancement of MTX e f f e c t can b e produced by l a r g e r dosages witho u t t h e t o x i c i t y a s s o c i a t e d w i t h t h e s e amounts. When g i v e n c o n c u r r e n t l y , l e u c o v o r i n reduced MTX t o x i c i t y a t t h e expense of tumor a c t i v i t y . However, r e c e n t work5’ h a s shown some advantage i n c o n c u r r e n t a d m i n i s t r a t i o n . I n t h e case of MTX-sensitive c e l l s , “ f o l i n i c a c i d p r o t e c t i o n ” i n c r e a s e s t h e c e l l s u r v i v a l percentage. Rescue p r o c e d u r e , o r leucov o r i n given a f t e r a d e l a y p e r i o d , was most e f f e c t i v e (meas u r e d i n p e r c e n t a g e of c e l l s u r v i v a l ) i n t r e a t i n g MTXr e s i s t a n t c e l l s . The t h e r a p e u t i c e f f e c t of l e u c o v o r i n l i e s i n an e a r l i e r resumption of DNA s y n t h e s i s t h a n i f MTX were a d m i n i s t e r e d a l o n e . 5 6 Nahas e t a l . attribute this resumption t o s e v e r a l p o s s i b l e a c t i o n s of l e u c o v o r i n ( a s s t u d i e d i n L1210 leukemia c e l l s ) : a ) e f f l u x of MTX i s i n c r e a s e d i n t h e p r e s e n c e of 5fH4F; b) 5fH4F could deblock d i h y d r o f o l a t e r e d u c t a s e bound by MTX by b e i n g a p o t e n t i a l supply of d i h y d r o f o l a t e ; c ) t h e i n t a c t drug could p o s s i b l y d i s p l a c e some of t h e MTX; and d) 5fH4F competes w i t h MTX f o r c e l l u l a r uptake. C e l l u l a r uptake seems t o b e enhanced by methyl o r formyl groups a t N 5 on reduced f o l a t e s , by amino s u b s t i t u t i o n s on C 4 o f o x i d i z e d f o l a t e s , and by t e r minal glut am ate^.^' Thus 5fH4F, 5mH4F, and MTX appear t o u s e t h e s a m e c a r r i e r - m e d i a t e d t r a n s p o r t i n t o c e l l s , a system used by f o l i n i c a c i d t o a lesser e x t e n t . Another a u t h o r ” d e s c r i b e s t h e t r a n s p o r t of f o l a t e s a c r o s s memb r a n e s a s an exchange phenomenon because a l t h o u g h leucov o r i n competes w i t h MTX f o r c e l l u p t a k e , i t can a l s o s t i m u l a t e i n f l u x of t h e l a t t e r i f t h e c e l l s a r e a l r e a d y
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preloaded w i t h f o l i n i c a c i d . The i n f l u x i s n o t e d even i n c a s e s where d i h y d r o f o l a t e r e d u c t a s e h a s been i n a c t i v a t e d by p r e v i o u s MTX dosage.
6.
Methods of A n a l y s i s
6.1
Elemental A n a l y s i s
Below a r e l i s t e d e l e m e n t a l a n a l y s i s r e s u l t s o b t a i n e d from a t y p i c a l sample of calcium l e u c o v o r i n : Element
% Theoretical
% Found*
C
46.96
46.87
H
4.14
4.11
N
19.17
19.07
7.84
Ca
6 . 9 4 t , 7.71$
*C o r r e c t e d
f o r 10.4% HzO. +Found by a t o m i c a b s o r p t i o n . ?Found by s u l f a t e a s h . The h i g h e r calcium v a l u e o b t a i n e d by t h e a s h method i s no doubt due t o t h e p r e s e n c e of sodium ( t h e c o u n t e r i o n f o r a c e t a t e commonly found i n some l o t s ) .
6.2
E q u i v a l e n t Weight Determination
Because s y n t h e t i c p r o d u c t s a r e i s o l a t e d a s t h e barium o r , more f r e q u e n t l y , t h e c a l c i u m s a l t of l e u c o v o r i n , common a c i d - b a s e t i t r a t i o n s are n o t r e p o r t e d . I f t h i s t y p e of t i t r a t i o n o r one i n which t h e c a t i o n i s exchanged were f e a s i b l e , t h e r e s u l t s would r e q u i r e c a r e f u l i n t e r p r e t a t i o n because i m p u r i t i e s c o n t a i n i n g t h e g l u t a m i c a c i d moiety would respond s i m i l a r l y t o l e u c o v o r i n when t h e c a r b o x y l groups are b e i n g a n a l y z e d .
6.3
B i o l o g i c a l Assay
6.3.1
M i c r o b i o l o g i c a l Assay
Several microbiological procedures f o r a s s a y i n g CF have been d e s c r i b e d i n t h e l i t e r a t u r e . In g e n e r a l , t h e s e methods a r e designed t o measure CF c o n t e n t i n a b i o l o g i c a l f l u i d o r specimen. They a l l make u s e of t h e growth promotion of L. c i t r o v o r u m 8 0 8 1 , o r p. Ev i s i a e , as i t h a s been renamed. Before CF w a s i s o l a t e d
CALCIUM LEUCOVORIN
o r l e u c o v o r i n w a s s y n t h e s i z e d , S a u b e r l i c h and Baumann’ m e a s u r e d e n h a n c e d growth o f t h e m i c r o o r g a n i s m i n t h e p r e s e n c e o f v a r i o u s b i o l o g i c a l e x t r a c t s , e s p e c i a l l y l i v e r conc e n t r a t e s . Q u a n t i t a t i o n came from t u r b i d o m e t r i c r e a d i n g s a n d f o r N a O H t i t r a t i o n of a c i d p r o d u c e d . T h e i r r e s u l t s are r e p o r t e d i n t e r m s of c i t r o v o r u m u n i t s t h a t c o r r e s ponded t o t h e h a l f - o p t i m a l g r o w t h i n a s t a n d a r d r e t i c u l o g e n s a m p l e . The a u t h o r s r e a l i z e d t h e l i m i t s o f t h e i r a s s a y method s i n c e f o l i c a c i d a d d i t i o n s c a u s e d e n h a n c e d growth a f t e r a n i n i t i a l l a g . W i n s t e n a n d E i g e n ” t r i e d t o improve t h e method by c h r o m a t o g r a p h i n g t h e s a m p l e s on p a p e r b e f o r e t e s t i n g f o r p. c e r e v i s i a e g r o w t h , b u t t h e y , The b a s i s t o o , found more t h a n a s i n g l e a c t i v e component. Coopero f t h i s p a r t i c u l a r technique is s t i l l being used. man6’ r e f i n e d t h e p r o c e d u r e somewhat, b u t c o n t i n u e d t o measure t u r b i d i t y . F o l i c a c i d i n t e r f e r e n c e is minimized by i n c u b a t i o n f o r s h o r t p e r i o d s . Quantitation is in t e r m s o f mg/ml, u s i n g commercial s a m p l e s o f l e u c o v o r i n as s t a n In o n e r e c e n t l y p u b l i s h e d method, ’ p a p e r d i s c s dards. a r e i m p r e g n a t e d w i t h t h e t e s t s o l u t i o n s and CF c o n t e n t i s found by m a n u a l l y m e a s u r i n g L. c i t r o v o r u m ATCC 8 0 8 1 growth on agar p l a t e s . The a d v a n t a g e o f t h i s method i s t h a t CF c a n b e q u a n t i t a t e d i n s o l u t i o n w i t h a l a r g e excess o f amethopterin because t h e microorganisms are resistant t o S t a t i s t i c a l v a r i a t i o n on t h i s method i s 10%. the latter.
6.3.2
Enzyme Assay
S i l v e r m a n e t a 1 . 4 1 p u r i f i e d a hog l i v e r enzyme t h a t c a t a l y z e d t h e t r a n s f e r o f t h e f o r m y l g r o u p o f CF t o g l u t a m i c a c i d . I f n o t p r o t e c t e d from o x i d a t i o n , t h e t e t r a h y d r o f o l i c a c i d formed would s p o n t a n e o u s l y decompose t o p - a m i n o b e n z o y l g l u t a m a t e and p t e r i d i n e . A r y l a m i n e f o r m a t i o n c o u l d be m o n i t o r e d b y t h e B r a t t o n - M a r s h a l l method. T h i s method g i v e s a b e t t e r i n d i c a t i o n o f enzyme a c t i v i t y t h a n CF p u r i t y . The t e c h n i q u e d e v e l o p e d by P e t e r s a n d G r e e n b e r g , 4 z l a t e r r e f i n e d by G r e e n b e r g , 6 2 i s p e r h a p s more straightforward. The t e s t s o l u t i o n s a r e mixed w i t h ATP, MgSO,, a n d enzyme i s o l a t e d from s h e e p l i v e r i n a b u f f e r e d aqueous s o l v e n t . Absorbance a t 343 nm i s r e a d i n a specThe 5,lO-methenyltetrahydrofolate t r o p h o t o m e t e r a t 30” C . b e i n g formed s h o u l d g i v e a d i r e c t m e a s u r e o f t h e CF o r leucovorin present.
337
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The above b i o l o g i c a l a s s a y s a r e i n t e n d e d t o measure CF i n b i o l o g i c a l s o u r c e s r a t h e r t h a n t o d i r e c t l y measure l e u c o v o r i n o r CF p u r i t y . I n f a c t , commercial samples o f l e u c o v o r i n a r e u s u a l l y used t o d e t e r m i n e s t a n d a r d c u r v e s . 6.4
P o l a r o g r a p h i c Assay
Leucovorin, s i n c e i t i s t o t a l l y r e d u c e d , i s p o l a r o g r a p h i c a l l y i n e r t i n a pH 9 b u f f e r e d s o l u t i o n . 6 3 A f t e r a c i d t r e a t m e n t , t h r e e p o l a r o g r a p h i c waves a r e g e n e r a t e d , c o r r e s p o n d i n g t o a n a n o d i c o x i d a t i o n of a t e t r a h y d r o compound and two c a t h o d i c r e d u c t i o n s of unreduced p t e r i a i n e s ; presumably a t l e a s t one of t h e s e t h r e e i s a dihydro s p e c i e s . Polarography i s u s e f u l as a technique i n s t r u c t u r a l e l u c i d a t i o n , b u t a n a l y t i c a l d a t a would b e d i f f i c u l t t o o b t a i n from an a c i d - t r e a t e d s o l u t i o n c o n t a i n i n g several s p e c i e s , each w i t h i t s own p o l a r o g r a p h i c b e h a v i o r .
6.5
Spectrophotometric Analysis 6.5.1
Fluorometric Analysis
I n 1957, Duggan e t a1.64 r e p o r t e d t h a t maximum n a t u r a l f l u o r e s c e n c e o f f o l i n i c a c i d o c c u r r e d a t pH 7 , w i t h e x c i t a t i o n a t 370 nm and e m i s s i o n a t 460 nm. A c o n c e n t r a t i o n o f 0.15 vg/ml gave a f l u o r e s c e n c e of 10% f u l l - s c a l e d e f l e c t i o n a t maximum i n s t r u m e n t a l s e n s i t i v i t y . These a u t h o r s e x p l o r e d a n a l y z i n g f o l i n i c a c i d i n t h e p r e s e n c e of f o l i c a c i d and found t h a t e x c i t a t i o n a t 290 nm e f f e c t i v e l y s h i f t e d t h e e m i s s i o n band of t h e compound o f i n t e r e s t t o 370 nm, t h u s e n a b l i n g a n a l y s i s of a m i x t u r e . A l a t e r p a p e r s 5 r e p o r t e d a f l u o r e s c e n c e maximum f o r l e u c o v o r i n a t 365 nm when e x c i t e d a t 314 nm i n a pH 7 s o l u t i o n ; t h e c o n c e n t r a t i o n w a s 5 x lo-* M. V a r i a t i o n between t h e s e d a t a and o t h e r v a l u e s w a s a t t r i b u t e d t o sample i m p u r i t y , pH of s o l u t i o n , and quenching. The a u t h o r s made an a t t e m p t t o c o r r e l a t e s t r u c t u r e and f l u o r e s c e n c e of reduced f o l a t e s . S i m i l a r i t y between t e s t e d compounds and p-aminobenzoylg l u t a m a t e l e a d them t o c o n c l u d e t h a t t h i s p o r t i o n of t h e molecule i s r e s p o n s i b l e f o r maxima a t 360-425 nm when e x c i t e d a t 300-320 nm. They s u g g e s t e d t h a t i n t e n s i t y d i f f e r e n c e s may a r i s e from v a r i o u s s u b s t i t u t i o n s on t h e t e t r a h y d r o p t e r i d i n e moiety.
CALCIUM LEUCOVORIN
I n 1964, N e t r a w a l i e t a 1 . 6 6 d e s c r i b e d f l u o r e s c e n c e measurements of c a l c i u m l e u c o v o r i n i n NaHC03 s o l u t i o n a f t e r p a p e r chromatography and r e a c t i o n w i t h a c i d i c o r c i n o l . The gray-blue f l u o r e s c e n t s p e c i e s formed on t h e developed papergram w a s v e r y s e n s i t i v e f o r l e u c o v o r i n , showing a d e t e c t i o n l i m i t of 0 . 1 ug. I n t h e e l u t i n g s o l u t i o n , however, t h e r e q u i r e d c o n c e n t r a t i o n i n c r e a s e d t o 0 . 5 ug. Recovery by t h i s method w a s 100 k 15%, and r e s u l t s o b t a i n e d from f l u o r e s c e n c e were lower by 10 t o 20% t h a n t h o s e o b t a i n e d by m i c r o b i o l o g i c a l methods. 6.5.2
U l t r a v i o l e t / V i s i b l e Analysis
U l t r a v i o l e t s p e c t r o s c o p y does n o t l e n d i t s e l f t o l e u c o v o r i n a n a l y s i s f o r two r e a s o n s . F i r s t , b e c a u s e commercial samples a r e f r e q u e n t l y c o n t a m i n a t e d w i t h uv-absorbing i m p u r i t i e s , a r e l i a b l e molar a b s o r p t i v i t y h a s n o t been d e t e r m i n e d f o r l e u c o v o r i n . R e c e n t l y , i n t h i s l a b o r a t o r y a v a l u e of 3.09 x l o 4 I T 1 cm-' w a s d e r i v e d from thorough a n a l y s i s o f a r e l a t i v e l y p u r e sample. T h i s v a l u e i s i n r e a s o n a b l e agreement w i t h t h a t o f Zakrzewski and Sanson. ' Second, l e u c o v o r i n i s known t o d e h y d r a t e under a c i d i c c o n d i t i o n s t o form a n h y d r o l e u c o v o r i n , 5,10-methenyl H4F, which a b s o r b s a t 352-353 nm. I n t h e a b s e n c e of i n t e r f e r i n g s p e c i e s , * l e u c o v o r i n may b e a n a l y z e d by a c i d i f i c a t i o n w i t h 0 . 1 N H C 1 f o l l o w e d by u v measurement a f t e r 1.52 . 0 h o u r s . P u r i t y may b e d e t e r m i n e d r e l a t i v e t o a sample of known p u r i t y o r r e l a t i v e t o l i t e r a t u r e v a l u e s : E~~~ = 2.39-2.41 x l o 4 M-' cm-1.''
*
A b s o r p t i o n i n t e r f e r e n c e s would a r i s e from compounds o t h e r than le uc ovori n t h a t convert t o anhydroleucovorin a t a c i d i c pH. An example of such a compound i s 10fH4F, although i t i s not expected t o c o n t r i b u t e t o ab s o r p tio n due t o i t s i n s t a b i l i t y . However, 10-formyl-7,8d i h y d r o f o l a t e i s a p o s s i b l e contaminant. Ad d itio n al a b s o r p t i o n c o u l d a l s o r e s u l t from u n s a t u r a t e d p t e r i d i n e s .
339
LESLIE 0. PONT ET A L .
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6.6
Chromatography 6.6.1
P a p e r Chromatography
Both p a p e r and t h i n - l a y e r chromatography s e r v e as s e p a r a t i o n t e c h n i q u e s b e f o r e q u a n t i t a t i o n o f a c t i v e components. P a p e r chromatography h a s been u s e d by many e a r l y i n v e s t i g a t o r s t o s e p a r a t e b i o l o g i c a l s a m p l e s b e f o r e d e t e c t i n g by m i c r o b i o l o g i c a l a s s a y , t h e b i o a u t o g r a p h i c method. Winsten and E i g e n S 9 used 2 , 4 , 6 t r i m e t h y l p y r i d i n e t o d e v e l o p papergrams on Whatman No. 1 o r No. 4 . C o l 6 n Z 9 d e v e l o p e d h i s chromatograms i n i s o a m y l a l c o h o l : 5 % d i b a s i c sodium p h o s p h a t e , 1 : 2 . Netrawali e t a1.66 used ethanol:n-butanol:water:25% NH3, 50:15:35:5, on Whatman No. 1 and d e t e c t e d l e u c o v o r i n by forming a f l u o r e s c e n t o r c i n o l d e r i v a t i v e . The m o b i l e p h a s e s i n t h e s e s y s t e m s a r e n e u t r a l t o b a s i c due t o t h e a c i d i n s t a b i l i t y of leucovorin. 6.6.2
T h i n - l a y e r Chromatography
T h i n - l a y e r chromatography on c e l l u l o s e h a s been used a s a n i n t e r m e d i a t e clean-up p r o c e d u r e and f i n a l i s o l a t i o n t e c h n i q u e i n t h e s y n t h e s i s of l e u c o v o r i n . 2 2 A c a t i o n e x c h a n g e / c e l l u l o s e s u p p o r t w a s p r e p a r e d by Copenh a v e r and O ' B ~ i e n , ~and ' t h e m o b i l e p h a s e w a s 15% Na,HPO,* 12H20 (pH 8 . 5 ) c o n t a i n i n g 0 . 1 M m e r c a p t o e t h a n o l . Unfort u n a t e l y , t h i s s y s t e m d i d n o t s e p a r a t e 5f a n d 10fH4F from e a c h o t h e r o r from 5,10-methenyl H4F. S e p a r a t i o n o f t h e former two from t h e * l a t t e r w a s a c h i e v e d w i t h 11 N a 2 H P 0 4 * 1 2 H 2 0 . Leucovorin w a s d e t e c t e d w i t h a 6N HC1/ZnClz/sodium c i t r a t e spray. Brown e t a 1 . 6 8 h a v e developed a c e l l u l o s e p l a t e w i t h a fluorescent indicator. Compounds a r e d e v e l o p e d i n 3.0% (w/v) N H 4 C 1 and d e t e c t e d by f l u o r e s c e n c e q u e n c h i n g . These a u t h o r s a l s o u s e 0.5% m e r c a p t o e t h a n o l i n t h e i r m o b i l e p h a s e , b u t t h i s i s o n l y t o p r e v e n t o x i d a t i o n of t h e l a b i l e r e d u c e d p t e r i d i n e s , which a r e n o t a d e q u a t e l y p r o t e c t e d by s u b s t i tution a t the N5 position. Since n e u t r a l o r a l k a l i n e solut i o n s of l e u c o v o r i n a r e r e l a t i v e l y s t a b l e i n a i r , t h i s p r e c a u t i o n may n o t b e r e q u i r e d f o r r o u t i n e a s s a y .
CALCIUM LEUCOVORIN
6.6.3
Column Chromatography
L e u c o v o r i n h a s been chromatographed on columns of d i f f e r e n t p a c k i n g m a t e r i a l s s i n c e i t w a s f i r s t synthesized. E a r l y i n v e s t i g a t o r s used magnesium s i l i c a t e and a c t i v a t e d c h a r c o a l , g s t a r c h , 6 and--more r e c e n t l y - DEAE c e l l u l o s e ' ' i n t h e i r p u r i f i c a t i o n and i s o l a t i o n of leucovorin. Column t e c h n i q u e s h a v e b e e n c o u p l e d w i t h v a r i o u s d e t e c t i o n methods t o i d e n t i f y and q u a n t i t a t e CF and o t h e r f o l a t e s i n n a t u r a l l y o c c u r r i n g p r o d u c t s . Noronha and S i l ~ e r m a nused ~ ~ &. c a s e i , P . c e r e v i s i a e , a n d S. f a e c a l i s t o d e t e c t f o l a t e s i n chicken l i v e r e x t r a c t s chromatographed on DEAE c e l l u l o s e . A s i m i l a r method w a s u s e d by R o h r i n g e r e t a 1 . 7 0 t o m o n i t o r f o l a t e s i n h e a l t h y An e a r l i e r p u b l i c a t i o n " and i n f e c t e d wheat l e a v e s . r e p o r t e d anion-exchange chromatography on Dowex-lc h l o r i d e u s i n g uv a b s o r p t i o n o f c o l l e c t e d f r a c t i o n s f o r d e t e c t i o n . Due t o i t s i n s t a b i l i t y i n a c i d , l e u c o v o r i n w a s e l u t e d w i t h N a C l r a t h e r t h a n H C 1 , which i s commonly u s e d f o r o t h e r f o l a t e s . T h i s method w a s l i m i t e d t o synt h e t i c products r a t h e r than b i o l o g i c a l mixtures. The a u t h o r s f e l t t h a t s e n s i t i v i t y c o u l d be g a i n e d by microbiological detection. More r e c e n t l y , a t t e n t i o n h a s been p l a c e d on g e l p e r meation te c h n iq ues . Sephadex G-15 and G-25 columns c o u p l e d w i t h uv d e t e c t o r s w e r e u s e d t o s e p a r a t e f o l a t e s u s~e d found i n r a t k i d n e y e x t r a c t s . 7 2 K B s and C e r 1 - 1 9 ~ Sephadex G-10 t o s e p a r a t e f o l a t e s i n cow's m i l k , u t i l i z i n g s p e c t r o s c o p i c and m i c r o b i o l o g i c a l d e t e c t i o n . Nixon and B e r t i n ~ ' used ~ f l u o r e s c e n c e r a t i o s and m a r k e r s on DEAE Sephadex A-25 t o s e p a r a t e f o l a t e coenzymes. I n s e p a r a t i n g f o l a t e s from b i o l o g i c a l s o u r c e s , s e v e r a l a u t h o r s t r e a t e d t h e i r s a m p l e s w i t h t h e a p p r o p r i a t e conjugase t o hydrolyze polyglutamates. R a d i o a c t i v i t y measurement h a s been used t o d e t e c t doubly l a b e l e d 5fH,F and its metabolic products. 5 0
6.6.4
H i g h - p r e s s u r e L i q u i d Chromatography
A n a t u r a l e x t e n s i o n o f column chromatogr a p h y i s h i g h - p r e s s u r e l i q u i d c h r o m a t o g r a p h y , which comb i n e s s e p a r a t i o n , d e t e c t i o n , and q u a n t i t a t i o n (and i s o l a Perhaps t h e s i n g l e t i o n i n t h e c a s e of p r e p a r a t o r y w o r k ) .
34 I
9
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CALC IU h LEUCOVOR IF 8
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I
FOLIC ACID (INTERNAL STANDARD)
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5
4
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FIGURE 5
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9 12 15 18 21 24 MINUTES LSJ-59
HIGH PRESSURE LIQUID CHROMATOGRAM OF CALCIUM LEUCOVORIN
CALCIUM LEUCOVORIN
most a t t r a c t i v e f e a t u r e o f t h i s t e c h n i q u e , i s s p e e d , o n c e t h e chromatographic c o n d i t i o n s have been determined. V a r i o u s modes a r e a v a i l a b l e , b u t f o l a t e s h a v e b e e n r e s t r i c t e d t o i o n exchange o r p a r t i t i o n i n g d u e t o l i m i t e d s o l u b i l i t y i n o r g a n i c s o l v e n t s . D e t e c t i o n i s u s u a l l y by uv a b s o r p t i o n , a l t h o u g h i n t h e case of l e u c o v o r i n , s e n s i t i v i t y i s i n c r e a s e d s e v e r a l o r d e r s of m a g n i t u d e by e l e c t r o c h e m i c a l d e t e c t i o n . HPLC h a s b e e n u s e d r o u t i n e l y i n t h i s l a b o r a t o r y s i n c e 1973, and among t h e compounds a n a l y z e d a r e f o l a t e s . 7 5 The most v e r s a t i l e s y s t e m t h a t t h e s e a u t h o r s h a v e found i s a c h e m i c a l l y bonded C I S column w i t h 0 . 1 M KHIPOL (pH a d j u s t e d t o 4 . 0 ) c o n t a i n i n g v a r y i n g amounts of m e t h a n o l ( s e e F i g u r e 5 ) . An e a r l i e r s y s t e m u s i n g t h e same reverse p h a s e C I S column w i t h t r i s b u f f e r , 2-amino-2-(hydroxymethyl)-lY3-propanediol a t pH 6 . 7 , w a s abandoned i n f a v o r of t h e above p h o s p h a t e e l u e n t which b e t t e r r e s o l v e s c o n t a m i n a n t s from t h e m a j o r component. A s i m i l a r s e t of c o n d i t i o n s w a s u t i l i z e d by R e i f e t a 1 . 7 6 t o a n a l y z e f o l i c a c i d , u s i n g l e u c o v o r i n as a n i n t e r n a l s t a n d a r d . Other a u t h o r s 7 7 have used similar c o n d i t i o n s t o s t u d y e x t e n s i v e l y t h e i d e n t i t y of p o s s i b l e l e u c o v o r i n contaminants. In a d d l t i o n t o t h e s e p a r t i t i o n ' / i o n i z a t i o n s u r p r e s s i o n m e t h o d s , a n i o n exchange h p l c h a s b e e n u s e d t o s e p a r a t e CF from o t h e r n a t u r a l l y o c c u r r i n g f o l a t e s , 7 e and some c o r r e l a t i o n h a s been made between t h e number of glutamyl r e s i d u e s and r e t e n t i o n t i m e . 6.6.5
A f f i n i t y Chromatography
Although a f f i n i t y chromatography h a s n o t b e e n u s e d d i r e c t l y as a n a n a l y t i c a l method, i t may b e modified i n t h e f u t u r e t o produce a v i a b l e technique. L e u c o v o r i n h a s been used a s a n e f f e c t i v e s p a c e r i n o b t a i n i n g a c t i v e samples o f d i h y d r o f o l a t e r e d u c t a s e . 79 I f t h e enzyme c o u l d b e i m m o b i l i z e d w i t h o u t l o s i n g i t s a c t i v i t y , p e r h a p s i t c o u l d b e used t o s e p a r a t e f o l a t e s .
6.7
Radioassay
R e c e n t l y , r a d i o a s s a y methods h a v e been r e f i n e d t o measure f o l a t e s in b i o l o g i c a l s a m p l e s . These t e c h n i q u e s u s e r a d i o a c t i v e l y l a b e l e d f o l a t e s and c o m p e t i t i v e p r o t e i n binding. Johnson e t a l . compare t h i s method w i t h t r a d i t i o n a l m i c r o b i o l o g i c a l a s s a y w i t h L. c a s e i .
343
LESLIE 0.PONT ET A L .
344
Although t h i s method w a s d e s i g n e d f o r f o l a t e s i n g e n e r a l , d i f f e r e n t i a l microbiological t e s t i n g could give an indic a t i o n of r e d u c e d f o l a t e c o n c e n t r a t i o n . 7.
Acknowledgments
S u p p o r t e d by C o n t r a c t N01-CM-33723 from t h e D i v i s i o n of Cancer T r e a t m e n t , N a t i o n a l Cancer I n s t i t u t e , N a t i o n a l I n s t i t u t e s o f H e a l t h , Department o f H e a l t h , E d u c a t i o n , and W e l f a r e . The o p i n i o n s e x p r e s s e d a r e t h o s e of t h e a u t h o r s and n o t n e c e s s a r i l y t h o s e o f t h e N a t i o n a l Cancer Institute. The a u t h o r s wish t o t h a n k Michael C u l c a s i f o r t h e HPLC development, B a r b a r a S e n u t a , F l o r e n c e Yoshikawa, M a r t i n S t r u b l e , and J o h n Jee f o r t h e t e c h n i c a l a s s i s t a n c e and A r d a t h Trine f o r s e c r e t a r i a l support.
8.
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Analytical Profiles of Drug Substances, 8
METHIMAZOLE Hassan Y. Aboul-Enein and A . A . Al-Badr I,
2.
3. 4. 5. 6.
7.
Description I . I Nomenclature 1. I I Chemical Names I . 12 Generic Names I . 13 Trade Names 1 . 1 Formulae 1.2 I Empirical 1.22 Structural 1.3 Molecular Weight I .4 Elemental Composition 1.5 Appearance. Color, Odor Physical Properties 2. I Crystal Properties 2. I I Crystallinity 2. I2 Melting Point 2.2 Dipole Moments 2.3 Solubility 2.3 Identification 2.5 Spectral Properties 2.51 Ultraviolet Spectrum 2.52 Infrared Spectrum 2.53 Nuclear Magnetic Resonance Spectrum 2.54 Mass Spectrum and Fragmentometry Synthesis Stability, Decomposition Products. and Metal Complexes Metabolism Methods of Analysis 6. I Titrimetric Analysis 6.11 Aqueous 6.12 Nonaqueous 6.2 Spectrophotometric Methods 6.21 Infrared Spectrophotometric 6.22 Nuclear Magnetic Resonance Spectrometric 6.23 Ultraviolet Spectrophotometric 6.3 Chromatographic Analysis 6.3 I Thin-Layer Chromatography 6.32 Gas-Liquid Chromatography 6.33 Paper chromatography 6.0 Colorimetric Analysis 6.5 Potentiometric Analysis 6.6 Coulometric Analysis References 35 I
Copyright @ 1979 by Academic Press. Inc. All rights of reproduction in any form reserved. ISBN 0-12.260808-9
HASSAN Y . ABOUL-ENEIN AND A. A. AL-BADR
352
METHIMAZOLE
1.
Description
1.1
Nomenclature
1.11
Chemical Names 1,3-dihydro-l-methyl, 2-H-Imidazole-2-thione. 1-methylimidazole-2-thiol 1-methyl-2-thioimidazole 1-methy1-2-mercap to imidazo1e
1.12 Generic Names 1.13
Methimazole, thiamazole
Trade Names Thiamethazole, Bazolan, Dananti201, Faristan, Frentorox, Mercazole, Metazole, Tapazole, Thacapazol, Thycapazol, Strumazol, Meto thyr ine
.
1.2
Formulae 1.21 Empirical 1.22
‘qHgN2’
Structural
FH3
(iH3
114.17
1.3
Molecular weight
1.4
Elemental composition C 42.08%, H 5.30%, N 24.54%,
1.5
Appearance, color, odor White to pale buff, crystalline powder, having a faint characteristic odor. Its solution is practically neutral to litmus.
2. Physical 2.1
S 28.09%
properties
Crystal properties 2.11
Crystallinity
No detailed studies on the crystal structure
of methimazole is reported in the literature. Methimazole can be microscopically identified using Kofler’s method, the occurrence of polymorphous modification is indicated in methimazole.
353
METHIMAZOLE
2.12
Melting point USP X I X (1) s p e c i f i e s a m e l t i n g r a n g e f o r methimazole between 144 and 147O. L e a f l e t s from a l c o h o l m.p. 146-148O(2), b.p. 280' (some d e c o m p o s i t i o n ) .
2.2
Dipole Moments The d i p o l e moment of methimazole w a s determined i n benzene and 1 , 4 d i o x a n e s o l u t i o n a t 25O ( 3 ) and r e p o r t e d t o be 4 . 7 4 D and 5.53 r e s p e c t i v e l y . The r e s u l t s were d i s c u s s e d i n terms of tautomerism and m o l e c u l a r conformations.
2.3
Solubility F r e e l y s o l u b l e i n water, i n a l c o h o l and i n c h l o r o form, s l i g h t l y s o l u b l e i n e t h e r , petroleum e t h e r and benzene.
2.4
Identification The f o l l o w i n g t e s t s a r e c i t e d from USP X I X (1) :The i n f r a r e d a b s o r p t i o n spectrum of a potassium bromide d i s p e r s i o n of i t exhibitsmaxima o n l y a t t h e same wavelength a s t h a t of a s i m i l a r p r e p a r a t i o n of USP methimazole Reference S t a n d a r d . M e r c u r i c c h l o r i d e TS produces i n a s o l u t i o n (1 i n 200)a w h i t e p r i c i p i t a t e , b u t no p r e c i p i t a t i o n i s produced by t r i n i t r o p h e n o l TS. The s o l u t i o n i s c o l o u r e d i n t e n s e l y b l u e by molybdo-phosphotungst a t e TS. Methimazole c a n be i d e n t i f i e d by forming c r y s t a l s of w i t h gold bromide/HCl s o l u t i o n . P l a t e s , o f t e n i n c r o s s e s ( s e n s i t i v i t y : 1 i n 1000); potassium t r i - i o d i d e s o l u t i o n - bunches of r o d s o r n e e d l e s ( s e n s i t i v i t y 1 i n 1000) F i g . 1.
2.5
Spectral Properties 2.51
U l t r a v i o l e t spectrum Methimazole i n 0.1N s u l f u r i c a c i d shows maxima a t 211 nm ( E 1 % , 1 cm 593) and 251.5 nm ( E 1%, 1 c m 1 5 2 8 ) . I n n e u t r a l aqueous s o l u t i o n , methimazole a b s o r b s u l t r a v i o l e t r a d i a t i o n a t 251.5 nm ( F i g . 2 ) . Hayden _ e t -a1 ( 5 ) p u b l i s h e d a r e p o r t on t h e r e l a t i o n between t h e s p e c t r a and s t r u c t u r e of methimazole and some r e l a t e d compounds. The replacement of an oxygen atom a t C2 by s u l f u r c a u s e s a b i g s h i f t t o l o n g e r wavelength w i t h i n c r e a s e d a b s o r p t i o n ( 6 ) .
HASSAN Y . ABOUL-ENEIN AND A. A. AL-BADR
3 54
Fig. 1 -
Fig. 2
Methimazole
- KI/I2
crystals.
- Ultraviolet spectrum of Methimazole in methanol.
355
METHIMAZOLE
2.52
I n f r a r e d spectrum The i n f r a r e d spectrum of methimazole i s shown i n Fig. 3. The spectrum w a s o b t a i n e d from Nuj 01 m u l l . The s t r u c t u r a l assignments have been c o r r e l a t ed w i t h t h e f o l l o w i n g band f r e q u e n c i e s : Frequency (Cm-l) 2500
- 2450 broad weak
1580
Assignment
-
SH
C = N aromatic
Other f i n g e r p r i n t bands c h a r a c t e r i s t i c t o methimazole are a t 1466, 1570 and 1271 Cm-l a s shown i n F i g u r e 4 . Further information with regards t o the inf r a r e d s p e c t r a of methimazole i s g i v e n i n several r e f e r e n c e s ( 4 , 5 , 7 ) . 2.53
Nuclear Magnetic Resonance Spectrum A t y p i c a l N M R spectrum of methimazole i s shown i n F i g . 5. The sample w a s d i s s o l v e d i n CDC13. The spectrum w a s determined on ir Varian T-60 A NMR s p e c t r o m e t e r w i t h TMS a s t h e i n t e r n a l s t a n d a r d . The f o l l o w i n g s t r u c t u r a l a s s i g n ments have been made f o r Fig. 5. Chemical S h i f t ( 6 )
Assignment
S i n g l e t a t 3.63
N-CH
S i n g l e t a t 6.70
3 a r o m a t i c H and 4 H5 of t h e imidaz o l e r i n g system.
Further information concerning t h e NMR spectrum of methimazole c a n be o b t a i n e d from S a d t l e r NMR c a t a l o g (8) and a l s o from CRC A t l a s of s p e c t r a l d a t a (7) and A l d r i c h NMR catalog (9). 2.54
Mass Spectrum and Fragmentometry The mass spectrumof rnethimazole o b t a i n e d by e l e c t r o n impact i o n i z a t i o n shows a pronounced m o l e c u l a r i o n d a t m / e 114 ( F i g . 6 ) .
Bowie e t a 1 (10) s t u d i e d t h e mass s p e c t r a of s e v e r a l i m i d a z o l e s and methimazole w a s i n c l u d e d . They d i s c u s s e d t h e f r a g m e n t a t i o n
P 356
a al k cd k
H
w C
357
I
m
2
z
m
358
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HASSAN Y . ABOUL-ENEIN AND A. A. AL-BADR
patterns and modes which is substantiated by deuterium labelling, exact mass measurements and appropriate metastable ions. Skeletal rearrangements are rare in the imidazole ring system. 3.
Synthesis The method of preparation of methimazole illustrates the general synthesis of 2-mercaptoimidazoles by ring closure from a -amino-aldehydes or ketones and alkylisothiocyanates. This reaction gives 1-alkyl 2-imidazolethiols, and the simpler compounds unsubstituted in the 1-position can be made by the use of simple metallic thiocyanate in place of the alkyl compound. In the original synthesis of Wohl & Marckwald (Ber., 22, 1354, 1889) of which a number of variations have since been introduced. Methimazole is made by condensing methyl isothiocyanate with amino-acetal, NH2-CH2CH(0 Et)2 (a convenient substitute for aminoacetaldehyade) and cyclizing the product by heating with acid. The 2-mercaptoimidazols can be alkyl-
"H-CH
3
ated or acylated on the sulphur or the second nitrogen atom or the whole SH group can be removed by oxidation with HNO to give a simple imidazole. 3 Methimazole is also prepared (12,13) by the reaction of CH -NHCH2-CH(0-Et) with KSCN in the presence of dil. HC1. Hydrochloric acid t300 ml., 2N) was added gradually to a mixture of 72.5 gm of CH -NHCH2-CH(0 Et) and 56.4 gm of KSCN, the mixture kept 13 hours, evaporaged to dryness, the residue refluxed 1 hour with 200 ml. of anhydrous acetone. The mixture filtered, the precipitate washed with 50 ml acetone and the solution evaporated to give 63-8% of methimazole m.p. 147-8O Yield (75-80%). CH3-NH-CH2-CH(0CH CH ) + KSCN dil HC1 2 3 2
4. Stability, Decomposition product and metal complexes
Methimazole is a relatively stable compound at room temperature. However, it is recommended that it should
METHIMAZOLE
be kept i n a well-closed andinadry place.
36 I
container
p r o t e c t e d from l i g h t
Methimazvje forms metal complexes w i t h heavy metals e . g . C U + ~ , A 1 , Fe+3 i o n s . Foye and Lo (14) s t u d i e d t h e c h e l a t i n g p r o p e r t i e s of some i m i d a z o l e s and o t h e r r e l a t e d h e t e r o c y c l i c t h i o n e s , and r e p o r t e d a r e l a t i o n between t h e metal b i n d i n g s t r e n g t h s and t h e i r a n t i m i c r o b i a l a c t i v i t y . 5.
Metabolism When 20 mg/kg of methimazole w a s a d m i n i s t e r e d i . p . o r o r a l l y t o r a t s , u r i n a r y methimazole g l u c u r o n i d e s a c c o u n t e d f o r 36-48% of t h e d o s e i n 24 h o u r s . The o n l y o t h e r u r i n a r y m e t a b o l i t e accounted f o r 10-20% and w a s n o t c h a r a c t e r i z e d . An a d d i t i o n a l 14-20% of methimazole w a s e x c r e t e d unchanged i n 24 hour u r i n e . The b i l e c o n t a i n e d methimazole g l u c u r o n i d e and two u n i d e n t i f i e d m e t a b o l i t e s . One of which w a s t h e same a s t h e u n i d e n t i f i e d u r i n a r y m e t a b o l i t e s . Plasma p r o t e i n s bound 5% of methimazole which had no a f f i n i t y f o r a n y s p e c i f i c t i s s u e . Methimazole had a much g r e a t e r CHC13/H20 p a r t i t i o n c o e f f i c i e n t and H 2 0 s o l u b i l i t y t h a n d i d p r o p y l t h i o u r a c i l . Between 7 7 and 95% of t h e m e t h i mazole w a s e x c r e t e d i n t h e u r i n e and a p p r o x i m a t e l y 10% i n the bile. Since f e c a l excretion w a s neglegible; an e n t e r o h e p a t i c c i r c u l a t i o n w a s p r e s e n t . The h a l f l i f e of u r i n a r y e x c r e t i o n w a s 5-7 h o u r s r e g a r d l e s s of t h e r o u t e o f administration (15).
35S - l a b e l l e d methimazole g i v e n i . p . t o r a t s accumulated i n t h e t h y r o i d g l a n d where i t w a s m a i n l y o x i d i z e d t o methimazole s u l p h a t e ( 1 6 ) . Most of t h e l a b e l w a s e x c r e t e d i n t h e u r i n e . The same r e s u l t s were found i n man t o o ( 1 7 ) . P i t t m a n e t a1 (18) showed t h a t b o t h t h e t h y r o i d and a d r e n a l g l a n d s had t h e h i g h e s t o r g a n t o plasma r a t i o s of t h e d r u g a f t e r f o u r d a y s of i . v . a d m i n i s t r a t i o n i n r a t s . I t w a s r e p o r t e d t h a t methimazole i n man, i s more s l o w l y a b s o r b e d and e x c r e t e d t h a n p r o p y l t h i o u r a c i l . The plasma h a l f - l i f e i n h o u r s o f methimazole 35S w a s 2 o r 5 t i m e s t h a t of l a b e l l e d p r o p y l t h i o u r a c i l . The blood r a d i o a c t i v i t c u r v e a f t e r t h e o r a l a d m i n i s t r a t i o n of c a r b i m a z o l e - 3 5 S was v e r y s i m i l a r t o t h a t of methimazole. I t w a s s u g g e s t e d by Alexander et a 1 t h a t t h e r e n a l f u n c t i o n may have a more i m p o r t a n t i n f l u e n c e on t h e b i o l o g i c a l h a l f - l i f e of t h e d r u g t h a n t h e t h y r o i d s t a t u s ( 1 9 ) . However, t h e i d e n t i f i c a t i o n of methimazole m e t a b o l i t e s s t i l l need more i n v e s t i g a t ion.
HASSAN Y . ABOUL-ENEIN AND A. A. AL-BADR
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6, Methods of analysis
6.1. Titrimetric methods Aqueous Several titremetric methods were developed for the analysis of methimazole Silver nitrate method (1) for the standard methimazole Dissolve about 250 mg of methimazole, accurately weighed, in 75 ml of water. Add from a buret 15 ml of 0.1 N NaOH, mix and add with agitation, about 30 ml of 0.1 N AgN03. Add 1 ml of bromothymol blue TS, and continue the titration with the 0.1 N NaOH until a permanent, blue green color is produced. Each ml. of 0.1N NaOH is equivalent to 11.42 mg of C4H6N2S. For methimazole tablets Weigh and finely powder not less than 20 methimazole tablets. Weigh accurately a portion of the powder equivalent to about 120 mg of methimazole and place in 100 ml volumetric flask. Add about 80 ml of water, insert the stopper and shake by mechanical means or occasionally by hand during 30 minutes, dilute with water to volume and mix. Filter and transfer 50.0 ml of the filtrate to a 125 ml conical flask. Add from a burett3.5 ml of 0.1N NaOH, mix, and add with agitation about 7 ml of 0.1N AgN03. Add 1 ml of bromothymol blue T.S. and continue the titration with 0.1N NaOH until a permanent, blue green color is produced. Each ml of 0.1N NaOH is equivalent to 11.42 mg of C H N S. 4 6 2 Iodometric methods Kossakowski _ et _ a1 (20) developed the following method for determination of methimazole (thiamazole) in substances and tablets. solution containing 10-60 ug thiamazole was buffered at pH 5.6, treated with NaN3 and then with 0.02 M iodine solution, left 10 minutes and titrated for unchanged iodine with 0.02 M Na3As03. The method was useful in determining methimazole in compound drugs provided they A
METHIMAZOLE
363
c o n t a i n no s-'
ions.
b) By t h e method Blazek e t a1 (21) The d e t e r m i n a t i o n i s done by o x i d a t i o n of t h e -SH group w i t h 0.1N i o d i n e s o l u t i o n i n NaHC03 solution v i s u a l l y with respect t o strength o r potentiometrically ( t h e equivalence point i s d i f f i c u l t t o r e c o g n i z e ) o r i n NaOH s o l u t i o n p o t e n t i o m e t r i c a l l y , which i s more f a v o r a b l e . The e r r o r of t h e method f o r a weight of lOmg amounts is a p p r o x i m a t e l y 0.5%. iii)
I o d i n e complex method ( 2 2 ) . The p o t e n t i a l c o l o r i m e t r i c u s e of t h e i o d i n e complexes of methimazole i n CHC13 and CCl4 i s s t u d i e d . The a b s o r p t i o n maximum of methimaz o l e - i o d i n e complex a t 269 nm could b e used analytically.
iv)
Bromometry method The method was d e s c r i b e d by Varga e t a1 ( 2 3 ) . To a 2-5 mg sample i n a q u e o u s s o l u t i o n , 10 m l of w a t e r , 10 m l of 0.1N KBr03, and e x a c t l y 0.5 gm. K B r a r e a c i d i f i e d w i t h 1 . 0 m l 50% H2S04. A f t e r 15 min. 5 ml 20% K I i s added, w i t h s t a r c h i n d i c a t o r and t h e i o d i n e t i t r a t e d w i t h 0.1N NazS203. 1 m l 0.1 KBr03 = 0.0009517 methimazole. The bromometric d e t e r m i n a t i o n of methimazole and o t h e r s i m i l a r compounds i s markedly i n f l u e n c e d by t h e p r e s e n c e of e x c e s s bromide. I n g e n e r a l , t h e g r e a t e r t h e amount of bromide p r e s e n t t h e lower t h e p e r c e n t a g e of t h e compound found. The d e v i a t i o n approa c h e s a l i m i t which i s d i f f e r e n t f o r each compound (24)
.
v)
Cerimetry method The method w a s developed by Varga e t a 1 (23) 0.03 - 0.10 gm sample i n 5 m l water i s cooled t o Oo and t i t r a t e d w i t h 0.1N C e (SO!) ,using t 2 p-ethoxychrysoiodine o r ( n o t r e v e r s i b l e ) methyl orange, methyl r e d , o r thymol b l u e a s indicator. 1 m l 0.1N C e ( S 0 4 ) ~= 0.011417 gm - 1% methimazole. The e r r o r i s l e s s t h a n + V e h i c l e s of t a b l e t s do n o t i n t e r f e r e .
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6.12. Non-aqueous t r t r a t i o n A non-aqueous t i t r a t i o n method w a s developed (25,26) f o r t h e d e t e r m i n a t i o n of b a s i c compounds w i t h thio(-S-) and mercapto (-SH-) groups. The r e a c t i o n of t h e S group w i t h Hg (OAc)2 i n a c e t i c a c i d makes t h i s p o s s i b l e . Methimazole and o t h e r compounds were a l l t i t rated with HC104 i n a c e t i c acid using gentian v i o l e t as indicator. 6.2
S p e c t r o p h o t m e t r i c methods 6.21
I n f r a r e d s p e c t r o p h o t o m e t r i c method A method recommended f o r a d o p t i o n a s o f f i c i a l , f i r s t a c t i o n (27). The method i n which methimazole i s s e p a r a t e d from t a b l e t e x c i p i e n t s by column chromatography on C e l i t e 545 w i t h chloroform as t h e e l u e n t and t h e n q u a n t i t a t i v e l y measured and i d e n t i f i e d by I R spectrophotometry. T h i s method w a s s t u d i e d c o l l a b o r a t i v e l y by 10 a n a l y s t s ; a v e r a g e r e c o v e r i e s from two s i m u l a t e d and two t a b l e t s m i x t u r e s ranged from 96.6% -t 1 . 0 t o 101.1% - 0.9 ( 2 8 ) .
-
6.22
+
Nuclear magnetic resonance s p e c t r o m e t r i c An NMR procedure i s d e s c r i b e d by which methimazole i s determined i n p u r e and t a b l e t f o r m u l a t i o n . The method i s r a p i d , a c c u r a t e , p r e c i s e (S.d. 0.95%) and a l s o p r o v i d e s a s p e c i f i c i d e n t i f i c a t i o n of methimazole. The spectrum was r u n i n 10% methylene c h l o r i d e i n carbon t e t r a c h l o r i d e w i t h u s e of b e n z o i c a c i d a s a n i n t e r n a l s t a n d a r d , u s i n g t h e N-CH3 p r o t o n s of methimazole a t 3.566 and t h e a r o matic p r o t o n s of benzoic a c i d a t 7 . 5 and 8.136 as c r i t e r i a f o r a n a l y s i s ( 2 9 ) .
6.23
U l t r a v i o l e t S p e c t r o p h o t o m e t r i c method I n t h i s method, a b s o r p t i o n s p e c t r a have been determined f o r methimazole (mercazolyl) i n aqeuous a c i d and a l k a l i n e s o l u t i o n s . Aqeuous s o l u t i o n s of methimazole have an a b s o r p t i o n band i n t h e medium have r e g i o n w i t h a max a t 250 nm. I n s t r o n g a c i d and a l k a l i n e media hypsochromic and hypochromiceffects a r e o b s e r ved ( 3 0 ) .
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6.3
Chromatographic A n a l y s i s
6.31
Thin Layer Chromatography Methimazole w a s determined i n chloroform e x t r a c t s of r a t u r i n e by t h i n l a y e r chromatography on s i l i c a g e l G. ( c o n t a i n i n g 1% Zn S i l i c a t e phosphor) p l a t e s w i t h CHC13/CH30H/H20 (32 :8 :5) as d e v e l o p i n g s o l v e n t and 2,6-dichloroquinone c h l o r i m i d e a s d e t e c t i o n r e a g e n t by d e n s i t o m e t r i c scanning ( 3 1 ) . T h i s method i s s u i t a b l e f o r routine a n a l y s i s ( b e t t e r than GLC because of t h e i n s t a b i l i t y of t h e S . methylmethimazole d e r i v a t i v e ) .
6.32
Gas Liquid Chromatography T h i s method i s used f o r S-methyl methimazole on a 10% Apiezon L 5% KOH/Chromosob W column a t looo w i t h N c a r r i e r g a s . The method i s more s e n s i t i v e and more p r e c i s e t h a n TLC method, b u t d u p l i c a t e measurements must b e made on t h e same day due t o i n s t a b i l i t y of Smethylmethimazole (32). C l a r k e ( 4 ) r e p o r t e d r e t e n t i o n t i m e of 0.43 r e l a t i v e t o diphenhydramine under c o n d i t i o n of methimazole d e s c r i b e d i n t h e monograph.
+
6.33
Paper Chromatography C l a r k e (4) d e s c r i b e d s e v e r a l s o l v e n t s systems used f o r paper chromatography of methimazole a s shown i n T a b l e 1. Table 1.
S o l v e n t System
V i s u a l i s i n g Agent
Acetate B u f f e r (pH 4.58)
ultraviolet i o d o p l a t i n a t e spray (white)
Phosphate B u f f e r (PH 7.4)
ultraviolet 0.00 i o d o p l a t i n a t e spray (white)
34,35
C i t r i c acid: H20: n-butanol ( 4 . 8 g : 130 m l : 870 m l ) .
ultraviolet iodoplatinate
36,37
Rf 0.27
0.72
Ref. 33
HASSAN Y. ABOUL-ENEIN AND A. A . AL-BADR
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6.4
Colorimetric A n a l y s i s I n t h i s method t h e r e a c t i o n of d i p h e n y l p i c r y l h y d r a aim w i t h methimazole ( t h i a m a z o l e ) w a s s u f f i c i e n t l y rapid f o r its use i n a spectrophotometric assay. -5 When t h e c o n c e n t r a t i o n of t h e r e a g e n t w a s 4 x 1 0 M and t h e molar r a t i o of methimazole t o t h e r e a g e n t w a s 2 : 1 0 , d e c o l o r a t i o n stopped a f t e r 90 m i n u t e s a t 26'. The r e a c t i o n m i x t u r e t h e n c o n t a i n e d b i s (l-methylimidazol-2-yl) disulphide, t h e reagent, diphenylpicrylhydrazine. A f t e r s e v e r a l h o u r s t h e decoloration s t a r t e d again giving rise t o a multip l i c i t y of c o l o r e d compounds some of which were a l s o formed i n a m e t h a n o l i c s o l u t i o n of t h e r e a g e n t . R e a c t i o n mechanisms were proposed f o r equimolar amounts of t h e r e a c t a n t s as w e l l as f o r t h e r e a c t i o n of methimazole w i t h e x c e s s of t h e r e a g e n t and f o r t h e r e a c t i o n of t h e r e a g e n t w i t h t h e d i s u l p h i d e of methimazole (38). Szabo e t a1 (39) d e s c r i b e d method f o r i d e n t i f i c a t i o n and d e t e r m i n a t i o n of methimazole by c o n v e r s i o n i n t o i t s coloured 1 : l C U + ~ complex which h a s an a b s o r p t i o n max. a t 614 nm. The complex i s n o t s t a b l e , b u t on t r e a t m e n t w i t h H C 1 , a 2 : l methimazole CuCl complex i s p r e c i p i t a t e d a s white c r y s t a l s .
6.5
P o t e n t i m e t r i c Analysis Methimazole w a s a n a l y s e d i n p h a r m a c e u t i c a l p r e p a r a t i o n s p o t e n t i m e t r i c a l l y u s i n g 0.1N chloramine. The method can d e t e c t amounts of up t o 5 mg of t h e drug w i t h an a c c u r a c y of 98-99.5% ( 3 9 ) . An a l t e r n a t i v e method w a s d r s c r i b e d by P i n z a u t i ( 4 0 ) f o r d e t e r m i n a t i o n of s e v e r a l a n t i t h y r o i d d r u g s p o t e n t i m e t r i c a l l y w i t h 0.01 M m e r c u r i c acet a t e w i t h u s e of a m e r c u r i c s u l f a t e r e f e r e n c e e l e c t r o d e and an amalgamated gold o r a s i l v e r i n d i cator-electrode. The method i s r a p i d and t h e res u l t s a r e reproducible; t h e e r r o r s are a l l within +- 0.36%.
_ et _ a1
6.6
Coulometric d e t e r m i n a t i o n C e r t a i n t h i o l s , i n c l u d i n g methimazole, were d e t e r mined c o u l o m e t r i c a l l by d i r e c t t i t r a t i o n w i t h e l e c t r o - g e n e r a t e d HgT2 ( 4 2 ) . The c o u l o m e t r i c a s s a y i s c a r r i e d o u t i n a c e l l having t h r e e compartments s e p a r a t e d from each o t h e r by s i n t e r e d - g l a s s d i s c s . One compartment c o n t a i n s t h e mercury f o r t h e e l e c t r o -
METHIMAZOLE
367
g e n e r a t i o n of Hg+2, t h e mercury i n d i c a t o r e l e c t r o d e and t h e S . C . E . ( e n c l o s e d i n a P e r l e y t u b e c o n t a i n i n g 4 M-sodium n i t r a t e t o a v o i d i n t e r f e r e n c e w i t h C S ) ; t h e second i s f i l l e d w i t h s u p p o r t i n g e l e c t r o l y t e (an aqueous s o h . 0.05 M i n Na2B407 and 0.5M KNO3 and of pH 9 . 3 ) ; and t h e t h i r d a c t s as a n a u x i l l i a r y compartment. The c o u n t e r - e l e c t r o d e i s of p o l i s h e d p l a t inium
.
REFERENCES 1. The United S t a t e s Pharmacopeia X I X , United S t a t e s Pharm a c o p e i a l Convention, I n c . , R o c k v i l l e , Md., 20852, p. 313-314. 2 . Merck I n d e x , N i n t h e d i t i o n , Merck & Co., N . J . , U.S.A., p. 78, 5841.
I n c . , Rahaway,
3. C.W.N. Camper, G.D. P i r k e r i n g , J. Chem. SOC., P e r k i n s T r a n s . , 2, 2045 (1972). 4. E . G . C . C l a r k e , " I s o l a t i o n and I d e n t i f i c a t i o n of Drugs", The P h a r m a c e u t i c a l P r e s s , London, 1969, p. 413. 5. A . L . Hayden and M. M a i e n t h a l , J . Assoc. O f f i c e . Agr. Chemists, 48, 596 (1965); t h r o u g h Chem., A b s t r . , 6793 ( 1 9 6 5 c 6. H . Y .
Aboul-Enein,
unpublished r e s u l t s
63,
.
7 . "CRC Atlas of s p e c t r a l d a t a and P h y s i c a l C o n s t a n t s of Organic Compounds'' e d i t e d by J . G . G r a s s e l l i , CRC Press, C l e v e l a n d , Ohio, 1973. 8 . S a d t l e r NMR C a t a l o g , S a d t l e r R e s e a r c h L a b o r a t o r i e s , I n c . , P h i l a d e l p h i a , Pa. 1970. 9. A l d r i c h L i b r a r y of NMR S p e c t r a , by C . J . P o u c h e r t and John R. Campbell, Vol. V I I I , s p e c t r u m 30A.
10. J . H . Bowie, R.G. Cooks, S . O . Lawesson and G. S c h r o l l , Aust. J . Chem., 20, 1613 (1967). 11. R.G.
J o n e s , E.C. K o r n f e l d , K.C. McLaughlin, and R.C. Anderson, J . h e r . Chem. S O C . , 71,4000 ( 1 9 4 9 ) .
HASSAN Y . ABOUL-ENEIN AND A. A. AL-BADR
368
12. I . B .
Simon and 1.1. Kovtunovskaya - Levshina, T r . Ukr., I n s t . Eksperim, E n d o r k r i n o l , 18,345 (1961), t h r o u g h Chem. A b s t r . , 50, 7 9 2 1 (1963), a l s o see Chem. A b s t r . , 50, 3 4 1 6 h (1960).
13. I . B .
Simon and 1.1. Kovtunovskaya-Levshina, T i o l o y e Soedinen. Med., Ukrain, Nauch, - I s s l e d o v a t e . S a n i t Khim I n s t . , Trudy Nauch Konf., 1957, 406 (Pub. 1959), through Chem. A b s t r . 54, 24760 (1960).
w.,
Foye, J. Lo, J . Pharm. S c i . ,
1 4 . W.O. 15. D.S.,
61,
1209 (1972).
S i t a r , D.P., T h o r n h i l l , J . Pharmacol, Exp. T h e r . , 184, 432 (1973).
91,
747
16. B .
Marchant, (1972).
17. B .
M a r c h a n t , W . D . A l e x a n d e r , J. C l i n . E n d o c r i n o l . Metab., 34, 847 (1972).
W.D.
Alexander, Endocrinology,
18. J . A .
P i t t m a n , R . J . Beschi, T . C . Smitherman, J. C l i n . E n d r o c r i n o l . Metab. 33, 182 (1971).
19. W.D.
Alexander, V. Evans, A. MacAulay, T.F. G a l l a g h e r , Jr. and J. Londons,Brit. Med. J . , 290 (1969).
2,
Act. 20. J . Kossakowski; J. Klopocki; T. Kuryl; B. Zbikowski, P o l . Pharm. 29, 465 (1972). 21. J. Blazek; J . Kracemar and Z . S t e j s k a l ; Ceskoslov. f a r m . , 6, 4 4 1 (1957); through _ Chem. __ A_ b s t_ r . -54, 9204 (1960). 22. E . Z o e l l n e r , G . Vastagh, Acta. Pharm. Hung., through Chem. A b s t r . 73, 69923c (1970).
5,29,
(1970)
23. E. Varga and E. Zb'llner, Acta. Pharm. Hung. 25, 1 5 0 (1955), through Chem. Abstr. 52, 12327 (1958).
Acta. Chem. Acad. S c i . Hung., 24. E. Z o e l l n e r and E. Varga, 12, 1 (1957), through Chem. Abstr., 52, 520SF (1958). 25. G. Posgay, Pharm. Z e n t r a l h a l l e 100, 65 (1961); Chem. A b s t r . 55, 14819 a (1961).
through
26. I . Bayer and G. Posgay, Acta. Pharm. Hung. 2, Suppl. 43 (1961), through Chem. A b s t r . 56, 7 4 3 1 (1962).
369
METHIMAZOLE
2 7 . A.L. Hyyden and L. Brannon, J. A s s . O f f i c . Anal. Chem., 50, 674 ( 1 9 6 7 ) .
28. O f f i c i a l methods of A n a l y s i s of t h e A s s o c i a t i o n of O f f i c i a l A n a l y t i c a l Chemist., p u b l i s h e d by OAAC, Washington DC 2 0 t h Ed., William Horwitz ( e d i t o r ) 1 1 t h ed. (1970) p . 685.
2. Pharm.
29. H. Y . Aboul-E n e i n , press).
Verzina, Farm.-Zh. (Kiev.) 2 3 , 28(1968)
30. T s . I . Shakh; A.E. 31. J . B .
Pharmacol. 31, 1979, ( i n
S t e n l a k e ; W.D.
S k e l l e r n , J . Chromatog.
W i l l i a m s ; G.G.
53, 285, (1970) and r e f e r e n c e s were c i t e d T h e r e i n . 32. E. Niomiya; H . U s a m i ; H . Yamada, A. Morikawa, K . Matsuyama, K . K a t o , I r y o 23, 273 (1969) t h r o u g h Chem. A b s t r . , 71, 536124. (1969). 33. H . V .
Street, (1962).
&.
Pharmacal. T o x i c a l . ,
34. H.V.
Street, J. F o r e n s i c S c i . SOC.
35. H . V .
Street,
36. A . S .
Curry and H. P o w e l l , N a t u r e ,
2.
Pharm. Pharmacol.
2,
19,312
and 325
118 (1962).
14,56 (1962) 2, 1143 ( 1 9 5 4 ) .
37. E . G . C . C l a r k e , Methods of F o r e n s i c S c i e n c e , ed. Frank L u n d g u i s t , New York, I n t e r s c i e n c e P u b l i s h e r s , Vol. 1, p. 31, 1962. 38. H.B. 39. A . E .
Berg, A cta, Pharm. S u e c i c a -
S,
431 ( 1 9 7 1 ) .
Szabe, G . S t a j e r , and E . V i n k l e r , Pharmazie, (1974).
2, 615
40. S.G. Avakyants, A.M. Murtazaev, DoL1. Akad. Nauk Uzb. S R . , 26 35 ( 1 9 6 9 ) ; t h r o u g h Chem. Ab s t r . , 72,103778a ( 1 9 7 0 ) . 41. S . P i n z a u t i , V . D a l P i a z and E. L a P o r t a , Farmaco., 3. P r a t . 28, 396 ( 1 9 7 3 ) ; t h r o u g h Anal. A b s t r . , 26, 1220 42. C . A . Mairesse Patriarche,
- Ducarmois, 2.
J . L . Vandenbalck, and G . J . Pharm. B e l g . , 28, 300 ( 1 9 7 3 ) .
HASSAN Y . ABOUL-ENEIN AND A. A. AL-BADR
370
ACKNOWLEDGEMENT
The authors would like to thank Mr. Dennis Charkowski, Department of Pharmacology, University of Iowa, Iowa City, Iowa 5 2 2 4 2 , U.S.A.,
for determining mass spectrum
of methimazole, Mr. Essam A. Lotfi and Mr. Muhammad Naeem
A. Akhtar, Faculty of Pharmacy, University of Riyad, Riyad for the ultraviolet determination and typing the manuscript respectively.
Analytical Profiles of Drug Substances, 8
NALIDIXIC ACID Patricia E . Grubb I.
2.
3. 4. 5.
6.
7. 8.
9.
Description 1 . I Name, Formula, Molecular Weight 1.2 Appearance, Color, Odor Physical Properties 2. I Spectral Properties 2.1 I Mass Spectrum 2.12 Infrared 2.13 NMR 2.14 Ultraviolet Spectrum 2.15 Fluorescence 2.2 Crystal Properties 2.21 Crystallinity and X-Ray Diffraction 2.22 Solubility 2.23 pKa 2.24 Melting Range 2.25 Differential Scanning Calorimetry Synthesis stability and Degradation Drug Metabolic Products and Pharmacokinetics 5 . I Metabolic Products 5.2 Pharmacokinetics Methods of Analysis 6 . I Elemental Analysis 6 . 2 Nonaqueous Titration 6.3 Spectrophotometric 6 . 4 Colorimetric 6.5 Polarographic 6.6 Chromatographic 6.61 Thin-Layer and Paper Chromatography 6.62 Liquid Chromatography 6.63 Gas Chromatography 6.7 Spectrofluorimetric Identification and Determination in Biological Fluids Identification and Determination in Biological Fluids References
37 I
Copyright @ 1979 by Academic Press. Inc. All rights of reproduction in any form reserved. ISBN 0-12-260808-9
312
1.
PATRICIA E. GRUBB
Description 1.1
Name, Formula, Molecular Fjeight
Nalidixic acid is l-ethyl-1,4-dihydro-7-methyl-4oxo-1,8-naphthyridine-3-carboxylic acid.
1.2
H N 0
Molecular Formula:
C
Molecular Weight:
232.24'l)
12 12 2 3
Appearance, Color, Odor
Nalidixic acid is a white to slightly yellow, odor(2) less crystalline powder. 2.
Physical Properties 2.1. Spectral Properties 2.11 Mass Spectrum The low resolution mass spectrum of nalidixic is presented in Figure 1. It was obtained on a Joel JMS OlSC Mass Spectrometer at an ionization potential of 75 eV. The fragmentation pattern is presented in Figure 2. The molecular ion (m/e=232) is present at an intensity of 18%; the loss of CO gives a fragment of mass 188 which is the most agundant ion. 2.12 Infrared The infrared spectrum of nalidixic acid in a K B r pellet is presented in Figure 3 . The spectrum was obtained on a Perkin-Elmer Infrared Spectro-
photometer Model 21. It agrees with the spectrum presented by Salim and Shupe. ( 2 )
7
0 0
Lo
0
PATRICIA E. CRUBB
374
Figure 2
Fragmentation Pattern
of Nalidixic Acid
PATRICIA E. GRUBB
376
The c a r b o x y l i c a c i d OH b a n d s i n t h e r e g i o n o f 3300-2500 cm-1 a r e weak and b r o a d , i n d i c a t i n g t h a t hydrogen bonding w i t h t h e c a r b o n y l may b e present.(3) The i n t e n s e p e a k a t a b o u t 1 7 1 5 cm-1 i s p r o b a b l y d u e t o t h e C=O s t r e t c h i n g of t h e c a r b o x y l i c a c i d . The peak a t 1620 c m - 1 may b e d u e t o t h e C=O s t r e t c h of t h e c a r b o n y l a t p o s i t i o n 4 o r t h e C=C s t r e t c h of C-2 and C-3, c o n j u g a t e d w i t h t h e c a r b o n y l , o r a c o m b i n a t i o n of t h e s e two vibrations. 2.13
NMR
The NMR s p e c t r u m of n a l i d i x i c a c i d i s p r e s e n t e d i n F i g u r e 4. I t w a s o b t a i n e d on a V a r i a n A60 s p e c t r o m e t e r . T h i s s p e c t r u m i s i n agreement w i t h t h e s e c t r u m p r e s e n t e d by Hamilton and cow o r k e r s . ( l ) The f o l l o w i n g a s s i g n m e n t s h a v e b e e n made.
t
ppm
I/p r o t o n s
description
1.75
3(triplet)
-CH CH
2.98
3(singlet)
5.12
2(quartet)
7.85
l(doub1et)
-2 C(6)H
8.85
1( d o u b l e t )
C(5)H
9.47
l(sing1et)
C(2)H
2 -3 -CH ( a r o m a t i c ) -3 N-CH -CH3
2.14 U l t r a v i o l e t Spectrum F i g u r e 5 shows t h e u l t r a v i o l e t s p e c t r a of n a l i d i x i c a c i d a t a b o u t 7 . 5 mcg/ml i n 0 . 1 N NaOH, m e t h a n o l , and c h l o r o f o r m , o b t a i n e d on a P e r k i n E l m e r 323 r e c o r d i n g s p e c t r o p h o t o m e t e r . The i n t e n s i t y , p o s i t i o n , and f i n e s t r u c t u r e p r e s e n t i n each spectrum i s r e l a t e d t o t h e s o l v e n t p o l a r i t y . These s p e c t r a are i n a g r e e m e n t w i t h t h e s p e c t r a p u b l i s h e d by S a l i m and Shupe, (2) Zubenko and Shcherba a l s o r e p o r t t h a t t h e r e a r e two bands i n methanol and 0 . 1 N NaOH, a t 258 nm and 324 o r 332 nm, r e s p e c t i v e l y T ( 5 ) G a f a r i ( 6 ) h a s r e p o r t e d t h r e e bands i n m e t h a n o l : 213-216 nm ( 1 L a > , 255 nm (1Lb) and 320-322 nm ( m ) . G a f a r i a l s o r e p o r t s a n a b s o r b a n c e i n 0 . 1 N NaOH a t 279-281 nm and 325 nm. These w a v e l e n g t h s a r e a b o u t 3-10 nm l o w e r t h a n t h o s e r e p o r t e d by o t h e r s o u r c e s . (2) ( 5 ) ( 7 )
--(?
--n
0-0
0 c
0
-0
--h
::
0 0 w
n
379
NALIDIXIC ACID
2.15 Fluorescence Nalidixic acid exhibits strong fluorescence in acidic solutions. McChesney and co-workers used 0.1 N H SO ( 8 ) with an excitation wavelength - 2 4 o f 330 nm, measuring emission at 375 nm. Browning(9) used 21.5 H SO with excitation at 4 325 nm and emission at 406 nm. Figure 6 shows the fluorescence excitation and emission spectra of nalidixic acid in 0.5 N H SO determined on an 2 4 Aminco Bowman Spectrophotofluorimeter
.
2.2
Crystal Properties 2.21 Crystallinity and X-ray Diffraction Prismatic crystals of nalidixic acid elongated along the c axis were grown in ethanollwater solution by Achari and Neidle.(lO) The crystals were found to be monoclinic and of the space group P21/C. The x-ray diffraction pattern of the single crystal was solved for the structure of the molecule. The bond lengths and angles of all nonhydrogen atoms were determined. The values found compare favorably with those reported for 1,8naphthyridine and 3-ethoxycarbonyl-4-oxo-6-methyl homopyrimidazole. Nalidixic acid is calculated to be slightly non-planar; each ring is planar but the ring fusion has induced a slight buckling of the ten-membered ring. The above-mentioned compounds also have similar buckling. An intramolecular hydrogen bond is found between the carbonyl oxygen and the hydrogen of the carboxylic acid. The parameters of the monoclinic crystal are
a b =13.133 a
a
=
8.913
c
=
9.31
2
a
=99.75
2
The measured density is 1.41, the calculated density is 1.425 g/cm3 for Z=4. The refractive indices of crystals of nalidixic acid have been reported as a=1.510, 8=1.800, and “6‘=1.880. (4)(11)
PATRICIA E. GRUBB
380
Figure 6
FLUORESC ENCE SPECT RUM
of Nalidixic Acid
Excitation maximum 330 nm Emission maximum 365 nm (uncorr e ded spectrum)
200
25 0
300
350
nm
400
450
500
NALlDlXlC ACID
38 I
2.22 Solubility The solubilities of nalidixic acid in various solvents at 23" are listed below. Solvent chloroform toluene ethyl acetate methanol ethanol isopropanol water (distilled) ethyl ether
Solubility (mg/ml) 35
1.6 .8
1.3
.9 .4 .I
.1
The partition coefficients between water and various organic solvents have been reported by Sulkowska and Staroscik. ( 1 2 ) The pH-solubility profile has been studied by these workers and also by Takasugi and coworkers. (13) 2.23 pKa The pKa of the protonation of the nitrogen in position 8 has been reported as 6.02 and the pKa for the carboxylate anion formulation has been reported as -0.94. These were determined by Staroscik and Sulkowska by a spectrophotometric method.(l4) Further study by the same workers on the partition equilibria of nalidixic acid between water and various organic solvents led to calculations of the pKa values of 5.99 + 0.03 for Nprotonation and -0.86 + 0.07 for-carboxylate anion formation. (12) Takasugi and co-workers reported the apparent pKa of nalidixic acid to be 5.9 at 28" by a spectrophotometric method. ( 1 3 ) 2.24 Melting Range The melting range of nalidixic acid is reported to be 225-231", determined as a class 1 compound. (1) (2)
PATRICIA E. GRUBB
382
2.25 Differential Scanning Calorimetry A DSC scan for nalidixic acid was performed The instrument used was a by Houghtaling.(g) Perkin-Elmer DSC-1B at a scan rate of l"/min. The curve is presented in Figure 7. A sharp peak at 229-230.5" (corr) represents the sample melting.
3.
Synthesis
The synthesis of nalidixic acid was reported by Lesher and Gruett. (15) (16) It may be prepared by the procedure shown in Figure 8. 4.
Stability and Degradation
Nalidixic acid is stable up to five years under reasonable conditions of temperature and humidity. Pawelczyk and Plotkowiakowa(l7) subjected sodium nalidixate solutions to accelerated aging, but were unable to identify decomposition products. Detzer and Huber(l8) studied the photolysis and thermolysis of nalidixic acid in the presence of oxygen. Photolysis produced de-carboxylated nalidixic acid, structure A, and a diketone product, structure B y as well as carbon dioxide and ethylamine.
Structure A
Structure B
Thermolysis also produced the decarbonylation product plus a dimer, structure C.
Structure C
NALIDIXIC ACID
383
Figure 7
-I
I
,
.-.
,
.
I
1-
1
I
p / n LI n
--t-- ---I
T t
---ti--
+ t. t
---
-
-.---rI
__
i
. ,
_.
.
~
*
I
--t I
-
t----
-
t -
._
I
. _.
I
-- -
.+__
ii
I 1
it9
- - r .I ' C
1
I
---?--i
I
4--
n CI
0
a
Y
I c
*Z
v)
N
m
N
r
8 0 0
V
v
I"
+ m
m
n
I
+ N
I
r
I
Ql
fiZ
( \= / J I"'
\
I
"p" om I
NALIDIXIC ACID
5.
385
Drug M e t a b o l i c P r o d u c t s and P h a r m a c o k i n e t i c s 5.1
Metabolic Products
N a l i d i x i c a c i d i s a s y n t h e t i c a n t i b a c t e r i a l compound t h a t i s used i n t h e t r e a t m e n t of u r i n a r y t r a c t i n f e c tions. It i s more a c t i v e a g a i n s t gram-negative t h a n g r a m - p o s i t i v e organisms. ( 4 ) The compound i s r a p i d l y a b s o r b e d as t h e f r e e a c i d ; i t i s e x c r e t e d i n t h e u r i n e by man i n s e v e r a l forms. ( 8 ) A s m a l l amount is e x c r e t e d unchanged, b u t a much l a r g e r f r a c t i o n is c o n j u g a t e d as t h e monoglucuronide, The most i m p o r t a n t m e t a b o l i t e i s
l-ethyl-1,4-dihydro-7(hydroxymethyl)-4-oxo-l,8naphthyridine-3-carboxylic a c i d , r e f e r r e d t o as hydrox y n a l i d i x i c a c i d . T h i s m e t a b o l i t e h a s shown t h e same o r d e r o f m i c r o b i o l o g i c a l a c t i v i t y i n v i t r o as n a l i d i x i c a c i d . The monoglucuronide c o n j u g a t e of 7-hydroxynalid i x i c a c i d h a s a l s o been found, a s w e l l as t h e 3,7No a n t i b a c t e r i a l a c t i v i t y d i c a r b o x y l i c a c i d product. h a s been found f o r t h e g l u c u r o n i d e s o r f o r t h e 3,7d i c a r b o x y l i c a c i d . I n a d d i t i o n , no g l u c u r o n i d e of t h e 3 , 7 - d i c a r b o x y l i c a c i d h a s been r e p o r t e d . S i m i l a r m e t a b o l i t e s were found produced by man(l9) (20) ( 2 1 ) , monkeys ( 8 ) , dogs ( 8 ) , c h i c k e n s ( 2 2 ) , c a l v e s ( 2 3 ) and m i c r o o r g a n i s m s ( 4 ) . The r a t i o s of t h e s e m e t a b o l i t e s , however, were found t o v a r y w i t h t h e i n d i v i d u a l . The o v e r a l l c o n v e r s i o n of n a l i d i x i c a c i d t o h y d r o x y n a l i d i x i c a c i d had been r e p o r t e d by McChesney(8) t o b e n o r m a l l y a b o u t 32%; b i c a r b o n a t e supp l e m e n t a t i o n i n c r e a s e d t h i s t o a b o u t 40%. B i c a r b o n a t e s u p p l e m e n t a t i o n a l s o i n c r e a s e d t h e amount of t o t a l n a p h t h y r i d i n e e x c r e t e d i n t h e b i o l o g i c a l l y a c t i v e form.
Two s e p a r a t e s t u d i e s have r e p o r t e d on t h e r a t i o s of t h e various metabolic products excreted i n t h e u r i n e by man. I n a d d i t i o n , Portmann and co-workers c a l c u l a t e d t h e o r e t i c a l amounts based on t h e i r r a t e equations. ( 2 4 )
PATRICIA E. GRUBB
386
Compound
Calc.amts. Found (24) Found (21) (mg per lg dose) (mg per lg dose) %
Nalidixic acid
9
8 +- 3
0.5-5 %
Hydroxynalid ixic acid
105
129 + - 8
2.5-6 %
NA-glucuronide
517
537 + - 49
24-80%
1-HNA-glucuronide
221
229 + - 32
11-12%
3,7-dicarboxylic acid
74
43 + - 6
not reported
In glucuronides were not found as metabolic products by Hamilton(4) in studies of various fungi. The major metabolite of the microorganisms was hydroxynalidixic acid. The dicarboxylic acid was also found as a product in a number of microorganisms. The mechanism of action of nalidixic acid against
-E. coli. was found to be inhibition of DNA synthesis.(25) No selective effect on purines or pyrimidines was found and no inhibition of initiator synthesis was demonstrated. In addition the nalidixic acid could be removed from cultures after exposures up to 75 minutes by rinsings and cells would recover from the block. 5.2
Pharmacokinetics
The pharmacokinetics of nalidixic and hydroxynalidixic acids have been studied by several different groups. Takasugi et a1 studied in-situ and in-vitro absorption of nalidixic acid from the gastrointestinal tracts of rats as a function of pH. They reported that the absorption of non-ionized nalidixic acid was faster than the ionized form, with the maximum absorption rate constant found when the drug was administered from a pH=3 buffer solution. The absorption in-situ was found to be ten times the rate in-vitro, but this was dependent on several factors. (13) Moore and co-workers(19) described a simplified model for nalidixic acid metabolism by combining the
NALlDIXlC ACID
387
two m i c r o b i o l o g i c a l l y a c t i v e f o r m s , n a l i d i x i c and h y d r o x y n a l i d i x i c a c i d , and t h e two c o n j u g a t e d p r o d u c t s of t h e a c t i v e forms. T h i s model i s shown below i n F i g u r e 9. Figure 9 S i m p l i f i e d Model f o r K i n e t i c pathways of N a l i d i x i c a c i d i n Man
Nalidixic acid
lag time
> A kA,B
A =Nalidixic acid in GI tract B =totalactivedrug in body CB=conjugated drug in body U =total active drug excreted CU= conjugated drug excreted
“.I
cu
The r a t e c o n s t a n t s f o r metabolism and e x c r e t i o n were f u r t h e r combined t o a r a t e c o n s t a n t f o r t h e d i s a p p e a r a n c e of t h e d r u g , kd. Four d o s a g e forms were s t u d i e d and i t w a s found t h a t k was d c o n s t a n t f o r a l l forms e x c e p t f o r a c o a r s e , s l o w l y d i s s o l v i n g powder. Portmann and co-workers t h e n s t u d i e d t h e k i n e t i c pathways i n man f o r h y d r o x y n a l i d i x i c a c i d , t h e a c t i v e p r i m a r y m e t a b o l i t e . ( 2 6 ) The r a t e constants f o r glucuronide formation, oxidation t o t h e d i c a r b o x y l i c a c i d and e x c r e t i o n of hydroxyn a l i d i x i c a c i d were c a l c u l a t e d . E s s e n t i a l l y t o t a l a b s o r p t i o n of h y d r o x y n a l i d i x i c a c i d w a s found i n e v e r y c a s e . Good agreement between e x p e r i m e n t a l and t h e o r e t i c a l plasma l e v e l s , based on t h e f i r s t o r d e r r a t e a p p r o x i m a t i o n s used f o r t h e model, w a s found. Again, t h e d i s a p p e a r a n c e r a t e c o n s t a n t , kd2, w a s found t o b e v e r y s i m i l a r f o r e a c h s u b j e c t , a l t h o u g h t h e i n d i v i d u a l e x c r e t i o n and m e t a b o l i c The d i s a p p e a r a n c e r a t e c o n s t a n t s v a r i e d widely. r a t e c o n s t a n t , k d 2 , w a s d e f i n e d as t h e sum of t h e e x c r e t i o n r a t e c o n s t a n t , kE2, and t h e m e t a b o l i c r a t e c o n s t a n t s t o t h e g l u c u r o n i d e and d i c a r b o x y l i c a c i d , kM and kM4, r e s p e c t i v e l y . 3
PATRICIA E. GRUBB
388
This data was then used in another study by Portmann and co-workers(24) of nalidixic acid metabolism in man in which a more elaborate model was developed and various rate constants were reported (Figure 10). This model was based on the oral administration of 1 g of nalidixic acid. Theoretical curves for plasma levels of nalidixic and hydroxynalidixic acid vs. time agreed with experimental values. McChesney and co-workers(27) then studied the effect of repeated oral dosage of nalidixic acid and found some carry-over of nalidixic acid from day to day but reported no important change in the metabolism due to multiple dosings. The half-life of nalidixic acid in plasma in man was found to be between 85 and 100 minutes by McChesney and co-workers(8) and was reported as about 100 minutes by Bruehl and co-workers(27). Another study by McChesney and co-workers on the metabolism of nalidixic acid in the immature calf (23) demonstrated a pattern of metabolism very different than in man. The half-life of nalidixic acid was found to be about 24 hours and a large amount was excreted into the feces. The immature calves were also unable to excrete nalidixic acid into the urine at concentrations greater than found in the plasma and conjugated drug was present at low levels only. Calves seven months old had metabolic patterns much closer to man; the plasma half-life was about 1.5 hours, the concentration of excretion into the urine was at least ten times that in plasma and the extent of conjugation was increased. The inability to metabolize nalidixic acid by the immature calf was considered to be due to incomplete development of its metabolic system. A similar effect was seen in human infants. (29)
6.
Methods of Analysis
6.1 Elemental Analysis The molecular formula is C H N 0 12 12 2 3'
NALIDIXIC ACID
389
F i g u r e 10
METABOLIC PATHWAYS of Nalidixic Acid in Man
Nalidixic Acid inGI tract
I
kA Nalidixic Acid in body
lkMl 4
Nalidixic Acid in
urine
kMz
Hydroxynalidixic Acid in body
‘y l k ~ 3
Hydroxynalidixic Acid in urine Hydroxynalidixic Acid Glucuronide in body
~
:*r
Nalidixic Acid GIuc ur onide
Nalidixic Acid Glucuronide in urine Dicarboxylic Acid in body
I“.’
Hydroxynalidixic Acid Dicarboxylic Acid Glucuronide in urine In urine kMl=4.5 3 xIO-’ min kA=1.8x10-2 mill-’ kEl=1.0x
min -I
k, 2=1.93X 10 -3 min-1
kM2=5.77xIO-’ min-l kM3=4.05xlO-’mn-’ k,,=
1.37~10-~ mid
PATRICIA E. GRUBB
390
Element C H N 6.2
Theory
Found for standards(30)
62.07% 5.21% 12.07%
62.11 5.21 12.00
61.98 5.20 12.32
Non-aqueous Titration
The titration of nalidixic acid in DMF with lithium methoxide has been reported(1) (2) with thymolphthalein as the indicator. It has also been titrated with sodium methoxide in ethylenediamine or DMF:methanol 1:2 with thymol blue indicator.(31) An error for this titration was reported as + 0.7%. A titration with sodium borohydride Followed potentiometrically or with thymol blue indicator has also been reported by Bachrata and co-workers. The standard deviation was reported as + - 0.60%. (32) 6.3
Spectrophotometric
The ultraviolet absorption spectrum of nalidixic acid in methanol or chloroform has an absorption maximum at about 258 nm and a broad double peak at 324 to 333 nm. In 0.1 N NaOH the band at 324 nm is shifted to a single peak at about 332 nm. The a of the band at about 258 nm is approximately 110 but varies with the solvent. ( 2 ) (5) (6)(7)
6.4 Colorimetric Nalidixic acid and sodium nalidixate form a strong colored complex with iron 111. The maximum of absorbance of the complex is 410 nm and Beer's Law is obeyed from 10 to 250 ug of nalidixic acid per m1(33), and from 0.43 to 17.05 mg iron I11 per ml. (34) Nalidixic acid complexes through the 0x0-group on C-4 and the carboxylic acid group on C-3. Three moles o f nalidixic acid complex with one mole of iron 111. The instability constant of the complex was calculated to be 2.11 x 10-8 by Dick and Murgu.(34)
NALlDIXlC ACID
391
6.5 Polarographic The polarographic behavior of nalidixic acid has been studied by Staroscik and co-workers. (35) The pH range of -2.9 to 11 in 20% DMF was investigated in the concentration range of 5 x 10-4111 and three stages of reduction were found. The potentials were found to vary linearly with pH for the first two reduction stages, while the third was constant and appeared at pH >8. The carbonyl on C-4 was shown to be reduced to the 4-hydroxy product. Nalidixic acid was reduced with sodium borohydride and the product was demonstrated to be the same as that in the polarographic reduction by TLC. 6.6
Chromatographic
6.61 Thin-layer and paper chromatography Several thin-layer and paper chromatographic systems for nalidixic acid are listed below. Chromatographic Systems for Nalidixic Acid Mobile Phase
Rf
Ref. -
toluene:dioxane(9:1) descending
.6
8
butano1:acetic acid: H 2 0 (4:l:l)
--
36
propano1:ethanol:water (6:1:3)
--
36
paper impreg. with 0.1 M Na and HPZ4
iso-butano1:ethanol:ethyl acetate:water:acetone (8.2: 1:5 : 2 ) ascending
.73
17
silica gel
methano1:water:ammonia (100:12:16)
.88
35
ch1oroform:methanol:formic
.54
37
Ad sorbent paper
silica gel
acid (90:7:3) silica gel
ethyl acetate:methanol: isopropylamine (76:20:4)
.18
37
silica gel
benzene in ethano1:acetic acid (80:10: 10)
.5
23
392
PATRICIA E. GRUBB
6.62 Liquid chromatography A high-performance liquid chromatographic method for nalidixic acid on a strong anionexchange resin column has been reported, using a mobile phase of 0.01 sodium tetraborate at pH 9.2 and 0.003 sodium sulfate. The relative retention time for nalidixic acid in the system reported by Sondach and Koch was 0.86 with sulfanilic acid as the standard at
1 . 0 0 , (38) 6 . 6 3 Gas chromatography A gas chromatographic procedure for nalidixic acid after esterification has been reported for biological samples. (39)
6.7
Spectrofluorimetric
Nalidixic acid has a strong fluorescence spectrum which has been used for its determination in biological fluids. ( 8 ) ( 9 ) (24) (26) ( 4 0 )
7.
Identification and Determination in Biological Fluids
The first spectrofluorimetric methods reported for the determination of nalidixic acid and its metabolites in biological fluids did not differentiate between nalidixic acid and hydroxynalidixic acid. The determination of free nalidixic acid and the hydroxy-metabolite in human urine plasma and feces was performed by extraction by toluene from acidified biological fh i d and subsequent fluorimetric measurement at 3251375 nm of sample re-extracted into aqueous solution. (8) Conjugated nalidixic and hydroxynalidixic acids were determined by acid hydrolysis and then toluene extraction for fluorimetric measurement of the total drug. The conjugated nalidixic acid was then determined by difference. A refined method involving extractfon of two aliquots of biological material, buffered at two different p H ' s , by toluene, and re-extraction into aqueous solution allowed the simultaneous determination of nalidixic and hydroxynalidixic acid(24) ( 2 6 ) by their differential extractabilities and fluorescent intensities. This method was extended to the differential determination of the conjugated forms of nalidixic and hydroxynalidixic acid.
NALIDIXIC ACID
393
The 3,7-dicarboxylic acid metabolite was also measured fluorimetrically by extraction with ethyl acetate:chloroform 1:l at pH=l and re-extraction into aqueous solution. The fluorescence was determined at 3501435 nm; there was no cross interference with the nalidixic acid determination. ( 8 ) Extraction of nalidixic acid with chloroform from urine has also been reported. ( 4 0 ) Another fluorimetric method for chicken liver and muscle containing not less than 100 ppb nalidixic acid was reported by Browning(9) using an ethylacetate extraction and alumina column to retain the nalidixic acid. The fluorescence was measured at 3251408 nm. Spectrophotometric measurements of nalidixic acid have been reported. Gafari -et al(41) used an extraction with ultraviolet measurement at 255 or 327 nm for blood and tissue samples. Takasugi and co-workers extracted buffered tissue homogenate with chloroform and measured the optical density at 334 nm.(l3) Several chromatographic procedures have been used for nalidixic acid and metabolites in biological fluids. Urine samples were extracted with chloroform and chr.omatographed on filter paper using the system toluene dioxane (9:l) descending chromatography. The known spots were eluted off the paper with methanol and quantitatively measured spectrophotometrically. ( 8 ) Other chromatographic systems reported include butano1:acetic acid:water (4:l:l) and propanol: ethano1:water (6:1:3) for paper chromatography. The glucuronides were also separated without prior hydrolysis using isopropano1:ethyl acetate:water (6:1:3) or propano1:ethyl acetate:acetic acid:water (5:5:1:3). (36) A high performance liquid chromatographic method was developed by Shargel and co-workers for the assay of nalidixic and hydroxynalidixic acids in human plasma and urine. (42) Extraction into chloroform and re-extraction into aqueous solution was used as the sample treatment. The column used was a 0.5 M stainless steel (2.1 mm i.d.) packed with Zipax SAX strong anion exchange resin. The column pressure was 600 psi with a flow rate of 0.8 ml/min. A modification of this procedure, using a 1 m column with a column pressure of 900 psi and a flow rate of 0.7 ml/min. and an internal standard of l-ethyl-1,4-dihydro-4-oxo-7-(4-pyridiyl)3-quinolinecarboxylic acid, was used by Goehl and coworkers (43) €or improved separation. A separate liquid chromato raphic procedure for the dicarboxylic acid was used by Lee( 4) et al. The column used was a 25 cm x 4.6 mm i.d.
8
PATRICIA E. GRUBB
3 94
Partisil PXS 10125 PAC pre-packed Magnum 9 column with a mobile phase of methano1:pH 3 0.1 citrate buffer 85:15 with a flow rate of 1.6 mlfmin. The retention time of the dicarboxylic acid was 12 minutes. A thin-layer gas chromatographic system was devised by Pittman and Shekosky(39) for chicken tissue and feces. A TLC system of benzene:methanol:acetic acid (9:l:l) was used for prior separation; the spots were then removed and esterified in 14% BF3 in methanol. A 4 ft. 3% OV-17 column at 240" was used. Retention times of about 7 minutes for nalidixic acid, 10 minutes for hydroxynalidixic acid and 17 minutes for the dicarboxylic acid were reported. A pulse polarographic system for detection of the dicarboxylic acid in the presence of nalidixic and h droxynalidixic acids was devised by Koss and Warner. (457 The reduction potential in the system used was -.54V vs. SCE. Microbiological assay procedures for nalidixic acid have also been used for biological samples. Since nalidixic and hydroxynalidixic acids have the same order of antibacterial activity in-vitro, then cannot be determined separately. Organism P. boviseptica
8.
Reference 8
B. pumilus
46
E. coli
25,47, 48,49
Identification and Determination in Dosage Forms
Nalidixic acid has been determined spectrophotometrically in tablets after chloroform extraction at a wavelength maximum of 258 nm.(1)(2) Another source reported 259 nm as the maximum for chloroform and 258 nm for 0.1 N NaOH. (7) The infrared spectrum has also been used to identify nalidixic acid in tablets.(7) Non-aqueous titration of tablet extracts with sodium methoxide(27) or lithium methoxide(1) ( 2 ) has been reported. A polarographic determination of nalidixic acid in tablets at -0.6V v s . SCE in 20% aq. DMF with 0.1 N HC1 has also been used. (35)
NALIDIXIC ACID
High performance liquid chromatography was used by Sondack and K ~ c h ( ~to ~ )assay nalidixic acid in aluminum hydroxide gel suspension.
A microbiological detection has been described for use for pharmaceutical preparations of nalidixic acid. A diffusimetric determination using E. coli (Bruxelles) was reported by Monciu. ( 4 8 )
3 95
PATRICIA E. G R U B B
396
References
1. National Formulary, =:477. 2. Salim,E.; Shupe,I.; J.Pharm.Sci. (1966) 55 (11) :1289-90. 3. Parikh,V.M., Absorption Spectroscopy of Organic Molecules, Addison-Wesley Publishing Co., (1974) :244. 4. Hamilton,P.B.: et al; Appl.Microbio1. (1969) 17 (2) ~237-41. 5. Zubenko,V.; Shcherba,I.; Farm.Zh, (1975) 30 (3):28-33 through CA 83:152437Z. 6. Gafari,A.; Farm.Zh., (1977) 1:53-6 through CA 86:179821u. 7. da Silva,M.; Noqueira,M.; Rev.Port.Farm. (1965) 15 (3):290-4 through CA 64:9513h. 8. McChesnG,E.; et al; Toxicolxnd Appl.Pharmacol (1964) 6:292-309. (1970) :723-4. 9. J.A.o.A.c. 10. Achari,A.; Neidle,S.; Acta Crysta1logr.Sect.B (1976) 32 (2) ~600-2. 11. HoughtaFng,W. ; Sterling-Wintrhop Research Institute; unpublished data. 12. Sulkowska,J.; Staroscik,R; Pharmazie (1975) 30:405-6. 13. Takasugi,N.: et al; Chem.Pharm.Bul1. (1968) 16 (1) :13-16. 14. Staroscik,R.; Sulkowska,J.; Acta Pol.Pharm. (1971) 28 (6):601-6 through CA 76:158322k. 15. Lesher,G. ; et al; J.Med.PharEChem. (1962) 5~1063-4. 16. Lesher,G.; et al; US Patent //3,149,104. 17. Pawelczyk,E.; Plotkowiakowa,Z.; Acta Pol. Pharm.(1970) 27 (2):105-11 through CA 73:91300u. 18. Detzer,N.; Hucr,B.; Tetrahedron (1975) 31:1937-41 19. Moore,W. ; et al; J.Pharm.Sci. (1965) 54 (1):36-41. 20. Pereny1,T. ; et al; Acta Microbiol.AcaxSci. Hung. (1975) 22 (4):433-45 through CA 84385914h. 21. Graber,H.; etTl; Gyogyszereink (19E) 25 (3):97-106 through= 84:173528r. 22. Browning,R.; Sterling-Winthrop Research Institute, unpublished report. 23. McChesney ,E. , et al; Toxicol Appl Pharmacol , (1969) 14 (1)~138-50. 55 (1):72-8. 24. PortmanKG.; et al; J.Pharm.Sci. (1966) -
.
.
NALIDlXlC ACID
25. Goss,W.; et al; J.Bacterio1, (1965) 89:1068-74. 26. Portmann,G.; J.Pharm.Sci. (1966) 55 (1):59-62. 27. McChesney,E.; et al; J.Pharm.Sci. (1967) 56 (5) :594-9. 28. Brueh1,P.; et al; Arzneim.-Forsch (1973) 23 CA 80:33692g. (9):1311-13 through 29. Rohwedder,H.; et al; Z.Kinderheilk (1970) 109 (2):124-34 through 974:97455r. 30. Auerbach,M., Sterling Wintrhop Research Institute, unpublished data. 31. Ignat,V.; Bera1,H.; Rev.Chim.(Bucharest) (1966) 17 (1):50 through CA 64:17360h. 32. Bachrata,M.; et al; Pharmazie (1977) 32 7) : 398-401. 33. Murgu,N.; Pharmazie (1964) 2 (11):724-5 34. Dick,I.; Murgu,N.; Rev.Chim(Bucharest) ( 964) 15 (12):757-8 through CA 62:15600h. 35. Staroscik,R.; et al; Pharmazie (1974) 2 (6): 387-90. 36. Perenyi,T.; Acta Pharm.Hung. (1975) 45 ( 5 ) : 196-206 through CA 84:27577q. 37. Crain,A.V.R. ; Sterling Winthrop Research Institute, unpublished data. 38. Sondack,D., Koch,W.; J.Chromatog. (1977) 132:322-5. 39. Pittman,K.; Shekosky,J. ; Sterling W i n t h r o p Research Institute; unpublished data. 40. Staroscik,R.; Sulkowska,J.; Acta Pol.Pharm. (1973) 30 (5):459-66 through CA 81:33082d. 41. Gafari,X; et al; Farm.Zh. (1F7) 2:92-3 through CA 87:33391c. 62 (9): 42. Sharge1,c; et al; J.Pharm.Sci. (1973) 1452-4. 43. Goeh1,T; et al; Sterling Winthrop Research Institute; unpublished report. 44. Lee,F.; et al; Sterling Winthrop Research Institute; unpublished report. 45. Koss,R.; Warner,C.; Sterling Winthrop Research Institute, unpublished report. 46 Ciuro,C.; Cienc.Ind.Farm. (1973) 5 (2):54-7 through CA 82:152437z. 47. Bauernfezd,A. ; Gruemmer,G. ; Z.Med.Mikrobio1. Immunol., (1968) 154 (1):35-9 through CA 69:33474k. 48. Monciu,D. ; et al; Farmacia(Bucharest) (1972), 20 (8):459-66 through CA 17:168693s. 49. Goss,W.; Deitz,W.; Bacteriol.Proc. (1963):93. The literature was reviewed to June 19, 1978.
397
Analytical Profiles of Drug Substances, 8
NEOMYCIN William F. Heyes I.
2.
3.
4. 5.
6.
Description 1.1 Composition, Name, Formula, Molecular Weight 1.2 Appearance, Color, Odor, Taste I .3 Definition of International Standard Physical Properties 2.1 Spectra 2. I 1 Infrared Spectrum 2.12 Ultraviolet Spectrum 2.13 NMR Spectrum 2.14 Mass Spcetrum 2.2 Physical Properties of the Solid 2.21 Hygroscopic Nature 2.22 Solubility 2.23 Specific Surface Area 2.2 Physical Properties of Solutions 2.31 Density 2.32 Viscosity 2.33 Surface Tension 2.34 Adsorption by Clays, Soils, and Minerals 2.35 Adsorption by Ion Exchange Resins Salts, Derivatives, and Complexes 3.1 Salts 3.2 Derivatives 3.3 Complexes Synthesis and Production 4.1 Commercial Biosynthesis 4.2 Synthesis of Radio-Labelled Material Stability and Degradation 5.1 Hydrolytic Degradation 5.2 Stability of Bulk Material 5.3 Stability in Aqueous Solution 5.4 Stability in Pharmaceutical Formulations 5 . 5 Compatibility with Excipient Materials 5.6 Compatibility with Other Actives Methods of Analysis 6. I Identification 6.2 Chemical Procedures 6.21 Titrimetry 6.22 Polarography 6.23 Polarimetry 6.24 Radio-Chemical Procedures 6.25 Fluorimetry 6.26 Spectrophotometry 6.3 Chromatographic Procedures 6.3 1 Counter-Current Distinction 6.32 Electrophoresis 6.33 Column Chromatography 399
Copyright @ 1979 by Academic Press, Inc. All rights of reproduction in any form reserved. ISBN 0-12-260808-9
400
WILLIAM F . HEYES
7 6.5 6.6 6.7
6.34 Paper and Thin-Layer Chromatography 6.35 Gas-Liquid Chromatography Microbiological Procedures 6.41 Turbidimetric Assay 6.42 Agar-Diffusion Assay Automated Procedures Use as an Analytical Reagent Determination in Body Fluids and Tissues
1.
Description.
6.4
1.1. C o m p o s i t i o n , N a m e , Formula, -- M o l e c u l a r Weight
Composition Commercial neomycin i s a complex mixt u r e of a m i n o g l y c o s i d e a n t i b i o t i c s o r i g i n a l l y i s o l a t e d from a c u l t u r e of S t k c p X o m y c e b d k a d i a e by Waksman and h i s c o - w o r k e r s i n 1 9 4 9 . The p r i n c i p l e components of t h e m i x t u r e are neomycin B ( 1 ) and neomycin C ( I 1 ) t o g e t h e r w i t h a s m a l l q u a n t i t y of n e a m i n e l , a d e g r a d a t i o n p r o d u c t of neomycin f o r m e r T a b l e 1 shows t h e c o n t e n t l y known as neomycin A. v a r i a b i l i t y o f neomycin B and C and neamine i n commercial s a m p l e s of neomycin a s r e p o r t e d i n t h e literature. Neomycins LP-A, LP-B and LP-C which c h e m i c a l l y a r e t h e mono N - a c e t y l d e r i v a t i v e s o f neomycins A , B and C2 may a l s o b e p r e s e n t i n s m a l l amounts. S e v e r a l o t h e r minor components h a v e rec e n t l y been i d e n t i f i e d as paromamine, paromomycin I and paromomycin I13. ( A l s o known as neomycins D , E and F r e s p e c t i v e l y ) . Table 1 C o n t e n t V a r i a b i l i t y of Neomycin Source Canada
U.K.
U.S. S. R.
Reference Neomycin B Neomycin C Neamine C o n t e n t % C o n t e n t % C o n t e n t P, to 97.5
30.8 to 4.0
80.5 to 92.0
17.5 to 8.0
63.7 to
40.0
69.2
91.6
to 3.4
N i l
5
0
6
to 2.5 N i l
7,8
40 1
NEOMYCIN
.............
neamine..
. .: H
2 6N5 q
...........
I
R l = H
R 2 = CH2NH2;
neomycin B
I1
R1 = CH2NH2
R2 = H
neomycin C
F i g u r e 1.
;
S t r u c t u r e of neomycin and neamine
WILLIAM F. HEYES
402
Names The following are alternative names for the neomycin complex, all of which have been used by Chemical Abstracts:Colimycin, Colistin(not to be confused with Polymixin) , Dextromycin,Flavomycin,Fradiomycin, Framycetin, Mycerin, Mycifradin, Neomix, Soframycin, Streptothricin BI, BII. 4 Chemical Names Neomycin B
0-2,6-diamin0-2,6-3dideoxy-aD-glucopyranosyl-(1-+4) -0-[0-"2, 6-diamino-2,6-dideoxy-@-L-a idopyranosyl- (1+3)- B-D-ribofuranosyl-s(1+5)] -2-deoxy-Dstreptarnine.
Neomycin C
0-2,6-diamino-2,6-3dideox -aD-glucopyranosyl- (1+4)-0-f0-=2, 6-diamino-2,6-dideoxy-a-D-c) glucopyranosyl-(1+3)-@-D-ribofuranosyl-3(1+5)] -2-deoxy-Dstreptamine
.
Ne amine ( formerly Neomycin A)
2-deoxy-4-0- (2,6-Cdiamino 2,6-dideoxy-a-D-glucopyranosyl) -D-streptamine
.
Chemical Abstracts Registry No. Neomycin B Neomycin C Neamine
119-04-0 66-86-4 3947-65-7
Formula Neomycin B,C
C23H46N6013
Ne amine
C12H26N406
Molecular Weight Neomycin B,C Ne amine
614.67 322.36
NEOMYCIN
1.2.
403
A p p e a r a n c e , C o l o u r , Odour, Taste
The s u l p h a t e s a l t o f neomycin ( t h e u s u a l commercial f o r m ) i s an amorphous, w h i t e o d o u r l e s s , powder which is p r a c t i c a l l y t a s t e l e s s . 1.3.
Definition of I n t e r n a t i o n a l Standard
The I n t e r n a t i o n a l R e f e r e n c e S t a n d a r d f o r neomycin9 i s d e f i n e d as c o n t a i n i n g 6 8 0 units o f a c t i v i t y p e r mg o r a l t e r n a t i v e l y 1 u n i t of a c t i v i t y i s c o n t a i n e d i n 0.0014 7mg of s t a n d a r d material. Similarly, the International R e f e r e n c e S t a n d a r d f o r neomycin B i s d e f i n e d a s containing 670 u n i t s per mg, or a l t e r n a t i v e l y 1 u n i t o f a c t i v i t y i s c o n t a i n e d i n 0.001492 mg of s t a n d a r d material. 2.
P h y s i c a l Properties 2.1. Spectra 2 . 1 1 . Infra-Red Spectrum
The s o l i d s t a t e i n f r a r e d s p e c t r a o f neomycins B & C s u l p h a t e h a v e been r e c o r d e d as a d i s p e r s i o n i n p o t a s s i u m bromide and are i l l u s t r a t e d i n F i g . 2 and 3 . The i n f r a r e d s p e c t r u m of neamine s u l p h a t e ( f o r m e r l y c a l l e d neomycin A ) a l s o as a p o t a s s i u m bromide d i s p e r s i o n i s i l l u s t r a t e d i n A l l s p e c t r a are o f a u t h e n t i c m a t e r i a l Fig. 4 . s u p p l i e d by The Upjohn Company, Kalamazoo. Sammul e t a l l o h a v e p u b l i s h e d t h e i n f r a r e d s p e c t r u m o f neomycin u n d e c y l e n a t e . 2.12.
U l t r a v i o l e t Spectrum
N o a b s o r p t i o n maxima i n t h e u l t r a v i o l e t r e g i o n 200-340nm i s o b s e r v e d w i t h s o l u t i o n s o f neomycin.
2.13.
NMR S p e c t r u m
The p r o t o n NMR s p e c t r u m of neomycins B and C h a s been u s e d by R i n e h a r t and c o - w o r k e r s 1 t o e l u c i d a t e t h e s t r u c t u r e and
3
2.5 0.0
5
4 1
00
I ,
WAVELENGTH (MICRONS) 8 6 7 . , I I . , . , II ,,. ... . I.J ... . I
- .
9
10
I
03
I
I
'
.
I
1
.
.
~-1 '
12
I
.
1
,
20
15
' .
30 4Ou) an ..
*
L
3 m
2500
2ooo
la00
1600 FREQUENCY
Figure 2.
1400
(CM')
1200
lo00
I n f r a r e d Spectrum of Neomycin B
800
wo
400
200
3
2.5
4Ooo
3500
3000
4
5
250
2000
Figure 3.
WAVELENGTH (MICRONS) 7 8 6
1800
1600 1400 FREQUENCY (CM’)
1200
9
10
1000
Infrared Spectrum of Neomycin C
12
800
20
15
600
30 4050
A00
200
33NVWOSW 31dWVS
0
u-l
..
c
H
N EOMY CIN
407
stereochemical configuration of these a n t i b i o t i c s . T r u i t t ” has extensively studied t h e 1 3 C NMR o f t h e neomvcins and d e m o n s t r a t e d t h e pH d e p e n d a n c e o f t h e s p e c t r u m o f neomycins B and C . The s p e c t r a o f t h e h e x a N - a c e t y l d e r i v a t i v e s however, w e r e shown t o be i n d e p e n d a n t o f pH t h u s allowing assignment of t h e observed chemical s h i f t s as g i v e n i n T a b l e 2 . 2.14.
Mass Spectrum
Neomycin i s i n s u f f i c i e n t l y v o l a t i l e f o r d i r e c t mass s p e c t r o m e t r i c a n a l y s i s . T o overcome t h i s p r o b l e m I n o u y e 1 4 p r e p a r e d t h e v o l a t i l e N - s a l i c y l i d e n e S c h i f f ’ s b a s e , t h e M.S. o f w h i c h , however, d i d n o t e x h i b i t a peak f o r t h e molecular i o n . T o o b s e r v e t h e m o l e c u l a r i o n i t w a s n e c e s s a r y t o use t h e o - t r i m e t h y l s i l y l e t h e r o f the N-salicylidene S c h i f f ’ s base. The s p e c t r u m o f N - s a l i c y l i d e n e neomycin w a s f o u n d t o b e d e p e n d a n t on t h e ion-chamber t e m p e r a t u r e i n d i c a t i n g t h a t thermal decomposition plays a s i g n i f i c a n t p a r t i n the fragmentation process. The M.S. e x a m i n a t i o n o f neomycin t r i m e t h y l s i l y l e t h e r f o l l o w i n g GLC h a s been rep o r t e d by Murata e t a l 1 5 . The f r a g m e n t a t i o n p a t t e r n o b t a i n e d by t h e s e w o r k e r s i s somewhat d i f f e r e n t t o t h a t o b s e r v e d by I n o u y e 1 4 . It is interesting t o note t h a t the m o l e c u l a r i o n c o r r e s p o n d i n g t o neamine ( a major p r o d u c t o f neomycin h y d r o l y s i s ) w a s n o t o b s e r v e d i n t h e mass s p e c t r u m o f e i t h e r t h e N - s a l i c y l i d e n e o r t h e T.M.S. d e r i v a t i v e .
I n an a t t e m p t t o a v o i d t h e n e e d f o r d e r i v a t i s a t i o n R i n e h a r t and Cook16 a p p l i e d t h e t e c h n i q u e o f F i e l d D e s o r p t i o n Mass S p e c t r o m e t r y t o neomycin a n d s u c c e s s f u l l y o b s e r v e d an i n t e n s e r e s p o n s e f o r t h e m o l e c u l a r i o n a t m / e 615(M + H ) t o g e t h e r w i t h v e r y s m a l l p e a k s a t m / e 455, 307 and 2 0 6 r e p r e s e n t i n g t h e loss o f s u g a r f r a g m e n t s .
WILLIAM F. HEYES
408
Table 2 ~13C NMR Absorptions of hexa-N-acetyl-neomycin12 Carbon atom (see Fig.1) A1 A2 A3 A4 A5 A6 D1 D2 D3 D4 D5 D6 R1 R2 R3 R4 R5 B1
B2 B3 B4 B5 B6 CH 3
co
6 ppm (from TMS)
Hex a-N- acetyl neomycin B 97.0 54.2 71.4 71.4 71.4 40.8 50.4 33.2 48.9 76.7 86 .O 74.5 109.3 74.5 77.2 82.4 62.2 98.8 51.8 70.3 68.5 74 .O 40.8 23.0(x 3) 22.9(x 3) 175.2 174.9 174.8 174.7 174.5 174.1
Hexa-N-acetyl neomycin C 96.9 54.1 71.4 71.4 71.4 40.8 50.4 33.1 48.9 76.8 86.0 74.5 110.0 73.5 75.2 81.8 62.9 97.3 54.3 71.7 72.3 71.4 40.6 23.2 22.8(x 5) 175.2 175.1 174.9(x 2) 174.6 174.1
NEOMYCIN
409
2.2 .Physical Properties of the Solid 2.21.
Hygroscopic N a t u r e
H i r t z e t a l l 7 demonstrated t h e h y g r o s c o p i c n a t u r e of neomycin s u l p h a t e u s i n g a thermogravimetric technique. I n a more r e c e n t s t u d y Russian w o r k e r s 1 8 determined t h e a d s o r p t i o n o f wate8 by neomycin s u l p h a t e a t t e m p e r a t u r e s of 23O, 9 0 & l O O z C . Table 3 g i v e s t h e r e s u l t s o b t a i n e d a t 23 C .
T a ble 3 A d s o r p t i o n o f M o i s t u r e by Neomycin S u l p h ate Humidity
Moisture adsorbed % (350 hours storage)
0, -0
0
0
10
4.15
15
5.25
25
6.90
40
10.20
60
16.70
80
38.90 2.22.
Solubility
The s o l u b i l i t i e s of e l e v e n s a l t s o f neomycfg ,30,3pme t w e n t y s i x s o l v e n t s h a v e been reported. The v a l u e s f o r t h e most commonly encountered s a l t s a r e l i s t e d i n Table 4. 2.23.
S p e c i f i c S u r f a ce Area
Using a method b a s e d on t h e f i l t r a t i o n of a i r t h r q y g h a c o m p r e s s e d l a y e r o f determined t h e v i s i b l e powder E z e r s k i i e t a 1 s p e c i f i c s u r f a c e a r e a o f neomycin s u l p h a t e t o b e 2 . 6 rn2g-l.
c
c, r(
-4
u4J
hal
m
N
m
O
A
A
N
~* I n mI n mrN
N
0
W
d
N
V
m
O V V N d c n W N
W
r-
d
d
m
Q)
In
N
d
d
A A A A
0
N
q W
0 0 0 0 A A A A
* * * 0 0 0 0
NNNN
m
N O O N 0
0 0
*
+I
a
4J
4
d d
3
ia
d
7
;
+I
0
0
N
m
z
. . 99 g
d
m
0 0 0
;Id d d
0 0
*v)
m
m o
*
InW
N O
* m o o o m
C o W O N W
.....
w d m w m
v)
ddddd
d m W O m
~
r-cnr-rl
~ c n m m ....
0
0 0
d d
m
w d
m O
Q ) dO A
u k
.rl
0
d
0 410
T a b l e 4 (Contd.. ) S o l u b i l i t y of Neomycin S a l t s ( m g / m l , c o r r e c t e d Solvent
-
Neomycin B hydrochl o r e
Petroleum e t h e r Is o o c t a n e E t h y l acetate Isoamyl acetate Acetone Methyl e t h y l ketone Diethyl ether Ethylene chloride Chloroform Carbon tetrachloride 1 , 4 dioxane Carbon d i s u l p h i d e Pyridine Form a m i d e Dimethylsulphoxide
N e omy c i n
N e omy c i n
su l p h a t e
undecylenate
0.0
0.005
0.03 0.03 0.06 0.04 0.058
0.028 0.06 0.15 C. 005
1.485* 0.005 0.06
0.07 0.0
0.075 0.14"
0.14"
0.323* 0.45"
0.923* 0.35"
A l l values
-+
for solvent blank)
0.025mg e x c e p t
oleate
Neomycin stearate
2.62 0.342 4.70" 7.36* 16.00* 5.795"
>20 15.852 6.885 14.080 9.260 6.578
1.030 7.014 2.083 1.742
7.989 0.77* >20* 7.938
11.288 3.257 >20 >20
7.328 0.217 9.463 1.046
6.485 9.40* >20*
13.038 >20 >20 1.365 10.580
4.500 3.918 >20 0.2 1 7 3.862
>20
* -+
N e omy c i n
0.05mg.
0.188 0.0
WILLIAM F . HEYES
412
2.3 .Physical P r o p e r t i e s of S o l u t i o n s 2.31.
Density
K i g e l e t a l l 8 have r e p o r t e d t h e d e n s i t y o f 6 & 1 8 % a q u e o u s neomycin s u l p h a t g s o l u t i o n s o v e r t h e t e m p e r a t u r e r a n g e 20° t o 8 0 C . The p u b l i s h e d v a l u e s a r e g i v e n i n T a b l e 5 . T a ble 5 D e n s i t i e s o f Neomycin S u l p h a t e S o l u t i o n s N e omy c i n
Density
Concen t r a t i on %
ooc
4 O°C
6 O°C
8 O°C
-
L
6
1.025
1.021
1.014
1.007
18
1.086
1.081
1.076
1.068
2.32. V i s c o s i t y T a b l e 6 shows t h e r e p o r t e d 1 8 v i s c o s i t i e s f o r 6 and 1 8 % a q u e o u s n e o m y c i n o s u l p b a t e s o l u t i o n s o v e r t h e t e m p e r a t u r e r a n g e 2 0 C-80 C . Table 6
--V i s c o s i t y o f Neomycin S u l p h a t e S o l u t i o n s Neomycin Concentration
Viscosity (cps) 2 ooc
4OoC
6 O°C
8OoC
6
1.25
0.86
0.64
0.623
18
1.99
1.30
0.95
0.74
9:
2.33.
S u r f a c e Tensiofl
Kigel e t a l l 8 h a v e r e p o r t e d t h e s u r f a c e t e n s i o n v a l u e s of 6 & 1 8 % aqueous neomycin sulphate s o l u t i o n s (Table 7 ) .
NEOMYCIN
413
Table 7 S u r f a c e T e n s i o n V a l u e s f o r Neomycin _Sulphate Solutions N e omy c i n
S u r f ace T e n s i o n (dynes/cm)
Concentration
2 ooc
4OoC
6
69.81
18
72.01
-%
6 O°C
8O°C
66.00
63.30
60.30
68.12
65.45
62.36
I
2.34.
--
-
A d s o r p t i o n by C l a y s , S o i l s & M i n e r als
The a d s o r p t i o n of a n t i b i o t i c s from a q u e o u s s o l u t i o n by c l a y s and m i n e r a l s h a s r e p o r t e d by a number of a u t h o r s . P i n c h e t concluded t h a t , f o r s t r o n g l y b a s i c a n t i b i o t i c s s u c h a s neomycin, a d s o r p t i o n by c l a y s s u c h as montmorillonite d i s t o r t e d the c r y s t a l l a t t i c e o f t h e c l a y 4.42, c o r r e s p o n d i n g t o m o n o l a y e r a d s o r p t i o n . The same a u t h o r s also s u g g e s t e d t h e bonding i n t h e monolayers t o be s t r o n g l y e l e c t r o s t a t i c . A t t e m p t s t o r e l e a s e t h e a n t i b i o t i c by the addition of b u f f e r s has en demonstrated t o be o n l y p a r t i a l l y successful". Phosphate b u f f e r s r e l e a s e d a p p r o x . 50% o f t h e a d s o r b e d a n t i b i o t i c w h e r e a s c i t r a t e , g l y c i n e and u n i v e r s a l b u f f e r s were c o m p l e t e l y i f f e c t i v e . In a recent study h a v e shown d i v a l e n t magnesium McGinity a n d H i l l " i o n s t o be more e f f i c i e n t t h a n m o n o v a l e n t sodium i o n s i n d i s p l a c i n g neomycin from t h e n e g a t i v e l y c h a r g e d c l a y s a t t a p u l g i t e and m o n t m o r i l l o n i t e .
!??'
From t h e s e s t u d i e s t h e l i m i t i n g a d s o r p t i v e c a p c i t i e s f o r t h r e e c l a y s w e r e calc u l a t e d u s i n g t h e Langmuir e q u a t i o n . Wayman e t a126 s t u d i e d t h e b i n d i n g of neomycin t o t h e f i l t r a t i o n m a t e r i a l s c e l i t e , c e l l u l o s e powder and S e i t z f i l t e r s . Neomycin w a s f o u n d t o b e a d s o r b e d on a l l t h r e e materials. Acid-washing t h e c e l l u l o s e powder f a i l e d t o d e s o r b a l l o f t h e neomycin.
414
WILLIAM F. HEYES
2 . 3 5 . A d s o r p t i o n by I o n Exchange R e s i n s During a s t u d y o f t h e physicoc h e m i c a l p r o p e r t i s o f some a m i n o g l y c o s i d e a n t i b i o t i c s Kuzyaeval' d e t e r m i n e d t h e s t a t i c and dynamic e x c h a n g e c a p a c i t i e s o f neomycin on t h e c a t i o n e x c h a n g e r e s i n KB-4P-2 ( a p h e n o x y a c e t i c acid-formaldehyde r e s i n ) u s i n g t h e r e s i n i n t h e Na form. K i l l f i n e t a127 h a v e r e p o r t e d v a l u e s f o r t h e e x c h a n g e e n t h a l p y o f neomycin € o r t h r e e i o n - e x c h a n g e r e s i n s . The v a l u e s of A H w e r e c a l c u l a t e d by a p p l i c a t i o n o f t h e Gibbs-Helmholtz e q u a t i o n ; t h e p u b l i s h e d r e s u l t s are t a b u l a t e d below:-
T ab le 8 Some Exchange E n t h a l p i e s f o r Neomycin Ion exchange resin
+ form
Type
AH c a l e q u i-1 v
.
methacrylic acidd iv i n y 1ben z e n e
-40
KMDM6 ,Na+form
methacrylic acidhexame t h y l e n e d i m e t h y 1 a c r y 1a m i d e
+34 0
KB4P2 ,Na+form
phenoxyacetic acidformaldehyde
+5 7 0
KFU,Na
Ig8a f u r t h e r p u b l i c a t i o n reported investigations i n t o t h e v a r i a t i o n of the S e l e c t i v i t y Coefficient ( K ) w i t h t h e amount o f neomycin a d s o r b e d f o r f o u r t e e n d i f f e r e n t ion-exchange r e s i n s . In a l l cases t h e s e l e c t i v i t y c o e f f i c i e n t i n c r e a s e d w i t h t h e amount o f a d s o r b e d neomycin ( e x p r e s s e d as t h e % surface-coverage o f t h e i o n exchange r e s i n ) , t h o u g h d i f f e r e n t t y p e s of i o n e x c h a n g e r s r e s u l t e d i n d i f f e r e n t r e s p o n s e s . T h e d e g r e e o f crossl i n k i n g of t h e i o n e x c h a n g e r e s i n was a l s o r e p o r t e d t o a f f e c t e d t h e v a l u e of t h e s e l e c t i v i t y coefficient. The a u t h o r s c o n c l u d e d t h a t p o l y c o n d e n s a t i o n - t y p e i o n exchange r e s i n s a d s o r b K i l ' f i n and Samsonov
NEOMYCIN
415
neomycin more s e l e c t i v e l y t h a n t h e p o l y m e r i s a t i o n t y p e r e s i n s and t h a t v a r i a t i o n of t h e components of e i t h e r t y p e of r e s i n had l i t t l e e f f e c t on t h e a d s o r p t i o n of neomycin. Klyueva and G e l ’ p e r i n 2 ’ have compared t h e e q u i l i b r i u m d i s t r i b u t i o n c u r v e s f o r t h e a d s o r p t i o n o f neomycin on i o n - e x c h a n g e r e s i n s from b o t h p u r e s o l u t i o n s and t y p i c a l f e r m e n t a t i o n broths. 3.
S a l t s , Derivatives 3.1.
&
Complexes
Salts
Many a t t e m p t s t o a l t e r t h e p h y s i c a l p r o p e r t i e s o f neomycin by t h e f o r m a t i o n o f v a r i o u s s a l t s have b e e n d e s c r i b e d . Thus t h e neomycin s a l t s of t h e h i g h e r f a t t y a c i d s , s u c h a s t h e s t e a r a t e , p a l m i t a t e and m y r i s t a t e 3 0 r 31 were p r e p a r e d and b e i n g w a t e r - i n s o l u b l e w e r e f o r m u l a t e d i n ointment bases. Similarly, t h e undecylenate s a l t h a s been re a r e d and p r o c e s s e s f o r i t s p r o d u c t i o n p a t e n t e d 3 5 39, ~ 3 4 * The u n d e c y l e n a t e and c a p r y l a t e s a l t s h a v e been d e s c r i b e d as b e i n p a r t i c u l a r l y s u i t a b l e as a n t i m i t o t i c compounds 85
.
V a r i o u s c a r b o x y l i c a c i d s a l t s have a l s o gal lard^^^ p r o d u c e d t h e m a l e a t e been r e p o r t e d . s a l t o f neomycin w h i c h , i t was c l a i m e d , improved t h e a q u e o u s s t a b i l i t y of t h e a n t i b i o t i c . A p r a c t i c a l l y t a s t e l e s s compound t h e c i t r a t e s a l t , h a s b e e n d e s c r i b e d by S z y s ~ k a ~ Neomycin ~ . mandelate h a s been claimed t o be p a r t i c u l a r 1 u s e f u l i n t h e t r e a t m e n t of u r o g e n i t a l i n f e c t i o n s s g w h i l e t h e d i hydroxy-d i n a p h t h l m e t h a n e - d i c a r b o x y l a t e 40 and t h e pamoate s a l t s 4 1 , g 7 1 6 8 h a v e a l o w i n t e s t i n a l abs o r p t i o n and a r e t h u s e f f e c t i v e t r e a t m e n t s f o r intestinal infections. F i s h e r and H a l l r e p o r t e d t h e p r o p i o n a t e s a l t t o be u n s u i t a b l e f o r u s e i n o p h t h a l m i c preparation^^^. O t h e r s a l t s d e s c r i b e d i n t h e l i t e r a t u r e a r e neom c i n g l u c u r o n a t e 4 2 , s u c c i ~ t, h a l a t e ~ ~ a n d n a t e 4 3 I 4 4 , l a c t a t e 42 a ~ c o r b a t e ~ h t h e s u l p h o s ~ c c i n a t e4~8 ~which r has the property of improved s k i n p e n e t r a t i o n .
416
WILLIAM F. HEYES
Amongst t h e o r g a n i c s u l p h o a c i d s u s e d
t o p r e p a r e neomycin s a l t s , t h e p - t o l u e n e s u l p h o n a t e h a s been r e p o r t e d and i n c o r p o r a t e d i n an
a e r o s o l s p r a y f o r m u l a t i o n 4 9 . S a l t s o f neomycin w i t h h a l o g e n s u b s t i t u t e d 8 - h y d r o x y q u i n o l i n e 5s u l p h o n i c a c i d s h a v e been d e s c r i b e d a s p o s s e s s i n g l o w t o x i c i t y , a n t i s e p t i c and a n t i a m e b i c b e s i d e s a n t i m i c r o b i a l pro erties50f51. Stankovics e t a 1 5 2 and V e ~ i a n ap r~e ~c i p i t a t e d a complex s a l t of neomycin, by m i x i n g a q u e o u s s o l u t i o n s of neomycin s u l p h a t e and sodium l a u r y l s u l p h a t e , which had improved a c t i v i t y a g a i n s t Staphylocaccub a u k e u d . I n a more r e c e n t i n v e s t i g a t i o n o f t h i s r e a c t i o n , found t h a t t h e p r e c i p i t a t e d Leucuta e t complex d i s s o l v e d on a d d i t i o n o f e x c e s s sodium I.R. s t u d i e s of t h e complex lauryl sulphate. have i n d i c a t e d t h a t amide g r o u p s , c o u p l i n g rea c t i o n s and H-bonding a r e i n v o l v e d i n t h e format i o n o f t h e compound. M i c h e l e and V a l e t t e h a v e rep o r t e d an enhanced a n t i b i o t i c a c t i v i t y and a reduced t o x i c i t y f o r t h e e u c a l y p t 0 1 ~ u l p h o n a t e ~ ~ . P r e p a r a t i o n of t h e d o d e c l b e n z e n e - s u l p h o n a t e 5 5 and t h e cyclohexylsulphonatex6has a l s o been d e s c r i b e d . The p a n t o t h e n a t e s a l t of neomycin , f i r s t d e s c r i b e d by K e l l e r e t a 1 5 7 , a l s o e x h i b i t s t h e p r o p e r t y of a lower t o x i c i t y t h a n t h e p a r e n t a n t i b i o t i c . A f u r t h e r p a p e r by t h e same a u t h o r s 5 8 a t t r i b u t e d t h e lower t o x i c i t y o f t h e p a n t o t h e n a t e t o be due t o a r e d u c t i o n i n t h e c a l c i u m - b i n d i n g a b i l i t y of t h e a n t i b i o t i c when i n t h e form of t h e p a n t o t h e n a t e s a l t . A s i m i l a r e f f e c t h a s been n o t e d by W e i t n a u e r e t a159 w i t h a n e q u i m o l a r m i x t u r e of neomycin and c a l c i u m g l u c o n a t e . Numerous p r o cedures f o r the preparation o t e pantothenate ~ ~ s a l t have been p a t e n t e d 6 0 , 6 1 , ‘ 2 r k 3 . A b b ~ urep o r t e d t h e p r e p a r a t i o n of a complex s a l t of neomycin w i t h a m i x t u r e of g l u t a m i c and p a n t o t h e n i c a c i d s and d e s c r i b e d t h e compound a s p o s s e s s i n g b e t t e r o r g a n o l e p t i c p r o p e r t i e s t h a n o t h e r neomycin salts. S a l t s w i t h t h e amino a c i d s N-methyls t e a r o y l g l y c i n e 6 5 and l u t a m i c a c i d 6 6 , and t h e v i t a m i n s a s c o r b i c a c i d 2 3 and n i c o t i n i c a c i d 6 3 have a l s o been e v a l u a t e d .
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C h l o r o p h e n o l s a r e of a s u f f i c i e n t l y a c i d i c n a t u r e t o be a b l e t o form s a l t s w i t h neomycin and h a v e been r e p o r t e d t o p o s s e s s h t h a n t i b a c t e r i a l and m y c o c i d a l proper tie^^^ ,7 0 r 7p. Shaw70 h a s d e s c r i b e d t h e t o p i c a l u s e of s u c h a compound, neomycin h e x a k i s p e n t a c h l o r o p h e n a t e , i n t h e t r e a t m e n t o f d e n t a l r o o t i n f e c t i o n and p e r i o dontic cavities. A s a l t formed by r e a c t i n g neomycin w i t h p-amino b e n z e n e s u l h o a c e t a m i d e was d e s c r i b e d by t w o g r o u p s of w o r k e r s T 2 I 7 3 . The s a l t combined t h e c h e m o t h e r a p e u t i c p r o p e r t i e s of t h e components. A n o t h e r u n u s u a l s a l t of neomycin d e s c r i b e d i n t h e l i t e r a t u r e i s t h a t w i t h m- u l p h o n y l b e n z a l d e h y d e i s o n i c o t i n o y l h y d r a z o n e78’7’. The compound i s rep u t e d t o be l e s s t o x i c t h a n neomycin and t o be more a c t i v e a g a i n s t t u b e r c u l e b a c i l l i t h a n t h e individual constituents.
S a l t s of neomycin w i t h t h e i n o r g a n i c The s u l p h a t e s a l t a c i d s have a l s o b e e n d e s c r i b e d . i s t h e u s u a l c o m m e r c i a l form i n u s e t o d a y b u t neomycin b o r a t e h a s been u s e d i n o p h t h a l m i c p r e p a r a t ions46. Not a l l neomycin s a l t s , however, p o s s e s s a d v a n t a g e s s u c h as a r e d u c e d t o x i c i t y . I n f a c t , t h e orotic acid (1,2,3,6-tetrahydro-2 ,6d i o x o - 4 - p y r i m i d i n e c a r b o x y l i c a c i d ) s a l t w a s rep o r t e d t o h a v e a g r e a t e r t o x i c i t y t h a n neomycin i t ~ e l f ~Some ~ u ~ n c~e r ~ t a i .n t y of t h i s f a c t i s a p p a r e n t a s o t h e r a u t h o r s have r e p o r t e d t h e two compounds t o b e o f a s i m i l a r t o x i c i t y 7 6 . The s a l t of neomycin w i t h u s n i c a c i d ( a n a n t i b a c t e r i a l s u b s t a n c e f o u n d i n l i c h e n s ) h a s been r e p ~ r t e d ~ ~ t o h a v e l e s s a n t i b a c t e r i a l a c t i v i t y t h a n t h e neomycin used i n t h e p r e p a r a t i o n of t h e s a l t . 3.2. Derivatives The neomycin m o l e c u l e c o n t a i n s b o t h f r e e amino and f r e e .hydroxy g r o u p s . Many w o r k e r s have e x p l o i t e d t h e p o s s i b i l i t y o f c h e m i c a l d e rivatisation a t these positions in attempts t o r e d u c e t h e t o x i c i t y of t h e p a r e n t a n t i b i o t i c . S u b s t i t u t i o n of methane s u l p h o n a t e g r o u p s a t t h e amino n i t r o g e n h a s been r e p o r t e d by U m e z a w a e t a183184 and by B o i s s i e r e t a185. Both g r o u p s o f w o r k e r s d e s c r i b e d t h e d e r i v a t i v e t o b e less t o x i c
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than t h e p a r e n t a n t i b i o t i c . Boissier claimed t h a t t h e ' i n v i t r o ' and ' i n v i v o ' a n t i b a c t e r i a l a c t i v i t y o f t h e neomycin i s p r e s e r v e d f o l l o w i n g derivatisation. However, Umezawa, w o r k i n g w i t h f r a d i o m y c i n , d e s c r i b e d t h e N-methyl s u l p h o n a t e d e r i v a t i v e a s having h a l f t h e a c t i v i t y of f r a d i o mycin when r e a s u r e d a g a i n s t gram-pos i t i v e b a c t e r i a and o n l y one t e n t h t h e a c t i v i t y when measured again s t gram-negative b a c t e r i a . Russian workers89 have r e p o r t e d t h e r e d u c t i o n i n a n t i b a c t e r i a l a c t i v i t y t o b e p r o p o r t i o n a l t o t h e d e g r e e o f Ns u b s t i t u t i o n . Alternative procedures f o r t h e p r e p a r a t i o n o f N-methyl s u l p h o n y l neomycin h a v e been r e p o r t e d by a number o f a u t h o r s 8 6 1 8 7 1 8 8 and t h e pharmacology o f t h e compound h a s been e x t e n s i v e l y i n v e s t i g a t e d by D i Marco and B e r t a z z o i g o . T h e p r e p a r a t i o n of t h e f o l l o w i n g s u l p h o d e r i v a t i v e s h a s a l s o been d e s c r i b e d : N-me t hy l s u l p h i no n e omyc i n
I
N - p h e n y l s u l p h o n y l neomycin93 N- a c e t amidop hen y Is u l phony 1 neomyc i n
N-p-aminophenylsulphonyl neomycing3 N- t r i c h lorome t h y l t h i o neomycin9 N - e t h y l t h i o c a r b o n y l neomycing3 and neomycin N - s u l p h o n a t e g 4 Vanderhaeghe8O h a s s t u d i e d t h e a l k y l a t i o n of neomycin. A r e d u c t i o n i n t o x i c i t y was n o t e d f o l l o w i n g a l k y l a t i o n b u t t h i s w a s c o u p l e d w i t h a c o m p l e t e loss o f a n t i b a c t e r i a l properties. The r e s u l t i n g compound, however, w a s found t o p o s s e s s good h y p o c h o l e s t e r e m i c a c t i v i t y . The e f f e c t of N - a l k y l a t i o n , 0 - a l k y l a t i o n , Na c y l a t i o n and O - a c y l a t i o n h a s been i n v e s t i g a t e d by Magyar e t a181. These w o r k e r s r e p o r t e d t h e l o s s o f b i o l o g i c a l a c t i v i t y t o be p r o p o r t i o n a l t o t h e number o f g r o u p s s u b s t i t u t e d . F u r t h e r i n v e s t i g a t i o n s by t h e s e w o r k e r s d e m o n s t r a t e d t h a t conv e r s i o n o f amino g r o u p s i n t o q u a t e r n a r y ammonium g r o u p s r e s u l t e d i n t h e p r o d u c t i o n of compounds having a mild t u b e r c u l o s t a t i c e f f e c t . Penasse e t a182 have d e s c r i b e d an a l t e r n a t i v e p r o c e d u r e f o r t h e p r e p a r a t i o n of N-alkyl d e r i v a t i v e s .
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3 . 3 . Complexes
The f o r m a t i o n o f a zinc-neomycin complex h a s been r e p o r t e d by Chornock95 and by K e l l e r and C o s a r g 6 . E l e c t r o p h o r e s i s w a s u s e d t o d e m o n s t r a t e t h e f o r m a t i o n o f a complex which was d e s c r i b e d as p o s s e s s i n g a s i m i l a r b i o l o g i c a l a c t i v i t y t o neomycin b u t a d e c r e a s e d t o x i c i t y . More r e c e n t l y Agrawal, H a r m a l k e r and V i j a y a w a r g i y a g 7 have d e s c r i b e d t h e f o r m a t i o n o f a copper-neomycin complex. With a s t o i c h i o m e t r y o f 1:1, t h e b l u e c o l o u r e d complex h a s been made t h e b a s i s o f a s p e c t r o p h o t o m e t r i c a s s a y method f o r neomycin ( S e e S e c t i o n 6 . 2 6 ) . The c o m p l e x a t i o n o f neomycin w i t h a number of b i o c h e m i c a l l y i m p o r t a n t compounds h a s been r e p o r t e d . I n t e r a c t i o n of t h e a n t i b i o t i c with h e p a r i n w a s f i r s t i n v e s t i g a t e d by Higginbotham and D o u g h e r t y 9 8 . U s i n g a s p e c t r o p h o t o m e t r i c p r o c e d u r e , which measured t h e amount o f dye r e l e a s e d f r o m a t o l u i d i n e b l u e - h e p a r i n complex on a d d i t i o n of neomycin s o l u t i o n , t h e s e a u t h o r s s t u d i e d a number of a n t i b i o t i c s and t h e i r r e a c t i o r . w i t h heparin. G u b e r n i e v a and S i l a e v g 9 employed elect r o p h o r e s i s t o i n v e s t i g a t e t h e n a t u r e of t h e n e o m y c i n - h e p a r i n complex and s u g g e s t e d t h e compound may b e more t h a n a s i m p l e c a t i o n - a n i o n i n t e r a c t i o n . The p o s s i b i l i t y o f a d d i t i o n a l H-bonding f o l l o w i n g t h e i n i t i a l i o n i c i n t e r a c t i o n was p o s t u l a t e d . A more d e t a i l e d s t u d y o f t h e c o m p l e x a t i o n o f n e o mycin w i t h h e p a r i n , DNA,RNA and p o l y h l o r e t i n p h o s p h a t e h a s been d e s c r i b e d by HeinyOO. The c o m p l e x e s w e r e p r e p a r e d by m i x i n g a q u e o u s s o l u t i o n s of neomycin s u l p h a t e and t h e c o m p l e x i n g a g e n t u n d e r i n v e s t i g a t i o n . The p r e c i p i t a t e which formed r e d i s s o l v e d on a d d i t i o n o f sodium h y d r o x i d e s o l u t i o n o r aqueous s o l u t i o n s of s i l v e r n i t r a t e , manganese s u l p h a t e and c o b a l t c h l o r i d e . S u b j e c t i o n o f t h e p r e c i p i t a t e d complex t o an a g a r d i f f u s i o n e x p e r i m e n t d e m o n s t r a t e d t h e compound t o b e b i o logically active. U s i n g an a g a r o s e g e l s y s t e m Kunin and Tupasi.101 o b s e r v e d t h e f o r m a t i o n o f a p r e c i p i t a t i o n band between z o n e s of d e x t r a n s u l p h a t e and neomycin. The a u t h o r s a t t r i b u t e d t h e p r e c i p i t a t i o n t o be a r e s u l t o f complex f o r m a t i o n
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and n o t t h e r e s u l t of an a n t i g e n - a n t i b o d y i n t e r a c t i o n which t h e s y s t e m i s u s u a l l y employed t o detect. H a r r i s l o 2 h a s s t u d i e d t h e complexat i o n of neomycin w i t h p e c t i n and d e m o n s t r a t e d t h e i n h i b i t i o n of complex f o r m a t i o n i n t h e p r e s e n c e of an e l e c t r o l y t e . P o t e n t i o m e t r i c measurements i n d i c a t e t h e mechanism o f t h e r e a c t i o n t o be a cation-anion i n t e r a c t i o n . H-bonding between t h e hydroxy g r o u p s o f p e c t i n and s u g a r m o i e t i e s o f neomycin h a s been s u g g e s t e d and would f u r t h e r s t a b i l i s e t h e compound.
The c o m p l e x a t i o n of neomycin w i t h a n i o n i c d y e s s u c h a s a m a r a n t h ( F . D . & C . Red No.2) i s w e l l known100,102 and h a s been made t h e b a s i s of a q u a n t i t a t i v e a s s a y f o r n e o m y ~ i n ~ ~ These ~ 1 ~ 5 . complexes a r e a g a i n of t h e c a t i o n / a n i o n t y p e and t h e i r f o r m a t i o n i s d e p e n d a n t on t h e i o n i c s t r e n g t h of t h e s o l u t i o n . I n o r g a n i c c o n d e n s e d p h o s p h a t e s have been r e p o r t e d t o complex w i t h neomycin and i n a s t u d y of t h e s e compounds I S i n g h l o 3 d e m o n s t r a t e d t h e s t r e n g t h o f t h e complex t o be d e p e n d a n t on t h e d e g r e e of p o l y m e r i s a t i o n of t h e p h o s p h a t e . By i n c r e a s i n g t h e number of p h o s p h a t e u n i t s i n t h e polymer o v e r t h e r a n g e 1 t o 1 6 u n i t s an i n c r e a s i n g s t r e n g t h of c o m p l e x a t i o n w a s o b s e r v e d . Beyond t h i s u p p e r l i m i t , however, t h e s t r e n g t h of t h e complex remained c o n s t a n t . Relative complex-strengths w e r e a s s e s s e d by t i t r i m e t r y w i t h p o t a s s i u m c h l o r i d e solution. A number of w o r k e r s h a v e u t i l i s e d e l e c t r o p h o r e s i s t o e s t a b l i s h t h e f o r m a t i o n of a complex between neom c i n and t h e r o t e i n s i n b l o o d Serum and plasma104 ,Yo511 0 6 1 1 0 7 , ,881 1 0 9 , 1 1 0 , 1 1 1 . However, t h e n a t u r e of t h e complex i s s t i l l unknown. Geitman h a s e x t e n s i v e l y s t u d i e d t h e phenomena of p r o t e i n - b i n d i n g o f a n t i b i o t i c s l l 1 t 1 l 2 . I n a p a p e r p u b l i s h e d j o i n t l y w i t h Kivman1l2, Geitman r e p o r t e d t h a t neomycin d i d n o t b i n d t o any of t h e p r o t e i n f r a c t i o n s when added t o serum b u t bound t o t h e i s o l a t e d albumin and g l o b u l i n f r a c t i o n s . An e a r l i e r p a p e r l l l d e s c r i b e d t h e g l o b u l i n - n e o m y c i n complex t o b e o f g r e a t e r s t a b i l -
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i t y t h a n t h e albumin-neomycin complex and e s t a b l i s h e d lmg o f serum p r o t e i n t o b i n d 0 . 0 6 u n i t s o f neomycin
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4.
S y n t h e s i s and P r o d u c t i o n 4.1.
Commercial B i o s y n t h e sis
Waksman e t a1286, i n 1 9 4 9 , f i r s t rep o r t e d t h e p r o d u c t i o n of neomycin by f e r m e n t a t i o n of a c u l t u r e o f S . d h a d i a ~ ( 3 5 3 5 ) .The same o r g a n i s m s u b s e q u e n t l y formed t h e b a s i s o f an i n d u s t r i a l f e r m e n t a t i o n rocess f o r t h e b i o s y n t h e s i s o f neomycin28712i8. I s o l a t i o n o f t h e a n t i b i o t i c from t h e f e r m e n t a t i o n media i s a c c o m p l i s h e d b y u s e of i o n - e x c h a n e r e s i n s , s u c h a s Amberlite I R C 50225 1 9 5 0 , 2 5 1 .
F o l l o w i n g t h e o r i g i n a l r e p o r t by Waksman, a number o f o t h e r a u t h o r s have d e s c r i b e d S . Q a a d i a e t o y i e l d a n t i b i o t i c s on f e r m e n t a t i o n . The r e s u l t i n g s u b s t a n c e s w e r e named s t r e p t o t h r i c i n B 1 2 8 9 , m y c e r i n 2 9 0 and c 0 l i m y c i n 2 9 1 ~b u t h a v e s i n c e b e e n shown t o be i d e n t i c a l t o t h e neomycin complex. 4.2.
S y n t h e s i s o f R a d i o - L a b e l l e d Neomycin
The b i o s y n t h e t i c p r e p a r a t i o n o f l 4 C l a b e l l e d neomycin w a s f i r s t d e s c r i b e d by Sebek267 who s t u d i e d a number o f s u b s t r a t e s f o r t h i s p u r p o s e b u t c o n c l u d e d 14C'labelled glucose was t h e most s a t i s f a c t o r y . A l t h o u g h 6 8 % o f t h e r a d i o n u c l i d e w a s l o s t as r e s p i r a t o r y I 4 C O , 1 9 % o f t h e t o t a l a c t i v i t y added p r i o r t o f e r m e n $ a t i o n w a s i n c o r p o r a t e d i n t o t h e neomycin s u l p h a t e . T h i s method o f p r e p a r i n g 1 4 C - l a b e l l e d neomycin h a s b e e n e x t e n s i v e l y u s e d t o s t u d y t h e mechanism o f neomycin b i o s y n t h e s i s . Stroshane13 has described t h e s y n t h e s i s o f 13C-neomycin and 15N-neomycin, a g a i n a s p a r t o f an i n v e s t i g a t i o n o f neomycin b i o s n t h e s i s . 13C-glucose s e r v e d a s p r e c u r s o r f o r y3C-neomycin and g l u c o s a m i n e l a b e l l e d w i t h I 5 N w a s u t i l i s e d f o r t h e p r e p a r a t i o n o f 15Nneomycin. A p r o c e d u r e f o r 1abe l l i n g neomycin w i t h t r i t i u m h a s been d e s c r i b e d by J a c k s o n e t
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a t 2 9 2 and i n v o l v e s p a s s i n g an e l e c t r i c d i s c h a r g e across a v e s s e l c o n t a i n i n g t r i t i u m and neomycin sulphate. L a b i l e t r i t i u m was removed by w a s h i n g w i t h a p o l a r s o l v e n t and t h e t r i t i u m - l a b e l l e d neomycin p u r i f i e d by m u l t i p l e r e c r y s t a l l i s a t i o n . 5.
S t a b i l i t y and D e g r a d a t i o n 5.1.
Hydrolytic Degradation
The d e g r a d a t i o n of neomycin h a s b e e n e G t e n s i v e l y s t u d i e d by R i n e h a r t l a s a means o f e s t a b l i s h i n g t h e s t r u c t u r e s o f t h e neomycin compon e n t s . F i g . 5 i l l u s t r a t e s t h e r o u t e by which comp l e t e d e g r a d a t i o n of t h e a n t i b i o t i c w a s a c h i e v e d . Extremely vigorous c o n d i t i o n s are n e c e s s a r y f o r t h e h y d r o l y s i s o f n e m i n e a s t h i s compound i s r e s i s t a n t t o acid-hydrolysis. However, u n d e r t h e s e c o n d i t i o n s t h e c h e m i c a l e n t i t i e s neosamine C ( f r o m n e a m i n e ) and r i b o s e are n o t o b s e r v e d b e c a u s e v i g o r o u s h y d r o l y s i s i m m e d i a t e l y decomposes t h e compounds f u r t h e r . By d e r i v a t i s i n g t h e amino g r o u p s o f t h e neamine and n e o b i o s a m i n i d e m o l e c u l e s R i n e h a r t w a s a b l e t o lower t h e r e s i s t a n c e of t h e s e compounds t o h y d r o l y s i s and t h u s u s e mild h y d r o l y t i c c o n d i t i o n s t o s u c c e s s f u l l y i s o l a t e neosamine C and r i b o s e : (CHJCO)
a ) neamine
CH30H
0
*5, o C
t e t r a N - a c e t y l neamine
-
J
3N HC1
lOhr @ 9 5 O C
deoxystreptamine
+
neosamine
PhCOCl
blmethyl neob i o s a m i n i d e
0.1N
ribose
N aOH
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methyl N,N'-dibenzoyl neob i o s a m i n i d e 1.6N
HC1
d4 CH OC H O(OH)3 3 5 6
Rus s i a n w o r k e r s attempted t o prep a r e t h e d e g r a d a t i o n p r o d u c t s i n a p u r e f o r m by c a r r y i n g o u t t h e h y d r o l y s i s i n t h e p r e s e n c e of an i o n e x c h a n g e r e s i n which a d s o r b e d t h e i n t e r m e d i a t e
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n eomy c i n I
F i g u r e 5.
H y d r o l y t i c d e g r a d a t i o n of neomycin C
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hydrolysis products,thereby preventing f u r t h e r dec o m p o s i t i o n . The d e g r a d a t i o n p r o d u c t s w e r e rel e a s e d from t h e r e s i n by g r a d i e n t - e l u t i o n . 5.2.
S t a b i l i t y o f Bulk M a t e r i g
J a p a n e s e w o r k e r s l5 h a v e d e s c r i b e d t h e s t a b i l i t y of b u l k f r a d i o m y c i n (neomycin B l s u l p h a t e which was shown t o h a v e r e t a i n e d 9 9 % o f i t s microb i o l o g i c a l p o t e n c y a f t e r s t o r a g e f o r 2 4 months. Neomycin s u l p h a t e powder h a s been r e o r t e d t o b e s t a b l e f o r a t l e a s t 3 y e a r s a t 2OoC 5 9 8 ,305. Neomycin s u l p h a t e may a l s o b e h e a t e d a t llO°C f o r 10 hours, during dry-heat sterilisat i o n , w i t h o u t l o s s o f p o t e n c y , t h o u g h some d e g r e e of yellowing i s apparent298. 5.3.
S t a b i l i t y i n Aqueous S o l u t i o n
Swart e t a 1 h a v e d e m o n s t r a t e d t h e s t a b i l i t y of neomycin h y d r o c h l o r i d e i n a q u e o u s Further ins o l u t i o n o v e r t h e pH r a n g e 2-9293. v e s t i g a t i o n s by Simone and P o p i n o 2 9 8 c o n f i r m e d t h e a q u e o u s s t a b i l i t y a t 23OC b u t a t 45OC p o t e n c y l o s s e s o f u p t o 9 4 % w e r e n o t e d o v e r a p e r i o d of 2 y e a r s w i t h s o l u t i o n s i n t h e pH r a n g e 4-8. Leach e t a 1 2 9 4 d e s c r i b e d a p u r i f i e d neomycin t o be s t a b l e t o t h e a c t i o n o f a l k a l i b u t Refluxing t h e a n t i b i o t i c w i t h barium not t o acids. h y d r o x i d e f o r a p e r i o d of e i g h t e e n h o u r s f a i l e d t o show a l o s s i n m i c r o b i o l o g i c a l p o t e n c y . Japanese w o r k e r s have d e s c r i b e d a stable a q u e o u s s o l u t i o n of neomycin w i t h t h e i n c o r p o r a t i o n o f a b o r a t e b u f f e r (pH 6 ) and E . D . T . A . 2 9 5 The p r e s e n c e of 1-10% o f g l y c e r o l , p r o p y l e n e g l y c o l o r m a n n i t o l h a s b e e n c l a i m e d t o improve t h e s o l u t i o n a p p e a r a n c e by p r e v e n t i n g d i s c o l ~ r a t i o n ~ The ~~. p r e s e n c e of p o l y o l s a l s o p r e v e n t e d a d e c r e a s e i n pH v a l u e o f t h e s o l u t i o n . D i s c o l o r a t i o n may a l s o b e p r e v e n t e d by a d d i t i o n of 0.1% sodium m e t a b i s u l p h i t e a t a s o l u t i o n pH of 6 . 6 t o 6 . 8 2 9 7 .
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S t a b i l i t y i n Pharmaceutical Formulations
Numerous r e p o r t s c o n c e r n i n g t h e s t a b i l i t y of neomycin i n v a r i o u s d o s a e forms have been p u b l i s h e d . Simone and Popino j 9 8 s t u d i e d t h e s t a b i l i t y o f neomycin i n l i q u i d dosage forms s u c h a s n a s a l d r o p s , mouth washes and t i n c t u r e s . The a n t i b i o t i c w a s s t a b l e i n a l l t h e formulations t e s t e d , e x c e p t D o b e l l s s o l u t i o n ( a mouth w a s h ) , f o r a t l e a s t 6 months a t 2 0 O C . Some f o r m u l a t i o n s were s t a b l e f o r considerably longer. Heyd2” h a s s t u d i e d t h e s t a b i l i t y o f neomycin i n aqueous g e l s and f o r m u l a t e d a s a t i s f a c t o r y p r o d u c t by a d s o r b i n g t h e a n t i b i o t i c on an i o n exchange r e s i n , Amberlite IRP-69M, p r i o r t o incorporation i n the gel. R e c o n s t i t u t e d aqueous s u s p e n s i o n s o f neomycin s u l p h a t e , c o n t a i n i n g t r a g a c a n t h and s u g a r have been shown t o b e s t a b l e f o r 10 d a y s when s t o r e d a t 4OC b u t some loss of p o t e n c y w a s o b s e r v e d when t h e s u s p e n s i o n was exposed t o d a y l i g h t 3 ” . Non-aqueous s u s p e n s i o n s c o n t a i n i n g p e a n u t o i l and l a n o l i n have been r e p o r t e d 2 9 8 which are s t a b l e f o r 1 year a t 200C. Simone and pop in^^'^ have c o n s i d e r e d t h e s t a b i l i t y of neomycin i n b o t h h y d r o p h o b i c and hydrophilic ointment bases. No l o s s of p o t e n c y o v e r a p e r i o d of 1 y e a r a t 2OoC w a s r e p o r t e d f o r formulations containing carboxymethylcellulose, polyethylene glycol(P.E.G.) o r white-soft paraffin. However, f o r m u l a t i o n s c o n t a i n i n g h y d r o u s A l l materlanolin w e r e reported t o be unstable. i a l s u s e d i n t h e f o r m u l a t i o n s were o b t a i n e d from U.S. sources. C o a t e s e t a1301 i n v e s t i g a t e d t h e u s e o f P . E . G . from B r i t i s h s o u r c e s and d e s c r i b e d neomycin a s b e i n g i n c o m p a t i b l e w i t h t h e m a t e r i a l s tested. S o l i d d o s a g e forms of neomycin as t a b l e t s and t r o c h e s have been p r e p a r e d 2 9 8 and a r e r e p o r t e d t o b e s t a b l e a t 2OoC and a t 56OC. I n t h e a r e a of animal h e a l t h n u t r i t i o n a feed-premix c o n t a i n i n g neomycin and oxyt e t r a c y c l i n e h a s been d e s c r i b e d . With neomycin
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a t a l e v e l of 20g/lb t h e p r o d u c t is s t a b l e f o r 1 y e a r a t 20°C, though an 8 % loss o f p o t e n c y was obs e r v e d on s t o r a g e f o r 6 months a t 380C305. A medi c a t e d d r i n k i n g - w a t e r c o n t a i n i n g 100 ppm o f neomycin and p r e p a r e d w i t h t a p - w a t e r , showed n o s i g n i f i c a n t l o s s of p o t e n c y a f t e r 48 h o u r s s t o r a g e a t 38OC i n e i t h e r g l a s s c o n t a i n e r s o r g a l v a n i s e d troughs305. 5 . 5 . C o m p a t i b i l i t y w i t h E x c i p i e n t Materials The r e a c t i o n of neomycin w i t h many compounds h a s been d e s c r i b e d i n S e c t i o n 3 , h e n c e numerous r e p o r t s o f neomycin i n c o m p a t i b i l i t y may b e e x p e c t e d . D a l e and Rundman304 h a v e e x t e n s i v e l y reviewed t h e c o m p a t i b i l i t y o f neomycin w i t h s u b s t a n c e s t h a t may b e e n c o u n t e r e d by t h e f o r m u l a t i o n pharmac i s t . K u d a l k e r e t a1303 have d e s c r i b e d t h e incomp a t i b i l i t y o f t h e a n t i b i o t i c w i t h r a n c i d o i l s , and the i n c o m p a t i b i l i t y with b e n t o n i t e , a montomorillo n i t e c l a y , h a s been r e p o r t e d by D a n t i and Guth306. The i n c o m p a t i b i l i t y w i t h l a c t o s e , c a u s i n g a d i s c o l o r a t i o n o f t h e m i x t u r e h a s b e e n s t u d i e d by Hammouda and Sa1akawy3O7. The amount of browning produced w a s shown t o be d e p e n d a n t on t h e i n i t i a l pH of t h e s o l u t i o n . The r a t e of d i s c o l o r a t i o n of t h e l a c t o s e / n e o m y c i n powder w a s d i r e c t l y r e l a t e d t o t h e t e m p e r a t u r e o f s t o r a g e and t h e r e l a t i v e h u m i d i t y of t h e a t m o s p h e r e . D i s c o l o r a t i o n w a s o v e r come by a d d i t i o n of sodium b i s u l p h i t e . F l o r e s t a n o e t a l 308 compared t h e rel e a s e of neomycin from P . E . G . d i e s t e r o i n t m e n t b a s e s and g r e a s e - t y p e b a s e s and c o n c l u d e d t h e former t o b e p r e f e r r e d though Coates e t a1301 h a v e d e s c r i b e d P . E . G . from B r i t i s h s o u r c e s t o b e incomp a t i b l e w i t h neomycin. 5.6.
Compatibility with Other Actives
Neomycin forms an i n s o l u b l e complex when added t o aqueous s o l u t i o n s of c o r t i c o s t e r o i d phosp h a t e s . T o overcome t h i s i n c o m p a t i b i l i t y , McGinty and Brown304 i n c o r p o r a t e d d i s o d i u m h y d r o g e n phosp h a t e i n t h e o p t h a l m i c f o r m u l a t i o n . The mechanism by which t h e c o m p l e x a t i o n i s p r e v e n t e d h a s n o t y e t been f u l l y d e t e r m i n e d .
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6 . Methods of A n a l y s i s 6.1.
I d e n t i f i c a t i on
T a b l e 9 l i s t s a number of c o l o r i m e t r i c t e s t s which h a v e b e e n u s e d a s i d e n t i t y t e s t s f o r neomycin. N o one t e s t , h o w e v e r , h a s been demons t r a t e d t o b e s p e c i f i c f o r neomycin and i t i s t h u s a l s o a d v i s a b l e t o e s t a b l i s h t h e a b s e n c e of o t h e r c h e m i c a l l y s i m i l a r a n t i b i o t i c s by s u i t a b l e means. Table 9 Colorimetric Identity T e s t s f o r N eomy c i n Test
G l u cos amine Molisch Ninhydrin Fur f u r a 1 Ph lorog l u c i n o1
Chemical g r o u p ing u t i l i s e d i n re a c t i o n
Colour obtained
Reference
g l y c o si d e pentose amino ribose ribose
cherry purple purple pink-red pink-red
114 115 115,116 116 117
Both t h i n - l a y e r and p a p e r chromatog r a p h y w i l l p r o v i d e s p e c i f i c i d e n t i f i c a t i o n of neomycin. Numerous s y s t e m s f o r t h i s p u r p o s e w i l l b e found l i s t e d i n s e c t i o n 6 . 3 4 . I n a d d i t i o n t o t h e above c h e m i c a l t e s t s a number o f m i c r o b i o l o g i c a l p r o c e d u r e s have b e e n have d e s c r i b e d a reported. Heinmann e t simple t e s t t o d i f f e r e n t i a t e neomycin-like m o l e c u l e s from t e t r a c y c l i n e s and c h l o r a m p h e n i c o l . When added t o a column of i n n o c u l a t e d a g a r o n l y t h e n e o m y c i n - l i k e m o l e c u l e s show a n a r e a of g r o w t h i n h i b i t i o n a t t h e t o p o f t h e column. A more s p e c i f i c m i c r o b i o l o g i c a l p r o c e d u r e h a s b e e n r e p o r t e d by F r e r e s and B u l l a n d 1 l g . By u s i n g f o u r t e s t OrganiSmS(8aCillUb c e k e u n , BacilCub b u b t i l i b , Sahcina C u t e a and M i c k u c o c c u b 6Cavub)patterns of i n h i b i t i o n w e r e determined f o r e a c h of t h e 1 2 a n t i b i o t i c s e x t r a c t e d i n t o t h r e e solvents. Comparing t h e i n h i b i t i o n p a t t e r n o f a n
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unknown a n t i b i o t i c w i t h t h e s t a n d a r d p a t t e r n s , t h e a u t h o r s were a b l e t o i d e n t i f y t h e p r e s e n c e o f i n d i v i d u a l s u b s t a n c e s i n animal t i s s u e . A s i m i l a r t e s t h a s a l s o b e e n d e s c r i b e d by T i e c c o e t 6.2.
Chemical P r o c e d u r e s 6.21.
T i t r i m e t r i c Assay
The d e t e r m i n a t i o n of neomycin by non-a u e o u s t i t r a t i o n h a s been d e s c r i b e d by Penau e t a l q 2 1 . Neomycin b a s e i s a l l o w e d t o r e a c t w i t h standardised perchloric acid; the excess acid i s t h e n b a c k - t i t r a t e d w i t h p o t a s s i u m hydrogen p h t h a l a t e u s i n g c r y s t a l v i o l e t a s i n d i c a t o r . To d e t e r mine t h e neomycin c o n t e n t of t h e s u l p h a t e s a l t t h e same a u t h o r s p r e c i p i t a t e d t h e s u l p h a t e w i t h b e n z i d i n e b e f o r e r e a c t i n g t h e neomycin w i t h p e r c h l o r i c a c i d . The amount o f b e n z i d i n e r e q u i r e d t o p r e c i p i t a t e t h e s u l p h a t e i s c a l c u l a t e d from t h e s u l p h a t e c o n t e n t which i s i t s e l f d e t e r m i n e d by t i t r a t i o n w i t h sodium h y d r o x i d e . An a l t e r n a t i v e method f o r d e t e r m i n i n g t h e s u l p h a t e c o n t e n t o f neomycin s u l h a t e h a s been r e p o r t e d by Roets and Vanderhaeghey22. The p r o c e d u r e i n v o l v e s a t i t r a t i o n w i t h b a r i u m c h l o r i d e and m u s t be c a r r i e d o u t i n a 30-40% s o l u t i o n of a l c o h o l i n o r d e r t o o b t a i n a s h a r p endA s the antibiotic is insoluble i n alcohol point. it i s n e c e s s a r y t o remove t h e neomycin p a r t o f t h e This i s accomplished molecule p r i o r t o t i t r a t i o n . u s i n g a c a t i o n e x c h a n g e r e s i n s u c h a s Dowex 5 0 - X 8 .
D u r i n g an i n v e s t i g a t i o n of t h e c o m p l e x a t i o n p r o p e r t i e s of neomycin, H a r r i s 1 O 2 r e p o r t e d t h e ti t r a t i o n o f neomycin conduc t o m e t r i c a l l y w i t h a m a r a n t h ( F . D . and C Red N o . 2 ) . The e n d - p o i n t o f t h e t i t r a t i o n i s s h a r p and h a s good reproducibility. 6.22.
Polarography
The u s e of d i f f e r e n t i a l p u l s e p o l a r o g r a p h y t o d e t e r m i n e neomycin s u l p h a t e i n aqueous s o l u t i o n s h a s been d e s c r i b e d by S i e g e r m a n et F o l l o w i n g a c i d h y d r o l y s i s of neomycin, t h e s o l u t i o n was a d j u s t e d t o pH 4 and 0 . 1 M a c e t a t e
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b u f f e r ( p H 4 ) added a s s u p p o r t i n g e l e c t r o l y t e . R e d u c t i o n p o t e n t i a l s of -0.19 and -0.36V w e r e obtained. The above a u t h o r s a l s o d e s c r i b e d t h e a p p l i c a t i o n of t h i s t e c h n i q u e t o t h e e x a m i n a t i o n o f s a m p l e s of s k i n p r e v i o u s l y t r e a t e d w i t h neomycin-containing formulations. 6.23. Polarimetry Neomycins B and C h a v e b e e n shown t o d i f f e r i n t h e i r s p e c i f i c r o t a t i o n v a l u e s , neomycin B h a v i n g a s p e c i f i c r o t a t i o n of + 80° and neomycin c a s e c i f i c r o t a t i o n o f + 1 2 0 0 1 2 4 , 1 2 7 . Brooks e t a 1 12g made t h i s f a c t t h e b a s i s f o r a number o f methods t o d e t e r m i n e t h e B & C c o n t e n t o f commercial neomycin. The s p e c i f i c r o t a t i o n o f t h e t e s t s o l u t i o n i s d e t e r m i n e d a t 25OC and t o t a l neomycin d e t e r m i n e d e i t h e r t i t r i m e t r i c a l l y o r s p e c t r o p h o t o m e t r i c a l l y . By s u b s t i t u t i o n of t h e s e v a l u e s i n a s u i t a b l e e q u a t i o n t h e c o n c e n t r a t i o n o f neoI n a s e c o n d method mycins B and C a r e c a l c u l a t e d . t h e same a u t h o r s d e t e r m i n e d t h e s p e c i f i c r o t a t i o n of t h e t e s t - s o l u t i o n a t t e m p e r a t u r e s o f 25O and 7 5 O C . The c h a n g e i n t h e v a l u e of s p e c i f i c r o t a t i o n on i n c r e a s i n g t h e t e m p e r a t u r e from 25Oto 75OC c a n t h e n b e u s e d t o c a l c u l a t e t h e amounts of neomycin B and C i n t h e s a m p l e . The u s e o f an a u t o m a t i c p o l a r i m e t e r w i t h a f l o w - c e l l h a s been r e p o r t e d by d e Rosri126 , t o m o n i t o r t h e e l u a t e from an i o n e x c h a n g e column (Bio-Rad A G l - X 2 ) t h r o u g h which a s o l u t i o n of neomycin w a s p a s s e d . The d e t e c t i o n o f an o p t i c a l l y a c t i v e s u b s t a n c e was r e c o r d e d e l e c t r o n i c a l l y w i t h a s u i t a b l e pen r e c o r d e r . By d e t e r m i n i n g t h e a r e a s of t h e p e a k s r e c o r d e d , t h e amounts of neomycir,s B and C and neamine i n a number of c o m m e r c i a l s a m p l e s have b e e n d e t e r m i n e d . 6.24.
R a d i o - c h e m i c a l Assay
To d e t e r m i n e t h e r e l a t i v e amounts o f neomycins B C and neamine by r a d i o chemical method, K a i s e r i 2 8 s e p a r a t e d t h e “C - l a b e l l e d Na c e t y l d e r i v a t i v e s by p a p e r c h r o m a t o g r a p h y and q u a n t i t a t e d t h e chromatograms by l i q u i d s c i n t i l l a t i o n c o u n t i n g . A c o e f f i c i e n t of v a r i a t i o n of 3 . 6 % w a s obtained.
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Seaman and Stewart1’’ have described a radio-chemical assay f o r determining neomycin on c o t t o n - f a b r i c . Neomycin i s r e a c t e d with carbon d i s u l p h i d e forming a d i t h i o c a r b o n a t e silver which i s t h e n decomposed w i t h [lloAg] n i t r a t e . The p r e c i p i t a t e d [ll0Ag] s i l v e r s u l p h i d e , which i s d i r e c t l y r e l a t e d t o t h e amount o f neomycin p r e s e n t , i s e s t i m a t e d by c o u n t i n g . Recently an i s o t o p e d i l u t i o n method h a s been r e p o r t e d 1 3 0 f o r a s s a y i n g neomycin s u l p h a t e . However, it i s f i r s t n e c e s s a r y t o p r e p a r e I 4 C - l a b e l l e d neomycin s u l p h a t e T h i s i s a c c o m p l i s h e d by a d d i n g 1 4 C - l a b e l l e d g l u c o s e t o a small-scale fer m entation of S . dtadiae.. 14C-labelled neomycin c a n t h e n be e x t r a c t e d by s o l v e n t - e x t r a c t i o n o r by ion-exchange c h r o m a t o g r a p h y .
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6.25.
Uorimetric Assay
The neomycin m o l e c u l e d o e s n o t e x h i b i t fluor escence b u t following s u i t a b l e der i v a t i s a t i o n two s p e c t r o f l u o r i m e t r i c d e t e r m i n a t i o n s reported the have been d e s c r i b e d . Maeda e t c o m p l e x a t i o n of s i m p l e h e x o s a m i n e s w i t h p y r i d o x a l and z i n c i o n s t o r e s u l t i n a f l u o r e s c e n t d e r i v a l y i n g t h i s p r o c e d u r e t o neomycin, tive. demonstrated a l i n e a r response over t h e Simpson c o n c e n t r a t i o n r a n g e 0-50 uq/ml o f neomycin s u l p h a t e .
33
The r e a c t i o n of neomycin w i t h f l u o r e s c a m i n e t o form a f l u o r e s c e n t complex h a s been r e p o r t e d by K u s n i r & Barna133. The f l u o r e s c e n c e i n t e n s i t y v a r i e s w i t h b o t h t h e pH of t h e s o l u t i o n (optimum pH r a n g e 7 . 5 - 9 . 5 ) and t h e amount of f l u o r e s c a m i n e added. T h i s p r o c e d u r e may b e u s e d t o d e t e r m i n e neomycin a t v e r y low l e v e l s , t h e minimum c o n c e n t r a t i o n d e t e r m i n a b l e b e i n g 45 ng/ml. 6.26.
S p e c t r o p h o t o m e t r i c Assay
Spectrophotometric a s s a y s of neomycin may be c o n v e n i e n t l y d i v i d e d i n t o t w o groups: -
(a) (b)
Direct methods, i n v o l v i n g t h e i n t a c t neomycin m o l e c u l e . I n d i r e c t methods , i n v o l v i n g h y d r o l y s i s of neomycin p r i o r t o a s s a y .
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43 1
( a )D i r e c t Methods 0 ' Keefe and R u ~ s o - A l e s i l ~ i r~sft r e p o r t e d t h e a p p l i c a t i o n of n i n h y d r i n t o t h e a s s a y o f n e o mycin, t h e p r o c e d u r e b e i n g an a d a p t a t i o n of t h a t d e s c r i b e d by Moore and S t e i n 1 3 5 f o r t h e a s s a y o f amino a c i d s and i n v o l v i n g measurement a t 570nm o f t h e p u r p l e - c o l o u r e d complex formed. Maehr and S h a f f n e r 1 3 6 have a p p l i e d t h i s p r o c e d u r e t o t h e d e t e r m i n a t i o n o f neomycin i n c h r o m a t o r a p h y column e l u a t e s . Gerosa and M e l a n d r i attempted t o a p p l y t h e Moore and S t e i n method t o t h e q u a n t i t a t i v e d e t e r m i n a t i o n of neomycin i n p h a r m a c e u t i c a l preparations b u t reported a l i n e a r response only o v e r t h e s h o r t c o n c e n t r a t i o n r a n g e o f 400-600pg/ml o f neomycin. B o r ~ w i e c k a land ~ ~ Thorburn-Burns e t a1139 however, r e p o r t e d no s u c h l i m i t a t i o n and s u c c e s s f u l l y a p p l i e d t h e method t o t h e a s s a y o f neomycin i n p h a r m a c e u t i c a l f o r m u l a t i o n s . P r e g n a l a t t o and S a b i n o 2 0 0 i n c o r p o r a t e d g l y c e r i n e i n t o t h e n i n h y d r i n s o l u t i o n and r e p o r t e d an i m proved s e n s i t i v i t y and r e p r o d u c i b i l i t y e n a b l i n g neomycin c o n c e n t r a t i o n s a s l o w a s 4 pg/ml t o be d e t e r m i n e d . An a u t o m a t e d n i n h y d r i n a s s a y h a s b e e n d e s c r i b e d by K a p t i o n a k , B i e r n a c k a and P a z d e r a l 4 0 b a s e d on a m o d i f i e d Moore and S t e i n m e t h o d l 4 1 . An a l t e r n a t i v e r e a g e n t which a l s o reacts w i t h t h e p r i m a r y amino g r o u p s of neomycin h a s r e c e n t l y been d e s c r i b e d l 7 2 . The r e a g e n t , d i c l o n e ( 2 , 3 - d i c h l o r o - l , 4 - n a p h t h o q u i n o n e ) , r e a c t s w i t h neomycin b a s e t o form an o r a n g e - c o l o u r e d p r o d u c t when t h e s o l u t i o n i s a d j u s t e d t o pH 4 .
C o m p l e x a t i o n of neomycin w i t h v a r i o u s d y e s was r e p o r t e d by H e i n l o o and t h e a q u e o u s i n s o l u b i l i t y o f t h e complex w i t h a m a r a n t h ( F . D . & C Red N o . 2 ) h a s been u t i l i s e d by H i l l 2 5 and by B u f t o n and S a d d l e r 1 4 2 t o a s s a y neomycin i n a q u e o u s s o l u t i o n . Amaranth may a l s o be u s e d t o d e t e r m i n e neomycin i n p r o d u c t i o n s a m p l e s from f e r m e n t a t i o n r e c o v e r 1 6 8 , The d y e , Orange 11, h a s b e e n s i m i l a r l y 1 4 3 d e s c r i b e d ( 1 max. = 484 nm) Complex f o r m a t i o n between neomycin and t h e dye i s v e r y d e p e n d a n t on t h e i o n i c s t r e n g t h o f t h e s o l u t i o n , thus n e c e s s i t a t i n g c a r e f u l c o n t r o l of reaction c o n d i t i o n s t o e n s u r e c o m p l e t e p r e c i p i t a t i o n of t h e complex d u r i n g t h e a s s a y p r o c e d u r e . R e a c t i o n of sodium l 1 2 - n a p h t h o - q u i n o n e - 4-su l p h o n a t e w i t h
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n e 0 m y c i n l 4 ~ p r o d u c e san o r a n g e / y e l l o w product,Xmax 460nm i n a c e t i c a c i d , which h a s been u t i l i s e d t o d e t e r m i n e t h e neomycin c o n t e n t o f o p h t h a l m i c s o l u t i o n s g i v i n g r e s u l t s i n good a g r e e m e n t w i t h microbiological assays. S t r o n g l y b a s i c a n t i b i o t i c s may be p r e c i p i t a t e d by f o r m a t i o n of t h e c o l o u r e d r e i n e c k a t e s a l t which may t h e n be d e t e r m i n e d s p e c t r o p h o t o m e t r i ~ a l l y l ~B~i c .k f o r d l 6 6 d i s s o l v e d t h e p r e c i p i t a t e d neomycin r e i n e c k a t e i n a c e t o n e and h a s s u c c e s s f u l l y u s e d t h i s p r o c e d u r e t o a s s a y neomycin e x t r a c t e d from t o p i c a l f o r m u l a t i o n s . Roushdi e t a1173 p r e f e r r e d t o oxidise the p r e c i p i t a t e with potassium p e r m a n g a n a t e and t h e n c o l o r i m e t r i c a l l y e s t i m a t e t h e chromate produced w i t h d i p h e n y l c a r b a z i d e . A r o m a t i c a l d e h y d e s r e a c t w i t h p r i m a r y amines f o r m i n g S c h i f f ' s b a s e s which a r e o f t e n c o l o u r e d . The c o l o u r may t h e n be u s e d t o q u a n t i t a t e t h e amine. Using t h i s p r i n c i p l e Kocy167 h a s shown neomycin t o form a y e l l o w - c o l o u r e d S c h i f f ' s b a s e w i t h s a l i c y l a l d e h y d e t h o u g h t h e q u a n t i t a t i v e a s p e c t of t h i s p r o c e d u r e i s , as y e t , i n c o m p l e t e . The c o m p l e x a t i o n o f neomycin w i t h c o p p e r r e s u l t s i n t h e f o r m a t i o n of a b l u e - c o l o u r e d compound which h a s a l s o been made t h e b a s i s o f a c o l o r i m e t r i c d e t e r m i n a t i o n o f neomycin i n pharmac e u t i c a l f o r m u l a t i o n s g 7 . Maximum c o l o u r i n t e n s i t y was o b s e r v e d a t a s o l u t i o n pH of 10. F u r t h e r i n v e s t i g a t i o n showed t h e s t o i c h i o m e t r y of t h e comp l e x t o be 1:l i n a l k a l i n e s o l u t i o n . ( b) I n d i r e c t Methods H y d r o l y s i s p r o d u c t s o f neomycin may b e an a m i n o - s u g a r , a p e n t o s e o r f u r f u r a l d e p e n d i n g on t h e r e a c t i o n c o n d i t i o n s c h o s e n . Each o f t h e s e e n t i t i e s h a s been u t i l i s e d f o r i n d i r e c t s p e c t r o p h o t o m e t r i c d e t e r m i n a t i o n o f neomycin. The p r e s e n c e o f a s u g a r m o i e t y i n neomycin was d e m o n s t r a t e d by Hamre e t a1145 who u s e d c a r b a z o l e and a n t h r o n e t o q u a n t i t a t e neomycins B and C i n commercial neomycin. The p r o c e d u r e s employed were t h o s e p r e v i o u s l y a p p l i e d t o manosido~ t r e p t o m y c i n,147. l ~ ~ Penau e t r e p o r t e d poor
N E O MY CI N
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a g r e e m e n t b e t w e e n r e s u l t s o b t a i n e d by t h e a n t h r o n e a s s a y and m i c r o b i o l o g i c a l p r o c e d u r e s and s u g g e s t e d t h e p r e s e n c e of c a r b o h y d r a t e i m p u r i t i e s i n neomycin t o be t h e r e a s o n . O t h e r r e a g e n t s which f o r m c o l u d comp l e x e s w i t h s u g a r s s u c h a s o r c i n o l 1 4 % 1 5 ? 9 ,1 5 0 ( 3,5d i h y d r o x y t o l u e n e ) and p h l o r o g l ~ c i n o (1 l ~,3~,~ 5t r i h y d r o x y b e n z e n e ) have b e e n r e p o r t e d f o r t h e s p e c t r o p h o t o m e t r i c a s s a y o f neomycin. Hoodless c l a i m e d t h e p h l o r o g l u c i n o l p r o c e d u r e t o be less time-consuming t h a n o t h e r methods117 and a p p l i e d t h i s p r o c e d u r e t o neomycin s u l p h a t e raw m a t e r i a l . D ~ u l a k a s la d ~ o~p t e d a s i m i l a r p r o c e d u r e t o d e t e r mine t h e neomycin s u l p h a t e c o n t e n t o f o p h t h a l m i c ointments. I n t e r f e r i n g substances co-extracted from t h e o i n t m e n t were s e p a r a t e d from neomycin by TLC b e f o r e r e a c t i n g t h e a n t i b i o t i c w i t h p h l o r o glucinol. The o r c i n o l p r o c e d u r e h a s been u s e d t o a s s a y t h e neomycin c o n t e n t of f e r m e n t e r b r o t h s 1 4 8 I 1 4 9 I 150 though i t i s n e c e s s a r y t o f i r s t s e p a r a t e t h e a n t i b i o t i c by i o n - e x c h a n g e c h r o m a t o g r a p h y . Korchegin15O r e p o r t e d good a g r e e m e n t between t h e o r c i n o l a s s a y f production samand t h e m i c r o b i o l o g i c a l a s s a ples. Khromov-and S t a r u n o v ay7' and K o r c h a g i n e t compared t h e o r c i n o l and m i c r o b i o l o g i c a l a s s a y s f o r d e t e r m i n i n g t h e neomycin c o n t e n t of p o l y m e r - f i l m s a n d , a g a i n , good a g r e e m e n t b e t w e e n t h e two p r o c e d u r e s was n o t e d . A f t e r m i l d h y d r o l y s i s , neomycin h a s been shown t o g i v e a p o s i t i v e Elson-Morgan r e a c t i o n 1 5 1 , a r e a c t i o n c h a r a c t e r i s t i c o f amino-sugars152. A method i n v o l v i n g t h i s r e a c t i o n h a s been made t h e b a s i s of a q u a n t i t a t i v e a s s a y f o r n e ~ m y c i n l ~ ~ which h a s been u s e d t o d e t e r m i n e t h e neomycin cont e n t of f e r m e n t a t i o n b r o t h s 1 5 4 . V i g o r o u s h y d r o l y s i s o f neomycin r e s u l t s i n be q u a n t i t a t e d i n a number of d i f f e r e n t ways15xf156 . D u t c h e r e t a1157 u s e d a UV s p e c t r o p h o t o m e t r i c p r o c e d u r e , m e a s u r i n g t h e a b s o r b a n c e of t h e s o l u t i o n a t 280nm. A s i m i l a r p r o c e d u r e combined w i t h measurement of t h e o p t i c a l r o t a t i o n h a s b e e n u s e d by Brooks e t a l l 5 8 t o d e t e r m i n e t h e neomycin B and C c o n t e n t t h e f o r m a t i o n o f f ~ r f u r a l which l ~ ~ ma
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of t h e a n t i b i o t i c . Colorimetrically, the furfural o b t a i n e d from neomycin may be a s s a y e d w i t h an a n i l i n e by m e a s u r i n g t h e amount o f p i n k / r e d complex formed. Morgan e t a1159 u s e d 4 - b r o m o a n i l i n e i n t h i s c o n t e x t , t h e 4-bromo d e r i v a t i v e b e i n g more resist a n t t o t h e formation of i n t e r f e r i n g coloured prod u c t s t h a n a n i l i n e i t s e l f l 6 0 . T h i s method h a s been a p p l i e d t o v a r i o u s p h a r m a c e u t i c a l f o r m u l a t i o n s and r e s u l t s show good a g r e e m e n t w i t h m i c r o b i o l o g i c a l a s s a y s . A n i l i n e h a s been u s e d t o d e t e r m i n e t h e neomycin c o n t e n t o f f e r m e n t e r b r o t h s and o t h e r p r o d u c t i o n s a m p l e s l 6 1 , neomycin u n d e c y l e n a t e and neomycin c a p r y l a t e l 6 2 . Much work h a s been c a r r i e d o u t t o e s t a b l i s h optimum c o n d i t i o n s f o r a r e p r o d u c i b l e c o n v e r s i o n of neomycin t o f u r f u r a l , q u a n t i t a t i v e c o n v e r s i o n of t h e p e n t o s e m o i e t y t o f u r f u r a l b e i n g d i f f i c u l t and The a c i d s t r e n g t h t h e procedures tedious163t164. f o r optimum p r o d u c t i o n o f f u r f u r a l must b e s u c h t h a t i t i s s t r o n g enough t o h y d r o l y s e t h e s u g a r m o l e c u l e , y e t i n s u f f i c i e n t l y s t r o n g t o decompose t h e f u r f u r a l formed. A r e v i e w o f t h e l i t e r a t u r e by I v a s h k i v 1 7 0 showed 1 2 % h y d r o c h l o r i c a c i d t o b e a c c e p t e d a s optimum f o r c o n v e r s i o n o f p e n t o s e s t o f u r f u r a l . However, a s neomycin must f i r s t b e decomposed t o t h e pentose b e f o r e h y d r o l y s i s of t h e s u g a r can t a k e p l a c e , more v i o r o u s c o n d i t i o n s a r e r e q u i r e d . Dutcher e t a l l Z 4 used 4 0 % s u l p h u r i c a c i d t o produce an a c i d c o n c e n t r a t i o n o f 37% i n t h e s o l u t i o n f o r h y d r o l y s i s and o b t a i n e d maximum f o r m a t i o n o f f u r f u r a l a f t e r 1% h r s r e f l u x . Morgan e t a1159 however, u s e d 7 0 % s u l p h u r i c a c i d t o p r o d u c e a 25% a c i d conc e n t r a t i o n i n t h e h y d r o l y s i s s o l u t i o n and o b t a i n e d maximum f o r m a t i o n o f f u r f u r a l a f t e r one h o u r . I v a s h k i v 1 7 0 h a s e v a l u a t e d t h e u s e of b o t h hydroc h l o r i c and s u l p h u r i c a c i d s and found up t o f o u r t i m e s more f u r f u r a l t o be p r o d u c e d by s u l p h u r i c acid, the y i e l d being extremely s e n s i t i v e t o the c o n c e n t r a t i o n of a c i d employed. C o n t i n u i n g f u r t h e r work w i t h s u l p h u r i c a c i d , t h e f o r m a t i o n o f f u r f u r a l a s a f u n c t i o n o f neomycin c o n c e n t r a t i o n was e x amined and t h e c o n c l u s i o n r e a c h e d t h a t b e t t e r y i e l d s of f u r f u r a l a r e o b t a i n e d a t low c o n c e n t r a t i o n s of t h e a n t i b i o t i c . Heyes171 h a s shown a cons t a n t amount of f u r f u r a l t o be p r o d u c e d on hydrol y s i s w i t h 27-28% s u l p h u r i c a c i d , r e f l u x i n g f o r 1 h o u r . T h i s makes i t u n n e c e s s a r y t o a c c u r a t e l y
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p i p e t t e concentrated s o l u t i o n s of sulphuric acid. From t h e above d i s c u s s i o n i t would, t h e r e f o r e a p p e a r n e c e s s a r y t o e s t a b l i s h optimum c o n d i t i o n s f o r f u r f u r a l p r o d u c t i o n i n e a c h i n d i v i d u a l case. 6.3. Chromatographic Procedures 6.31. Counter-Current D i s t r i b u t i o n S w a r t , L e c h e v a l i e r and Waksman 1 7 6 have examined neomycin by t h e method o f c o u n t e r c u r r e n t d i s t r i b u t i o n u s i n g a p a r t i t i o n - s y s t e m of b o r a t e b u f f e r ( p H 7 . 6 ) / p e n t a s o l ( s y n t h e t i c amyl a l cohol)/stearic acid. T h r e e m a j o r components w i t h v a r y i n g amounts of neamine were found i n s a m p l e s of neomycin B from v a r i o u s s o u r c e s . D e t e r m i n a t i o n o f t h e amount of a n t i b i o t i c r e m a i n i n g i n e a c h t u b e f o l l o w i n g p a r t i t i o n was c a r r i e d o u t m i c r o b i o l o g i cally. I n an e x t e n s i o n o f t h i s s t u d y t o t h e whole g r o u p of n e o m y c i n - l i k e m o l e c u l e s S c h a f f n e r 1 7 7 however, h a s been u n a b l e t o s e p a r a t e neomycin B i n t o t h e s e p a r a t e components r e p o r t e d by S w a r t e t u s i n g e i t h e r o f f o u r p a r t i t i o n s y s t e m s . The s y s t e m s employed w e r e : Systems 1-3) 0 . 5 M b o r a t e b u f f e r a t pH 7 . 3 , 7.6 o r 7 . 8 / p e n t a s o l / s t e a r i c acid. 4 ) 0 . 5 % b i c a r b o n a t e buf f e r / p e n t a s o l / stearic acid.
Both c h e m i c a l and m i c r o b i o l o g i c a l assays w e r e u t i l i z e d t o determine the d i s t r i b u t i o n of a n t i b i o t i c i n t h e t u b e s . In a l l experiments t h e m i c r o b i o l o g i c a l a s s a y r e s u l t s w e r e more e r r a t i c t h a n t h e c o r r e s p o n d i n g c h e m i c a l a s s a y s and on t h i s b a s i s S c h a f f n e r e x p l a i n e d t h e d i f f e r e n c e between h i s r e s u l t s and t h o s e of S w a r t e t who u s e d o n l y m i c r o b i o l o g i c a l d e t e r m i n a t i o n s . I n t h i s same work S c h a f f n e r w a s a b l e t o d e m o n s t r a t e t h e same d i s t r i b u t i o n p a t t e r n f o r b o t h f r a m y c e t i n and neomycins B and C and t h u s t e n t a t i v e l y i d e n t i Similarly, but using f i e d f r a m y c e t i n a s neomycin. a p a r t i t i o n s y s t e m o f 3% p - t o l u e n e s u l p h o n i c a c i d i n 1N a c e t a t e b u f f e r (pH 3 . 8 ) / b u t a n o l B a i k i n a e t have i d e n t i f i e d m c e r i n and c o l i m y c i n a s neomycin a n d S a n n i k o v 1 7 5 h a s i d e n t i f i e d f r a m i c i n w i t h neomycin.
WILLIAM F. HEYES
436
From a p r e p a r a t i v e a s p e c t , Peck e t a l l 8 ' have employed t h e c o u n t e r - c u r r e n t d i s t r i b u t i o n t e c h n i q u e w i t h a p a r t i t i o n s y s t e m of water/ b u t a n o l / p - t o l u e n e s u l p h o n i c a c i d t o s e p a r a t e and p u r i f y t h e neamine (neomycin A ) p r e s e n t i n commerc i a l neomycin. 6.32 Electrophoresis
Neomycin i s a r e a d i l y i o n i s a b l e m o l e c u l e and s h o u l d t h u s b e s e p a r a b l e from o t h e r a n t i b i o t i c s by a p p l i c a t i o n of an e l e c t r i c f i e l d ( z o n e e l e c t r o p h o r e s i s ) . V a r i o u s w o r k e r s have s u c c e s s f u l l y a p p l i e d t h i s t e c h n i q u e t o neomycin and T a b l e 10 summarises t h e c o n d i t i o n s r e p o r t e d i n t h e l i t e r a t u r e . A number o f a u t h o r s d e s c r i b e d t h e q u a l i t a t i v e s e p a r a t i o n o f neomycin from o t h e r c h e m i c a l - t p e s of a n t i b i o t i c s u s i n g p a p e r - e l e c t r o p h o r e s i s l 8 y t 1 8 5 , 1 8 7 w h i l e Ochab189 d e s c r i b e d s y s r e m s s p e c i f i c a l l y d e s i g n e d t o s e p a r a t e compounds within the i n o g l y c o s i d e group of a n t i b i o t i c s . C a r r e t all' have r e p o r t e d t h e q u a n t i t a t i v e d e t e r m i n a t i o n o f neomycin i n t h e p r e s e n c e o f p o l y m i x i n and b a c i t r a c i n . Using p a p e r e l e c t r o p h o r e s i s q u a n t i t a t i o n of neomycin w a s a c c o m p l i s h e d c o l o r i metrically with ninhydrin. Lightbown and DeRossi 188 s u b s t i t u t e d an a g a r - g e l s u p p o r t f o r t h e more u s u a l c h r o m a t o g r a p h y - p a p e r and s u c c e s s f u l l y s e p a r a t e d neomycin from a v a r i e t y o f a n t i b i o t i c s b u t n o t from paromomycin. However, ' q u a n t i t a t i o n o f t h i s p r o c e d u r e w a s n o t p o s s i b l e d u e t o t h e e l o n g a t e d zone of i n h i b i t i o n produced by neomycin on i n c u b a t i o n o f the agar-gel. The same a u t h o r s a l s o r e p o r t e d some anomalous b e h a v i o u r of t h e neomycin i o n i n t h e p r e s e n c e of c e r t a i n t y p e s of a g a r . Neomycin i s a b a s i c m o l e c u l e and u n d e r n o r m a l c i r c u m s t a n c e s would be e x p e c t e d t o b e h a v e a s a c a t i o n and m i g r a t e t o t h e anode. However, w i t h c e r t a i n t y p e s of a g a r t h e neomycin w a s o b s e r v e d t o m i g r a t e t o w a r d s t h e c a t h o d e . T h i s phenomena w a s r e p e a t e d l y c o n f i r m e d though n o t e x p l a i n e d . A s y s t e m s u i t a b l e f o r t h e q u a n t i t a t i v e e s t i m a t i o n of neomycin u s i n an a g a r g e l s u p p o r t h a s been d e s c r i b e d by Grynney83. T o o b t a i n a good c l e a r zone f o r neomycin i t w a s n e c e s s a r y t o change t h e b u f f e r e d e l e c t r o l y t e / a g a r - g e l t o a p h o s p h a t e s y s t e m a t pH 6 . 5 . D e t e c t i o n of t h e
rl
rl
m
c
-d
k
h
a
c c c
-4
Eu
\
3 m
Ln rl
k a, a ru a
k
7
om w k
k a,
m W Q
W
u
2
E
.
Ln
3 0 \ 0s 3 0
oa,
m
..
W W
. .
k a,
w 3 Q
w 7
a
5
4
a m
0
rl
Eu k
7
om w k
om
k
0
k
Lnc N
3 0
7
lclk
7
W k
3 0
3
\
3 0 0
In
-
oa,
m
0s
m N
.d
e
m..c
Ln
m
\ - a ,
z a a -L!
m
. . N
L13
=I
ru a,
u c
0 PI
Table lO(Contd..
.)
E l e c t r o p h o r e s i s of Neomycin Electrolyte
P
5. Trishydroxymethylaminomethane/maleic a c i d / sodium h y d r o x i d e ( 0 . 9 0 7 % :0.870%:0 . 0 0 2 % ) pH 5 . 6
agar-gel buffered pH 5 . 6
6.
paper
m w
2 M f o r m i c acid/O.lM toluene sulphonate/ p r o p ano l / w a C e r ( 5 0 : 50:5 :40)pH 1 . 8
(40:5:5:50)
7.
Conditions
Medium ~-
I
2 ooov 2 0 0 mA
3 40v
D e t e c t i n g Agent (See a l s o S ectio n 6.34)
B .n u b L L L L A
B . A u bLLk5A
189
ATCC 6633
1 89 paper
340v
toluene sulphonate/ water ( 4 0 : 5 :55)pH 1 . 9
8 . 1 M ammonium h y d r o x i d e / 1 M sodium h y d r o x i d e / 0 . 1 M toluene sulphonate/ p r o p a n ol / w at e r ( 2 0 : O . 5 : 10: 1 0 : 6 9 . 5 ) pH 1 0 . 8
188
NCTC 8 2 4 1
pH 1 . 9
2 M f o r m i c acid/O.lM
Reference
73. Aub&.k%A
189
ATCC 6633
paper
340v
B . AubLL&iA ATCC 6633
189
T a b l e 10 (Contd.
.. )
E l e c t r o p h o r e s i s o f Neomycin
9.
Electrolyte
Medium -
1M ammonium h y d r o x i d e / 1M sodium h y d r o x i d e / w a t e r
paper
(20:0.25:79.75)pH
3 40v
Detect i n g Agent R e f e r en c e (See a l s o S e c t i o n 6.343
B.bubXilib
189
ATCC 6633
11.5
10. i M sodium h y d r o x i d e / w a t e r ( 5 : 9 5 ) pH 1 2 - 2
11. Acrylamide g e l
Conditions
pH 4 . 6
'd P
ic
1 2 . pH 6.5 p h o s p h a t e b u f f e r (KHPO4 22g/l; KH2P04,28g/l)diluted 1 : 4 0 with d i s t i l l e d water.
paper
3 40v
B.aubtiLib
189
ATCC 6633
a c r y 1amide ge 1 a g a r -ge 1 buffered a t pH 6 . 5
lOOV, 2mA
Naphthalene Black
190
310 t o 360v
Staphalococcub
183
(current 5 50mA)
c p i d etr mid i b
ATCC 1 2 2 2 8
WILLIAM F. HEYES
440
a n t i b i o t i c was a c h i e v e d b i o a u t o g r a p h i c a l l y . The o r g a n i s m S f a p h a l o c o c c u a e p i d e h m i d i a ATCC 12228 w a s found t o be t h e m o s t s e n s i t i v e f o r t h i s p u r p o s e . (The d e s c r i p t i o n o f a l t e r n a t i v e b i o a u t o g r a p h i c a l s y s t e m s w i l l be found i n s e c t i o n 6 . 3 4 . ) Using an a c r y l a m i d e - g e l as s u p p o r t , CoombelgO h a s d e m o n s t r a t e d t h e q u a n t i t a t i v e a s s a y of neomycin w i t h a r e c o v e r y o f 9 6 % i n t h e p r e s e n c e of b a c i t r a c i n and p o l y m i x i n . I n t h i s case q u a n t i t a t i o n w a s a c h i e v e d by d e n s i t o m e t r y a f t e r s t a i n i n g the g e l with naphthalene black. E l e c t r o p h o r e s i s h a s a l s o been employed t o s e p a r a t e neomycin f r o m a n a l y t i c a l l y i n t e r f e r i n g s u b s t a n c e s s u c h a s p r o t e i n s . Hence B r a m m e r and Hemson182 have d e t e r m i n e d t h e neomycin c o n t e n t of b l o o d serum. Neomycin was s e p a r a t e d from t h e serum p r o t e i n s by e l e c t r o p h o r e s i s on c e l l u l o s e a c e t a t e and a s s a y e d c o l o r i m e t r i c a l l y f o l l o w i n g e l u t i o n from t h e s u p p o r t . A modified technique c o n s i s t i n g of an e l e c t r i c f i e l d a p p l i e d p e r p e n d i c u l a r t o a f l o w i n g b u f f e r s o l u t i o n and u s i n g c h r o m a t o g r a p h y p a p e r a s support(cross-electrophoresis) h a s been e x p l o i t e d t o s t u d y t h e r e a c t i o n of neomycin w i t h h e ~ a r i n ~ ~ E t vl i~d e~n c. e f o r t h e f o r m a t i o n o f a neomycin-heparin complex was o b t a i n e d by t h i s means.
6.33.
Column Chromatoqraphy
The column c h r o m a t o g r a p h i c s e p a r a t i o n of neomycin B , neomycin C and neamine on an ion-exchan e column h a s been d e s c r i b e d by Maehr and S c h a f f n e r ?3 6 Dowex 1 X 2 ( O H f o r m ) was t h e i o n e x c h a n g e r e s i n and w a t e r t h e e l u t i n g s o l v e n t . The column e l u a t e was m o n i t o r e d by r e a c t i o n w i t h n i n h y d r i n . Using a slower e l u t i o n r a t e and a s m a l l e r p a r t i c l e s i z e of t h e same i o n - e x c h a n g e r e s i n Inouye and Ogawa19 r e p o r t e d improved r e s o l u t i o n of t h e p e a k s . The a p p l i c a t i o n o f t h i s p r o c e d u r e t o t h e q u a n t i t a t i v e d e t e r m i n a t i o n of neomycin C and n e a mine i n commercial s a m p l e s of raw m a t e r i a l h a s a l s o b e e n d e s c r i b e d 6 . When compared w i t h TLC res u l t s on t h e same s a m p l e s , t h e column chromatog r a p h i c method gave c o n s i s t e n t l y h i g h e r r e s u l t s f o r t h e neamine c o n t e n t . TLC e x a m i n a t i o n o f t h e
.
NEOMYCIN
44 I
f r a c t i o n of e l u a t e c o n t a i n i n g neamine , d e m o n s t r a t e d t h e p r e s e n c e o f t h r e e o t h e r u n i d e n t i f i e d compounds which gave a p o s i t i v e n i n h y d r i n r e a c t i o n t h u s exp l a i n i n g t h e o b s e r v e d d i f f e r e n c e between t h e t w o procedures. R o e t s and Vanderhaeghe l9 h a v e a l s o examined neomycin by c h r o m a t o g r a p h y on Dowex 1x2 b u t t h e s e a u t h o r s m o n i t o r e d t h e column e l u a t e c o n d u c t o m e t r i c a l l y . G i l l e t e t a l l g 4 appl i e d a s i m i l a r p r o c e d u r e t o t h e e x a m i n a t i o n of v a r i o u s s a m p l e s of neomycin t o a s c e r t a i n t h e r a t i o of neomycin B:C. A number of minor components p r e s e n t i n commercial neomycin h a v e been s e p a r a t e d by column c h r o m a t o g r a p h y on a c a r b o x y l i c c a t i o n exchange r e s i n I A m b e r l i t e ~ ~ - 5 The 0 ~components ~ ~ . were e l u t e d from t h e r e s i n w i t h ammonium h y d r o x i d e s o l u t i o n . T . L . C . o f t h e e l u e n t f r a c t i o n s showed t h e p r e s e n c e of two p r e v i o u s l y u n r e p o r t e d i m p u r i t i e s which were t h e n i s o l a t e d on Dowex 1 x 2 and t e n t a t i v e l y i d e n t i f i e d u s i n g NMR and mass s p e c t r o metry.
When i n v e s t i g a t i n g t h e a c i d h y d r o l y s i s o f neomycin I B r a z h n i k o v a and K u d i n o v a l g 8 added a s u l p h o c a t i on i c - t y p e i o n -exchange re s i n t o t h e a c i d s o l u t i o n of a n t i b i o t i c t o a d s o r b i n t e r m e d i a t e h y d r o l y s i s p r o d u c t s and t h u s p r e v e n t f u r t h e r decomposition d u r i n g h e a t i n g . Following e l u t i o n o f t h e r e s i n . i n a column t h e p r o d u c t s o f neomycin h y d r o l y s i s w e r e i d e n t i f i e d and shown t o be d e p e n d a n t on t h e t i m e o f h y d r o l y s i s . An i o n - e x c h a n g e c h r o m a t o g r a p h i c p r o c e d u r e u t i l i s i n g Dowex 1x2 h a s been made t h e b a s i s of an i n d u s t r i a l process f o r manufacturing neomycin B which i s f r e e from neomycin C l g 5 .
The i s o l a t i o n o f neamine on A m b e r l i t e I R C 5 0 ( N a f o r m ) f o l l o w i n g t h e a c i d hydrol y s i s of neomycin h a s been d e s c r i b e d l g 6 . Neamine i s e l u t e d from t h e i o n - e x c h a n g e column w i t h h d r o chloric acid. T h i s p r o c e s s had been p a t e n t e d 7 9 7 a s a means of m a n u f a c t u r i n g neamine.
WILLIAM F. HEYES
442
Many column c h r o m a t o g r a p h i c p r o c e d u r e s have been d e s c r i b e d f o r t h e commercial s e p a r a t i o n and p u r i f i c a t i o n of neomycin f o l l o w i n g fermentation. 6.34.
Paper and Thin-Layer Chromatograph
The e x a m i n a t i o n of neomycin by p a p e r and t h i n - l a y e r c h r o m a t o g r a p h y h a s b e e n f o r t w o main p u r p o s e s : a ) t o s e p a r a t e and i d e n t i f y neomycin i n t h e p r e s e n c e of o t h e r a n t i b i o t i c s , and b ) t o s e p a r a t e i n d i v i d u a l components and d e g r a d a t i o n p r o d u c t s o f neomycin. The s o l v e n t s y s t e m s employed f o r t h e s e p u r p o s e s a r e summarised i n T a b l e s 1 2 and 1 3 ( p a p e r c h r o m a t o g r a p h y ) and T a b l e s 1 4 and 1 5 (thin-layer procedures)
.
V i s u a l i s a t i o n of t h e chromatograms h a s been r e p o r t e d u s i n g b o t h c h e m i c a l and m i c r o b i o l o g i c a l means. Chemical s p r a y r e a g e n t s which h a v e been d e s c r i b e d a r e l i s t e d i n T a b l e 1 6 . The v a r i o u s o r g a n i s m s t h a t have b e e n employed f o r b i o a u t o g r a p h y a r e g i v e n i n T a b l e 11. T a b l e 11
V is u a l i s a t i o n o f Chromatograms Bioautographically Organism
Reference 201,202,204,228 234,235
.
B putniluh
22 4
€a c h e t r i c h i a c o l i
205,206
S t a p h a l o c o c c u h aukeuh
2 0 7 , 2 2 0 , 2 3 1 , 2 32
ATCC 6538 s t r a i n
Table 12 P a p e r C h r o m a t o g r a p h i c S y s t e m s S e p a r a t i n g Neomycin from o t h e r A n t i b i o t i c s Paper
Direction
S o l v e n t Sys t e m
Rf V a l u e
Use
Reference
Whatman N o . 1
A s c e n d i n9
Water - s a t u r a t e d butanol
0.84
Whatman No.1
Ascend i n g
n-Butano l/ace t i c a c i d / w a t e r ( 2 :1:1)
0.85
Whatman N o . 1
Ascending
n-Butanol/pyridine/ w a t e r (1:0 . 6 :1)
0.94
) Identifi-
202
Whatman N o . 1 A s c e n d i n g
3 % Aqueous ammonium chloride
0.00
202
Whatman No.1
Ascending
Benzene/acetic acid/ w a t e r ( 2 : 1:1), o r g a n i c 1a y e r
0.89
) c a t i o n of Ineomycin i n ) t h e presence )of o t h e r )antibiotics
Whatman No.1
A s cend i n g
n -Bu t a n 0 1- s a t u r a t e d
0.07
)
202
1 202
1
1 ) )
202
202
water
Toyo No. 5 0
Ascending
Methanol/3 % a q u e o u s sodium c h l o r i d e ( 5 :1)
Descending for 9 hrs.
n-Butanol/pyridine/ acetic acid/water ( 1 5 : 10: 3 :1 2 )
0.03
) S e p a r a t i o n of neomycin from )other I streptomyces )antibiotics
203
204
Table 1 2 (Contd.. 1 P a p e r C h r o m a t o g r a p h i c Systems S e p a r a t i n g Neomycin from o t h e r A n t i b i o t i c s D i r e c tion
S o l v e n t System
Toyo N o . 5 0
Descending for 9 hrs.
2 % p-toluene sulphoni c acid + 2% pyridine i n wet n - b u t a n o l
Toyo No. 5 0
Ascending
t-Butanol/acetic w a t e r ( 5 5 :6 :39)
Whatman No.1
Ascending
Whatman N o . 1
Ascending
Paper
Rf V a l u e
Use
Reference
0 . 4 8 - 0 . 5 4 ) S e p a r a t i o n of Ineomycin f r o m ) other 1s t r e p t o m y c e s )antibiotics.
204
0.06
1
20 4
Water
0.98
)
205
Water-saturated n -bu t a n 0 1
Oe0
!i d e n t i f i c a t i o n
acid/
P
Systematic
'of the antibiotics
2 05
Whatman N o . 1 Ascending
Water-saturated e t h y l acetate
Whatman N o . 1 Ascending
W a t e r - s a t u r a t e d benzene
0.0
Whatman No.1
Methanol/water ( 4 0 : 6 0 )
0.21 )
205,206
Whatman N o . 1 Ascending
n-Propanol/water ( 4 0 : 6 0 )
0.20 )
205,206
Whatman N o . 1
Ascending
Methanol/3% a q u e o u s ammonium c h l o r i d e ( 7 0 : 3 0 )
0.11 )1
205,206
Whatman No.1
Ascending
Methyl e t h y l k e t o n e / n b u t a n o l / w a t e r ( 3 0 : 5 :6 5 )
0.27
Ascending
2 05
1 )
2 05
1 )
1
205,206
Table 1 2 (Contd..
.)
P a p e r C h r o m a t o g r a p h i c Systems S e p a r a t i n g Neomycin from o t h e r A n t i b i o t i c s Paper Whatman No.1
Direction Ascending
S o l v e n t System 6 6 . 6 % aqueous propanol/benzene/ethylene glycol/acetic a c i d ( 5 :5 :1 . 5 :1)
0.03 )
0.27
Whatman No.1
Ascending
5 0 % aqueous p r o p a n o l / a c e t i c a c i d ( 2 5 : 1)
Whatman N o . 1
Ascending
Water-saturated butanol/acetic acid/potassium c y a n i d e ( 100: 1:0: 0 5 9 ) n-Butanol/water/acetic acid(30:13:8)
Whatman No.3
Ascending
Whatman No.3
Ascending
Whatman No. 3
Ascending
Rf V a l u e
n-Butanol/acetic acid/ pyridine/water/ethanol ( 6 0 : 15: 6 :5 :5) n-Butanol/water/acetic acid/pyridine/sodium c h l o r i d e ( 3 0 : 1 2 : 7 :2: 0.1)
__ Use
R e f e re n c e
207
)
1
1
O.O0
' S e p a r a t i o n of neomycin from ch l o r a m p h e n i c o l , tetracycline ) and p e n i c i l l i n
1
207
207
)
Oso2
0.04
' s e p a r a t i o n of neomycin f r o m 'polymixin B and b a c i t r a c i n
186,208
!
186,208
1
1 0.05 )
1
1
186,208
Table 13
P a p e r C h r o m a t o g r a p h i c S y s t e m s S e p a r a t i n g Neomycin Components and D e g r a d a t i o n P r o d u c t s Paper
Direction
S o l v e n t Sy s t e m
Rf Value Neomycin Neamine B
-
P m P
Whatman No.1
Descending
-
Toyo No.50
Descending for 9 hrs
Water /bu t a n o 1/ m e t h a n ol / m e t h y 1 orange . ( 2 : 4 : 1:1:5 ) Butanol/pyridine/ w a t e r ( 6 0 : 30: 4 0 )
Butanol/pyridine/ w a t e r ( 3 :2: 1)
n-Propanol/ pyridine/acetic acid/water (15:10:3:12)
Use
Reference
C
N o t available
0.29
0.19
N o t available
0.13
-
0.15
0.28) ) ) ) )
Stability testing fradiomycin
209
Separation o f B and C as a c e t y l derivatives
2 10
Separation of B and C as a c e t y l derivatives
211
Separation of neamine f r o m neomycins B and C
204
Table 13 (Contd.. ) P a p e r C h r o m a t o g r a p h i c Systems S e p a r a t i n g Neomycin Components and D e g r a d a t i o n P r o d u c t s Paper
Direction
S o l v e n t System
Rf Value Neomycin Neamine B
Toyo N o . 50 Toyo
Descending for 9 hrs Ascending
No. 5 0
2 % p-toluene sulphonic acid in w a t e r s a t u r a t e d n-butanol
0.11-
1 . 5 % sodium c h l o r i d e i n 80% m e t h a n o l
0.08-
Use
Reference
C
0.20
0.11
0.23
0.22
)Separation
)of neamine
20 4
) from neo)mycins B )and C
1
P P 4
Grade M
Ascending
Butanol/acetic acid/wat er (4:l: 5)
Whatman NO. 4
Descending f o r 24-3g h r s , 28 C
n-Butanol/water/ piperidine (84:16:2)
Not a v a i l a b l e
Separation of B and C as acetyl derivatives
0.70 0.35 1-00 Q u a n t i t a t i v e (values r e l a t i v e spectrophotot o neamine) m e t r i c determ i n a t i o n of components
212
213
Table 1 3 ( C o n t d . .
.)
P a p e r C h r o m a t o g r a p h i c Systems S e p a r a t i n g Neomycin Components and D e g r a d a t i o n P r o d u c t s Paper
Direction
S o l v e n t System
Rf V a l u e Neomycin B
Whatman No. 1
Descending f o r 2 4- 36 h r s , 2527OC
P
Methyl e t h y l ke t o n e / t -bu t ano 1/ methanol/6.5N ammonium h y d r o x i d e (16:3:1:6)
Use
Reference
Neamine
C
0.54 0.30 1.00 (values r e l a t i v e t o neamine)
Separation a s f r e e bases Q u a n ti t a t i on by s p e c t r o ph ot o m e t r y
m P
Whatman No. 1
-
Descending f o r 8-400 hrs , 24 C
Methyl e t h y l k e t o n e / 0 . 5 7 0.34 1.00 isopropanol/6.5N (values r e l a t i v e ammonium h y d r o x i d e t o neamine) (80:20:30)
Radial
But an o l / p y r i d i n e / a c e t i c acid/water (15: 10: 3 :1 2 )
Whatman D e s c e n d i n g No.limf o r 18 h r s pregnated with PH 8 buffer
N o t available
Butanol/water(l:2) 0.5 containing 4% t o l u e n e s u l p h o n ic a c i d and 2 % p i p e r i d i n e hydrochloride
0.6
0
214
2 15
Separation of degradation products
216
S e p a r a t i o n of neamine from neomycin B and C
228
Table 1 4 T h i n L a y e r C h r o m a t o g r a p h i c Systems S e p a r a t i n q Neomvcin from O t h e r A n t i b i o t i c s Ads o r b e n t
S o l v e n t Sys tern
Rf Value
Use
Reference
n-Propanol/ethylacetate/ w a t e r / 1 3 . 4 M ammonium h y d r o x i d e ( 5 0 : 10: 30: 10)
0.52
S e p a r a t i o n of neomycin from o t h e r aminoglycoside antibiotics
217
Cellulose MN
n-Propanol/pyridine/ a c e t i c acid/water ( 1 5 :10: 3 :1 2 1
0.10
S e p a r a t i o n of neomycin from other w a t e r soluble basic a n t i b i o t ic s
2 18
Kieselgel G
Wate r / m e t hano l / b u t an o l / butyl acetate/acetic a c i d ( 1 2 :2.5 :7 . 5 :4 0 :2 0 )
0.0
S i l i c a ge 1 G/
aluminium o x i d e (1:1)
P \c
Kieselgel G
Kieselgel G
Water/butanol/pyridine/ a c e t i c a c i d . ( 1 4 :30: 2 0 : 6 ) ( 1 6 :4 0 : 8: 1 6 ) Water/butanol/acetic a c i d (39 :55 :6 )
219
)
1 S e p a r a t i o n of 1 neomycin from 1 bacitracin, ) p o l y m i x i n and
0.12
)
tyrothricin
219
0.00 )
1 1 0.00
)
219
T a b l e 1 4 (Contd..
.)
Thin L a y e r C h r o m a t o g r a p h i c Systems S e p a r a t i n g Neomycin from O t h e r A n t i b i o t i c s Ad s or b e n t Kieselgel G
Se ph adex G-15 P VI 0
S o l v e n t System Methanol/l7% aqueous ammonia c h l o r o f o r m , a q u e o u s l a y e r (10:10:20)
pH6 p h o s p h a t e b u f f e r (0.025M) + 0.5M sodium chloride
Rf V a l u e
0.31
Use ) Sep aratio n of ) neomycin from )bacitracin, ) p o l y m i x i n and )tyrothricin
Reference
219
1 1 0.75
) Identification
220
)of antibiotics Silica gel G Kieselgel G
Kieselgel G
Ben z e n e / a c e t one/ ace t i c a c i d ( 4 :4 :2 ) But a n o l / a c e t i c a c i d / pyridine/water (30: 2 2 : 6 : 3 8 ) Butanol/water/acetic acid/ethanol/pyridine ( 6 0 : 10:15: 5: 6 )
0.35
1 1
221
? Separation 0.14
of ’? nebmycin from zinc bacitracin ’1 and polymixin
186 208
0.05
1
186 208
T a b l e 14 (Contd..
.)
Thin Layer Chromatographic Systems S e p a r a t i n g Neomycin from Other A n t i b i o t i c s Ad so r ben t Kieselgel G Kieselgel G + Kieselguhr
S o l v e n t System Propanol/ethyl acetate/water/ 2 5 % ammonium hydroxide (100:20:60:20).
Use
Rf Value 0.08
)
Reference 222
1 0.14
)
222
1
G(1:l)
1
Kieselgel G + Kieselguhr G(1:2)
0.22
)
222
C e 1l u l o s e MN-300
0.32
) S e p a r a t i o n of 'glycosidic
222
antibiotics
1
Kieselgel G + aluminium oxide G type E ( 1 : l )
0.12
Kieselgel G impregnated w i t h sodium acetate
0.33
)
222
1
)
1
1
222
T a b l e 2 (Contd.. ) Thin Layer Chromatographic Systems S e p a r a t i n g Neomycin from Other A n t i b i o t i c s Ads o r b e n t Kieselgel G Kieselgel G + Kieselguhr G ( 1 : 1) Kieselgel G + Kieselguhr G(1:2)
S o l v e n t System Prop a n o l / e t hy 1 ace t a t e / w a t e r / 2 5 % ammonium hydroxide/ p y r i d i n e / 3 . 8 5 % aqueous ammonium a c e t a t e ( 100:2 0 :6 0 :2 0 :10:2 00) II
Rf
Value 0.11
Kieselgel G impregnated w i t h 3.85% aqueous ammonium acetate Kieselgel G Kieselgel G + Kieselguhr G(1:l) Kieselgel G + Kieselguhr G(1:2)
1 1
0.16
222
1 1
222
1
1 0.08
S e p a r a t i o n of glycosidic antibiotics 222
1 0.11
(100:20:60:20:10:200) It
222 222
0.08
Ethanol/ethylacetate/water/ 25% ammonium hydroxide/ p y r i d i n e / 3 . 8 5 % aqueous ammonium a c e t a t e
Reference
0.13
VI P h,
Use
222
1 0.12
222
1 1
.
Table 1 4 (Contd. ) Thin Layer Chromatographic Systems S e p a r a t i n q Neomycin from Other A n t i b i o t i c s Adsorbent --
S o l v e n t System
Use
Rf Value
Reference
Kieselgel G + aluminium oxide G ( t y p e E ) (1:1)
Ethanol/ethylacetate/water/ 2 5 % ammonium hydroxide/ p y r i d i n e / 3 . 8 5 % aqueous ammonium a c e t a t e (100: 2 0 : 6 0 : 2 0 : 10: 2 0 0 )
0.08
Kieselgel G
Methanol/ethyl a c e t a t e / water/25 % ammonium hydroxi d e / p y r i d i n e / 3 . 8 5 % aqueous ammonium a c e t a t e (100:20:60:20:10:200)
0.06
)
222
0.17
)
222
222
)
1 1
1 VI P
Kieselgel G + Kieselguhr G (1:1) Kieselgel G + Kieselguhr
11
0.14
222
1 1
G(1:2)
Kieselgel G + aluminium oxide G , type E ( 1 : l )
’)
S e p a r a t i o n of glycosidic antibiotics
Methanol/ethyl a c e t a t e / water/25% ammonium hydroxi d e / p y r i d i n e / 3 . 8 5 % aqueous ammonium acetate ( 100 :2 0 :6 0 :2 0 : 10: 2 0 0 )
0.11
)
1 1
1
222
Table -1 4 (Contd. . I Thin Layer Chromatographic Systems S e p a r a t i n g Neomycin from Other A n t i b i o t i c s
VI
Ads o r b e n t
So lven t System
Rf v a l u e
Kieselgel G impregnated w i t h 3.85% aqueous ammonium acetate
Methanol/ethyl acetate/ water/25% ammonium hydroxi d e / p y r i d i n e / 3 . 8 5 % aqueous ammonium a c e t a t e (100: 20: 60: 2 0 : 10: 2 0 0 )
0.08
Kieselgel G
Butanol/methanol/ethyl a c e t a t e / w a t e r / 2 5 % ammonium
0.06
fr
Kieselgel G + Kieselguhr G ( 1 : 1) Kieselgel G + Kieselguhr G(1:2)
hydroxide/pyridine/3.85% aqueous ammonium acetate
222
1 1 1 1 1 222
1
0.07
222
1
(100: 100: 20: 60: 20: 10: 2 0 0 )
0.13
) S e p a r a t i o n of ) glycosidic ) antibiotics
222
1 0.05
Kieselgel G + aluminium oxide G , type E ( 1 : l ) Kieselgel G + Kieselguhr G(1:2)
Reference
)
222
1 25 % ammonium hydroxide/ water/acetone (16: 144: 40)
0.36
1
222
T a b l e 1 4 (Contd.. 1 Thin Layer Chromatographic Systems S e p a r a t i n g Neomycin from Other A n t i b i o t i c s Adsorbent Kieselgel G + Kieselguhr G(1:2)impregnated with 2 % sodium a c e t a t e
%
S o l v e n t System 2 5 % ammonium hydroxide/ w a t e r/ a c e t on e (16:144 :40)
Kieselgel G + aluminium oxide G , t y p e E (1:1)
If
Kieselgel G + Kieselguhr G ( 1 : 1)impregnated with 2 % sodium a c e t a t e
11
Kieselgel G
Use -
Rf Value 0.34
1 1
Reference 222
1 1
0.48
) S e p a r a t i o n of glycosidic antibiotics
222
1 0.43
222
)
1 1 1 1 Water/sodium c i t r a t e / c i t r i c acid (100:20:5)
0.95
Classification of a n t i b i o t i c s
223
Table 15 Thin Layer Chromatographic Systems S e p a r a t i n g Neomycin Components and Degradation P r o d u c t s Adsorbent
Use
Rf Value
S o l v e n t System Neomycin B
Neomycin
Neamine
C
Acidified carbon
Water
0.10
0.10
0.60
Acidified carbon
0.5N s u l p h u r i c acid
0.21
0.43
0.61
Untreated carbon
Water
0.00
0.00
0.00
Untreated carbon
0.5N s u l p h u r i c acid
VI P
0.5N hydroCarbon chloric acid treated w i t h hydrochloric acid II
0.5N hydroc h l o r i c acid/ methanol ( 4 :1)
0.24 0.37-0.45
Reference
0.45 0.53-0.74
0.54 0.63-0.92
)Assay of ) neomycin )components ) i n commer) c i a 1 form)ulations
22 4
)
224
1 1
224
)
224
)
204
1 ) Separation ) of neomycins
)B and C and
0.44-0.72
0.58-0.81
0.64-0.91
) neamine )
1 1
20 4
T a bl e 15 (Contd.. -
.)
Thin L a y e r C h r o m a t o q r a p h i c Systems S e p a r a t i n g Neomycin Components and D e g r a d a t i o n P r o d u c t s Ad s or b e n t
S o l v e n t System Neomycin
B Carbon treated with w a t e r
Carbon/ gypsum treated with sulphuric acid
Carbon/ gypsum treated with water
0.5N hydrochloric acid
0.41
0.5N hydrochloric acid/ m e t h a n o l ( 4 : 1)
0.48
0.5N s u l p h u r i c acid
0.20
Rf V a l u e Neomycin
Use -
Reference
Neamine
C 0.57
20 4
0.62 )
0.58
0.68
1
204
)
1 0.59
0.80 ) Sep aratio n of neomycins ) B and C and ) neamine
20 4
1 1
1 0.5N s u l p h u r i c a c i d / m e t h a n o l ( 4 : 1) 0.5N hydrochloric acid
0.64
0.82
0.85 )
0.16
0.28
0.30
204
1 20 4 )
1
Table 15 (Contd.. ) Thin Layer Chromatographic Systems S e p a r a t i n g Neomycin Components and Degradation P r o d u c t s Adsorbent
R f Value
S o l v e n t System Neomycin
Carbon/ gypsum treated with water P
0.5N s u l p h u r i c acid
B
Neomycin C
0.24
0.40
Use
R e f er e n c e
Neamine
--
20 4
1 1 )Separation ) o f neomycin )B and C and ) neamine
I1
0.5N hydrochloric acid/ methanol (1:1)
0.36
0.36
0.46
11
0.5N hydroc h l o r i c acid/ p r o p a n o l ( 1 : 1)
0.48
0.48
0.52
Kieselgel H
3.85% aqueous ammonium acetate
0.13
0.13
0.36
Assay of neamine
196,9
Kieselgel H
3 . 4 % ammonium hydroxide
0.37
0.44
0.47
Assay of neomycin C
196,9
v, W
1 1
20 4
20 4
Table 15 (Contd.. ) Thin Layer Chromatographic Systems S e p a r a t i n g Neomycin Components and Degradation P r o d u c t s Ads orben t
C e 1l u l o s e MN
R f Value -
S o l v e n t System
Methyl e t h y l ketone/iso-
Neomycin
Neomycin
B
C
0.21
0.12
Use -
Neamine 0.31
propanol/6.5N ammonium hydroxide (80:20:30)
2 \o
Cellulose MN-300
Methyl e t h y l k e tone/me t h a n o 1/ isopropanol/7.9N ammonium hydro x i d e (10: 8.5 :3 :7 )
Cellulose MN-300
Propanol/pyridine/ a c e t i c acid/water ( 100 :6 6 :2 0 :80)
Silica gel G
11
R e fe r e n ce
Separation
of neomycin
2 15
components
0.52
0.24
single 0.25 double 0.33
development 0.20 0.47 development 0.25 0.60
0.57
0.66
0.61
236
)Assay of )neomycins B 226 land C and nea)mine i n pharm) a c e u t i c a l form0.73 ) u l a t i o n s 226
Table 15 (Contd.. ) Thin Layer Chromatographic Systems S e p a r a t i n g Neomycin Components and Deqradation P r o d u c t s Ad s o r ben t
S o l v e n t System Neomycin
m
0
Use
Rf Value B
Neomycin C 0.46
Cellulose MN-300/ Kieselguhr G(1:l)
Propanol/pyridine/ acetic acid/water (100: 66 :20: 80)
0.53
Silica gel G
Prop an o l /e t hy 1 acetate/water/25% ammonium hydroxide (100:20:60:20)
0.23
Reference
Neamine 0.73 )
226
1 1 0.23
0.42
)
226
1 1
Cellulose MN-300/ Kieselguhr G(1:l)
Methanol/3% aqueous 0.36 sodium c h l o r i d e ( 2 :1)
0.17
Silica gel G/ Kieselguhr G(1:2)
3.85 % aqueous ammonium a c e t a t e
0.22
0.22
)Assay of )neomycins B 0.43 ) a n d C and 226 )nearnine i n )pharmaceutical ) formulations
1 '0.39 )
1 1 1
226
Table 1 5 (Contd.. ) Thin Layer Chromatographic Systems S e p a r a t i n g Neomycin Components and Degradation P r o d u c t s Adsorbent
S o l v e n t System Neomycin B
Silica gel G
Kieselguhr
Rf Value Neomycin
Neamine
0.14
0.11
0.22
0.46
0.68
0.84
Propanol/e than0.18 ol/ethyl acetate/ water/25% ammonium hydroxide/pyridine/ 3.85%ammonium a c e t a t e (100: 100: 2 0 : 6 0 : 20: 10: 2 0 0 )
0.15
)Assay of )neomycins B ) a n d C and lneamine i n )pharmaceutical 0 - 38 f o r m u l a t i o n s
0.11
0.32 )
Methyl e t h y l ketone/ t b u t ano l / m e t han o1/ 6.5N ammonium hydroxide ( 1 6 0 : 30: 10: 6 0 ) II
purified
Silica g e l G/ Kieselguhr G(1:2)
Reference
C
G
Silica gel G
Use -
II
0.18
)
226
226
1 226
Table 1 5 (Contd.. ) Thin Layer Chromatographic Systems S e p a r a t i n g Neomycin Components and Degradation P r o d u c t s Adsorbent
S o l v e n t System
Use -
R f Value
Neomycin B
Neomycin
Reference
Neamine
C
1.5M Sodium a c e t a t e , pH 8.5
0.15
0.15
0.28
227
25SA)
+ 58.49 sodium chloride/ t - b u t a n o l ( 1 0 : 1)
S e p a r a t i o n of neamine from neomycins B and C
Silica ge 1
3% Ammonium hydroxide / a c e t o n e ( 1 6 0 : 40)
0.33
0.33
-
Quantitative a n a l y s i s of n e omy c i n sulphate
229
Kieselgel G
3% Ammonium hydroxide / a c e t o n e ( 1 6 0 : 90)
S t a b i l i t y of neomycin a f t e r e t h y l e n e oxide st e r i l i s a t i o n
233
Dowex 50x8 sodium form(1onex
N o t available
463
N EOMY CIN
T a b l e 16
V i s u a l i s a t i o n of Chromatograms by C h e m i c a l Means Spray Reagent
1. E t h a n o l i c sodium h ypoch 1o r it e f o l l o w e d by s t a r c h / potassium iodide solution 2 . Ch l o r i n e /e t h a n o 1 f o l l o w e d by s t a r c h / potassium iodide solution 3. C h l o r i n e / c a r b o n tetrachloride f o l l o w e d by s t a r c h / p o t as s ium i o d i d e / pyridine 4 . t - b u t y l hypochlor i t e / d i ch 1oromethane/acetic acid f o l l o w e d by s t a r c h / potassium iodide solution 5. N i n h y d r i n
Ninhydrin/cadmium acetate 7. p - d i m e t h y l aminoben z a l d e h y d e
6.
Ninhydrin/pd i m e t h y l aminobenzaldehyde 9 . Copper s u l p h a t e / ammonium h y d r oxide
Colour of Neomycin zone
R e f e r e n ce
Dark b l u e
210,211
Dark b l u e
212
Dark b l u e
213
Dark b l u e
196
Purple
186,203,208 2 1 4 , 2 1 5 ,2 1 6 217,218,219 229,231
Purple/p ink
227
Pink o r purple
223 226
8.
Blue
221
464
WILLIAM F. HEYES
Q u a n t i t a t i v e a n a l y s i s o f neomycin a f t e r c h r o m a t o g r a p h y u t i l i s i n g some o f t h e v i s u a l i s a t i o n t e c h n i q u e s g i v e n i n T a b l e s 11 and 1 6 have been r e p o r t e d . Majumder a n d Majumder213 s e p a r a t e d neomycins B a n d C a s t h e a c e t y l d e r i v a t i v e s on p a p e r t h e n , f o l l o w i n g c o n v e r s i o n t o t h e c h l o r o d e r i v a t i v e s , t h e c o l o u r formed by r e a c t i o n w i t h t h e starch/iodine/hydrochloric a c i d r e a g e n t w a s measure d a t 570nm. A l a t e r p a p e r by t h e same a u t h o r s 2 1 4 d e s c r i b e d t h e s e p a r a t i o n o f neomycins B and C as t h e f r e e b a s e s . The r e s u l t i n g chromatograms w e r e ded e v e l o p e d w i t h n i n h y d r i n t h e n t h e c o l o u r e d complex e l u t e d i n t o m e t h a n o l and t h e a b s o r b a n c e o f t h e s o l u t i o n measured a t 570nm. Thin- l a y e r c h r o m a t o g r a p h y h a s been u s e d b y F o p p i a n o and Brown229 t o a s s a y t h e t o t a l neomycin B and C c o n t e n t of neomycin s u l p h a t e . The neomycin zone w a s s c r a p e d o f f t h e p l a t e and rea c t e d w i t h o r c i n o l / f e r r i c c h l o r i d e r e a g e n t , t h e abs o r b a n c e o f t h e r e s u l t i n g c o l o u r b e i n g measured a t 665nm. By t h i s p r o c e d u r e a p r e c i s i o n o f 2% was achieved. Ninhydrin h a s also been used t o quantitate neomycin c o l o r i m e t r i c a l l y f o l l o w i n g t h i n - l a e r c h r o m a t o g r a p h y . P r e g n o l a t t o and S a b i n 0 2 5 0 r e p o r t e d t h e a d d i t i o n of g l y c e r i n e t o t h e n i n h y d r i n s o l u t i o n t o improve t h e s e n s i t i v i t y and An a l t e r n a t i v e r e p r o d u c i b i l i t y of t h e p r o c e d u r e . c o l o r i m e t r i c p r o c e d u r e f o r t h e q u a n t i t a t i o n of neomycin a f t e r c h r o m a t o g r a p h y h a s been d e s c r i b e d by D o u l a k a s l 7 4 . Neomycin i s e l u t e d f r o m t h e s i l i c a g e l w i t h pH 1 2 . 5 p h o s p h a t e b u f f e r t h e n o x i d i s e d w i t h sodium h y p o b r o m i t e . The r e s u l t i n g a l d e h y d e i s complexed w i t h p h l o r o g l u c i n o l y i e l d i n g a p i n k c o l o u r e d p r o d u c t which i s measured s p e c t r o p h o t o metrically. The u s e o f b i o a u t o g r a p h y f o r t h e q u a n t i t a t i o n of chromatograms h a s b e e n d e s c r i b e d by many w o r k e r s . E m i l i a n o w i c z - C z e r s k a and Herman228 s e p a r a t e d neamine f r o m neomycins B and C t h e n q u a n t i t a t i v e l y d e t e r m i n e d t o t a l neomycin B and C by b i o a u t o g r a p h y w i t h B.hubtiCih. A l i n e a r res p o n s e f o r c o n c e n t r a t i o n s between 0 . 2 5 and 1 O p g o f neomycin w a s o b t a i n e d . With a s i m i l a r t e c h n i q u e b u t using a mathematical a n a l y s i s of the bioauto-
NEOMYCIN
465
g r a m s , Simon230 r e p o r t e d a q u a n t i t a t i v e d e t e r m i n a t i o n o f neomycin s u i t a b l e f o r u s e w i t h i r r e g u l a r Brodasky224 employed b i o a u t o g r a p h y shaped zones. w i t h BaciLLuh pumiluh f o r t h e a s s a y o f neomycin and neamine a f t e r s e p a r a t i o n by T.L.C. on a l a y e r of c a r b o n . The q u a n t i t a t i o n o f s m a l l amounts of n e o mycin C however, p r o v e d d i f f i c u l t , t h e d i f f i c u l t ies b e i n g a s s o c i a t e d w i t h t h e enhanced growth of t h e o r g a n i s m i n t h e p r e s e n c e o f c a r b o n ( f r o m t h e T.L.C. p l a t e ) and ammonium i o n s ( f r o m t h e c h r o m a t o g r a p h i c procedure). Similar d i f f i c u l t i e s w e r e experienced by S o k o l s k i and L ~ m m i s 2 3who ~ a t t r i b u t e d p o o r neomycin z o n e s t o be t h e r e s u l t o f a n t a g o n i s m by t h e sodium c h l o r i d e p r e s e n t i n t h e b i o a u t o g r a p h i c s y s tem. An e x t e n s i v e s t u d y by L a n g n e r 2 0 1 d e m o n s t r a t e d maximum s e n s i t i v i t y f o r t h e d e t e r m i n a t i o n of neomycin t o b e a p p a r e n t u s i n g t h e o r g a n i s m B.dubtiLih (ATCC 6633) t o g e t h e r w i t h pH 8 T r i s a g a r . The d e t e c t i o n l i m i t f o l l o w i n g chromatography w a s r e p o r t e d t o be 0.05pg. 6.35.
G a s - L i q u i d Chromatography
T s u j i and R o b e r t s o n l g 2 a c h i e v e d t h e s e p a r a t i o n of neomycin B , neomycin C and neamine as t h e t r i m e t h y l s i l y l e t h e r s on a 6 f t . column of 0 . 7 5 % OV-1 on G a s Chrom Q a t a t e m p e r a t u r e of 290OC. The same c o n d i t i o n s have a l s o b e e n shown t o s e p a r a t e n e o b i o s a m i n e B , neosamine and d e o x y s t r e p t a m i n e from neomycin and neamine. Hence t h e method c o u l d b e u s e d t o s t u d y t h e s t a b i l i t y o f neomycin o r t o m o n i t o r t h e b i o s y n t h e t i c p r o d u c t i o n U s e of t h e p r o c e d u r e t o assess t h e s t a b process. i l i t y o f neomycin i n p h a r m a c e u t i c a l f o r m u l a t i o n s h a s b e e n d e m o n s t r a t e d by Van G i e s s e n and T s u j i 2 3 7 w i t h t r i l a u r i n as i n t e r n a l s t a n d a r d . H o w e v e r , t h e s e a u t h o r s recommended a 2 f t . column packed w i t h 3 % OV-1 on G a s Chrom Q as l o n g e r columns r e q u i r e d a h i g h e r t e m p e r a t u r e t o c h r o m a t o g r a p h neomycin and c o n s e q u e n t l y h a d a r e d u c e d column l i f e . A concent r a t i o n o f 3 % OV-1 w a s p r e f e r r e d , a s 2 % o r less r e s u l t e d i n i n c r e a s e d column a d s o r p t i o n o f neomycin. A f t e r a f u r t h e r s t u d y of t h e p r o c e d u r e Margosis and T s u j i 2 3 8 recommended a number of improvements t o o p t i m i s e t h e a n a l y s i s o f neomycin by G . L . C . The improvements t o t h e a s s a y i n c l u d e d t h e modif icat i o n o f t h e i n j e c t i o n p o r t t o p r e v e n t s a m p l e dec o m p o s i t i o n by c o n t a c t o f i n j e c t e d m a t e r i a l w i t h
WILLIAM F. HEYES
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m e t a l o r Teflon and t h e a d d i t i o n of an a c c u r a t e volume of s i l y l a t i n g r e a g e n t t o each sample and s t a n d a r d t o overcome i n c o n s i s t e n t d e r i v a t i s a t i o n . A comparison of t h e G.L.C. and microbiological(agar-diffusion) a s s a y s h a s been rep o r t e d by T s u j i e t a1239 who showed t h e neomycin c o n t e n t of neomycin s u l p h a t e powders determined by t h e G.L.C. method, t o c o r r e l a t e w e l l w i t h v a l u e s o b t a i n e d by t h e m i c r o b i o l o g i c a l a s s a y when it i s assumed neomycin C h a s 35% o f t h e b i o l o g i c a l act i v i t y of neomycin B.
Neomycin h a s been s e p a r a t e d from m i x t u r e s of o t h e r aminoglycoside a n t i b i o t i c s cont a i n i n g t h e 2-deoxystreptamine moiety a s b o t h t h e p e r t r i m e t h y l s i l y l d e r i v a t i v e and t h e N - t r i f l u o r o a c e t y l p e r t r i m e t h y l s i l y l d e r i v a t i v e u s i n g a column of 0.75% OV-1 on Gas Chrom Q 2 4 0 . The p r o c e d u r e may be used t o e s t i m a t e t h e number of s u g a r moieti e s bound i n t h e a n t i b i o t i c as a close r e l a t i o n s h i p e x i s t s between t h e number of r i n g s and t h e retention t i m e . Examination of neomycin B by a combined G.C.-M.S. procedure h a s been r e p o r t e d by Murata e t a l l 5 . G.C. w a s accomplished w i t h t h e t r i m e t h y l s i l y l d e r i v a t i v e on a l m column of 1%OV-1 on Chromosorb W , by which means neomycin was s e p a r a t ed from kanamycin. The r e s u l t i n g mass s p e c t r a of t h e neomycin d e r i v a t i v e e x h i b i t e d a minute molec u l a r i o n peak a t m / e 1550 i n d i c a t i n g t h a t a l l a c t i v e hydrogens of b o t h hydroxy and amine groups were completely s i l y l a t e d . 6.4.Microbiological Procedures 6 . 4 1 . T u r b i d i m e t r i c Assay Various organisms have 'been used t o a s s a y neomycin t u r b i d i m e t r i c a l l y . These are summarised i n T a b l e 1 7 w i t h t h e working concent r a t i o n f o r t h e a n t i b i o t i c as r e p o r t e d by t h e respective authors. O f t h e organisms t a b u l a t e d overl e a f K.pneumaniae i s g e n e r a l l y used f o r r o u t i n e assays.
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Table 1 7 C o n d i t i o n s of T u r b i d i m e t r i c Assay Organism
---
S.auheub NRRLB314 II II 209P 11
11
F1
s t h epzo cu cc U b
daecalib ATCC 1054 K l e bb i e l l a pneumaniae PC1602 Klebbiella pneumo n i a e
ATCC 10031
E.coli ATCC 10536 II
II
ATCC 11105
Lacto b a c i l l u b ahabino zua La c t o ba c i l l ub cab ei Lacto b a c i l l u a dehmenti L a c t u ba c i l l u n L eic hm a n n i Aeho b a c t e h aehogeneb I P L 22K5118
C o n c e n t r a t i o n Range of Assay ( T o t a l pg neomycin base required i n s o l u t i o n t o be assayed) 2.5 5.0
-
Reference
2 41
100-300
242
-
243
0.016
0.04
120-200
2 48
6-15
244
6-14
245 I 246 I 268
1- 3
247
1-20
253
3-7
2 48
20-60
248
2-6
248
4-6
248
0-6
249
H e i n 2 4 3 n o t e d an a p p a r e n t d e c r e a s e i n t h e p o t e n c y of neomycin when a s s a y e d t u r b i d i m e t r i c a l l y i f t h e i n n o c u l u m c o n t a i n e d e i t h e r sodium c h l o r i d e o r p o t a s s i u m phos h a t e . With S.auheub a s o r g a n i s m l S o k o l s k i e t a 125!? d e m o n s t r a t e d t h e p r e s e n c e of K C 1 t o a n t a g o n i s e t h e a c t i v i t y of neomycin C more t h a n t h a t of neomycin B.
WILLIAM F. HEYES
A c o m p a r a t i v e s t u d y o f t h e responce o f neomycin B and neomycin C i n t h e t u r b i d i metric a s s a y u s i n g K . pneumakziae (ATCC 10031) h a s been r e p o r t e d 2 3 9 . The r e s p o n s e - r a t i o neomycin B: neomycin C w a s 100:38.9. An a u t o m a t e d t u r b i d i m e t r i c p r o c e d u r e u s i n g a T e c h n i c o n A u t o a n a l y z e r h a s a l s o been d e s c r i b e d (See S e c t i o n 6.5)
.
6.42.Agar-Diffusion
Assay
T a b l e 18 l i s t s t h e o r g a n i s m s t h a t have been recommended f o r d e t e r m i n i n g t h e microb i o l o g i c a l p o t e n c y o f neomycin. T a ble 18 Recommended Organ i s m
Working Concentration (P g h l )
8. p u m i l i n
Reference
4-2 1
9
4-20
245
NCTC 8241
.
S aua eun ATCC 6538
.
S e p i d ekmidics ATCC 12228
0.64
-
1.56
245,268
I n a l l t h e above r e f e r e n c e s , t h e c y l i n d e r - p l a t e a s s a y p r o c e d u r e i s t h e one d e s c r i b e d though a l t e r n a t i v e p r o c e d u r e s have been r e p o r t e d i n t h e l i t e r a t u r e . Thus Davis and P a r k e 2 4 5 r e p o r t e d a l i n e a r - d i f f u s i o n s y s t e m i n which a s o l u t i o n o f t h e a n t i b i o t i c i s allowed t o d i f f u s e i n t o a g a r - f i l l e d The s t a n d a r d d e v i a t i o n s c a l glass capilliaries c u l a t e d f o r s e v e n e x p e r i m e n t s w e r e between 5 and 10&(100 r e s u l t s ) f o r t h e a s s a y o f neomycin. The p r o c e d u r e i s more economic i n t e r m s o f a g a r and n u t r i e n t s t h a n o t h e r d i f f u s i o n methods. K u z e l and Coffey255 m o d i f i e d t h e c o n v e n t i o n a l c y l i n d e r p l a t e p r o c e d u r e by u s i n g a c y l i n d e r s e a l e d a t one e n d , f o r m i n g a c u p . The c u p s are f i l l e d w i t h t h e a n t i b i o t i c s o l u t i o n s t o b e a s s a y e d , t h e n a p l a t e of i n o c u l a t e d a g a r i s i n v e r t e d and p l a c e d over t h e t o p of t h e c u p s . With t h i s method a s i g n i f i c a n t r e d u c t i o n i n t h e s t a n d a r d d e v i a t i o n f o r t h e a s s a y o f neomycin
.
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w a s c l a i m e d . The r e p l a c e m e n t o f c l i n d e r s by a e r 47Y d i s c s h a s a l s o been r e p o r t e d 2561275,278. ~~~~i claimed a standard d e v i a t i o n of 2% f o r the assay of neomycin by t h i s means and recommended t h e p a p e r d i s c p r o c e d u r e i n p r e f e r e n c e t o t h e c y l i n d e r method. The t y p e of p a p e r u s e d h a s been shown t o a f f e c t t h e ~~~ seed d i a m e t e r of t h e i n h i b i t i ~ n - z o n eWhatman t e s t p a p e r p r o d u c i n g t h e s m a l l e s t z o n e s . When d e t e r m i n i n g neomycin l e v e l s i n m i l k , K o s i k ~ w s k i ~ ~ ~ improved t h e s e n s i t i v i t y o f t h e p r o c e d u r e by s u b s t i t u t i n g d r i e d milk t a b l e t s f o r paper d i s c s . S e v e r a l s t u d i e s of t h e f a c t o r s a f f e c t i n g t h e i n h i b i t i o n - z o n e s i z e i n t h e neomycin a g a r d i f f u s i o n a s s a y have been r e p o r t e d . P i n z e l i k e t a1257 d e m o n s t r a t e d t h a t v a r i o u s d e l a y s d u r i n g t h e a n a l y t i c a l procedure a f f e c t e d t h e s i z e of t h e i n h i b i t i o n zone. Refrigeration of t h e agar-plates p r i o r t o i n c u b a t i o n c a u s e d an i n c r e a s e i n zones i z e when compared w i t h s i m i l a r p l a t e s h e l d a t 2OoC. T h i s p r i n c i p l e h a s been u t i l i z e d by S i d d i q u e e t a1264 t o improve s e n s i t i v i t y when d e t e r m i n i n g t h e neomycin c o n t e n t o f m i l k . The p r e s e n c e o f K C l , N a C l , C a C 1 2 h a s been shown t o m a r k e d l y i n c r e a s e neomycin d i f f u s i o n i n a g a r 2 5 8 , 2 6 5 194. C o n v e r s e l y t h e p r e f p h o s p h a t e s 2 5 8 and of g l u c o s e / s t a r c h w i t h NaCl d e c r e a s e s t h e s i z e of t h e i n h i b i t i o n z o n e . I n c o r p o r a t i o n of non- f at milk i n t h e a g a r s i g n i f i c a n t l y r e d u c e s t h e s i z e o f t h e i n h i b i t i o n z o n e bec a u s e o f t h e i n t e r a c t i o n o f neom c i n w i t h t h e f r e e c a r b o x 1 g r o u p of m i l k p r o t e i n 2 6 3 F e d o r k o and K a t z 2 6 3 d i l u t e d neomycin s o l u t i o n s w i t h b l o o d serum and r e p o r t e d an i n c r e a s e i n t h e s i z e o f t h e i n h i b i t i o n zone when compared w i t h s i m i l a r s o l u t i o n s d i l u t e d w i t h pH 8 phos h a t e b u f f e r . S o k o l s k i e t a1252 and Yousef e t a1559 d e m o n s t r a t e d t h e p h y s i c a l b i n d i n g o f neomycin t o a g a r , a p r o c e s s which may be r e v e r s e d by a d d i t i o n o f o t a s s i u m o r sodium c h l o r i d e . F u r t h e r s t u d i e s 2 6 0 t 5 6 1 , 2 5 2 have r e p o r t e d t h e b i n d i n g t o be a f u n c t i o n o f b o t h t h e p H o f t h e a g a r and t h e m a n u f a c t u r e r . I n c o r p o r a t i o n o f 0.1M t r i s b u f f e r w i t h t h e a g a r (pH 8 ) h a s b e e n recommende d 2 6 0 , 261 i n o r d e r t o a c h i e v e t h e h i g h e s t s e n s i tivity. T r i s buffer results in a greater sensitivi t y t h a n p h o s p h a t e b u f f e r 2 6 1 and d o e s n o t a f f e c t t h e s i z e o f t h e i n h i b i t i o n zone w h e r e a s t h e p r e sence o f p h o s p h a t e r e d u c e s zone s i z e 2 5 2 . G i l l e t e t , 1 1 9 4 c o n c l u d e d t h a t t h e q u a l i t y of t h e a g a r a f f e c -
.
WILLIAM F. HEYES
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t e d t h e i n h i b i t i o n zone s i z e . A comparison of 3 a g a r s showed t h e b e s t response f o r a g i v e n concent r a t i o n of neomycin w a s o b t a i n e d w i t h agarose.Comb i n i n g a g a r o s e w i t h recommendations d e s c r i b e d by o t h e r a u t h o r s , such a s t h e a d d i t i o n of C a C l and t h e use of t r i s b u f f e r , f u r t h e r i n c r e a s e d tge s i z e of t h e i n h i b i t i o n zone. The l i t e r a t u r e d e s c r i b e d above r e f e r s t o t h e a s s a y of t h e t o t a l neomycin complex i . e . neomycins B and C and neamine. To a s s a y neomycin B i n t h e p r e s e n c e of neomycin C and neamine by a m i c r o b i a l method S o k o l s k i and Carpenter265 adopted t h e f o l l o w i n g p r o c e d u r e . These a u t h o r s e m ployed a neomycin C - r e s i s t a n t organism (8.b u b i i l i b UC 564) and added K C 1 t o t h e a g a r t o t o t a l l y dep r e s s d i f f u s i o n of neamine and i n c r e a s e d i f f u s i o n of neomycin B . Neomycin B and C d i f f e r i n t h e i r b i o l o g i c a l a c t i v i t i e s though t h i s d i f f e r e n c e may v a r y w i t h t h e c o n d i t i o n s of t h e a s s a y . T y p i c a l l y neomycin C h a s an a c t i v i t y of 30-50% of t h a t of The p r e s e n c e of potassium c h l o neomycin B 2 6 6 r 2 3 9 . r i d e o r phosphate r e d u c e s t h e d i f f u s i o n of neomycin C more t h a n t h a t o f neomycin B252. Furthermore, t h i s a n t a g o n i s t i c e f f e c t of t h e s a l t s h a s been shown t o be more pronounced when u s i n g S . U U t r e U b a s organism than when u s i n g B.bubiilib. By a l t e r i n g t h e i o n i c s t r e n g t h o f t h e medium a system h a s been developed i n which t h e r e s p o n s e s of neomycins B and C a r e i d e n t i c a l 2 6 6 . The m i c r o b i a l assay of neomycin i n t h e p r e s e n c e of o t h e r a n t i b i o t i c s can p r e s e n t d i f f i c u l t i e s i f b o t h a n t i b i o t i c s are a c t i v e a g a i n s t t h e same t e s t organisms. The a s s a y o f neomycin i n t h e p r e s e n c e of d i h y d r o s t r e p t o m y c i n , t o which t h e t e s t organism S . U U t r e U b i s a l s o s e n s i t i v e , h a s been Levine e t a 1 2 6 9 r e n d e r e d t h e d i h y d r o reported. s t r e p t o m y c i n i n a c t i v e by h y d r o l y s i s w i t h barium hydroxide p r i o r t o t e r m i n i n g neomycin w i t h S. UUfLeUb DeNuzio 2% however, chose t o overcome t h e same problem by c u l t i v a t i n g a s t r a i n of S.uutreub which was r e s i s t a n t t o d i h y d r o s t r e p t o mycin. When a s s a y i n g neomycin i n a m i x t u r e cont a i n i n g t e t r a c y c l i n e , e n i c i l l i n and d i h y d r o s t r e p t omycin, Tanguay e t a12T1 found i t n e c e s s a r y t o
.
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s e p a r a t e t e t r a c y c l i n e and p e n i c i l l i n by s o l v e n t ext r a c t i o n b e f o r e d e t e r m i n i n g neomycin by t h e method of DeNuzio. The d e t e r m i n a t i o n of neomycin i n animal f e e d s h a s r e c e i v e d much a t t e n t i o n . B a r b i e r s and Neff272 recommended t h e u s e of a t r i s b u f f e r a t pH 8 t o p r e p a r e neomycin s o l u t i o n s and t h e a d d i t i o n of magnesium o r calcium c h l o r i d e t o t h e a g a r f o r enhancement of t h e i n h i b i t i o n zones. E x t r a c t i o n of neomycin from t h e f e e d r e q u i r e d t h e u s e of sodium c h l o r i d e s o l u t i o n f o r 100%r e c o v e r y . A c o l l a b o r a t i v e s t u d y of t h i s procedure by e i g h t e e n l a b o r a t o r i e s r e s u l t e d i n an average r e c o v e r y of 100.3% w i t h a c o e f f i c i e n t of v a r i a t i o n of 15.2%279. Modif i c a t i o n of t h e p r e v i o u s method h a s been d e s c r i b e d by Williams and Wornick273 who i n c o r p o r a t e d t h e t r i s b u f f e r i n t h e a g a r and d e l e t e d t h e a d d i t i o n of calcium c h l o r i d e . A t h r e e - f o l d i n c r e a s e i n s e n s i t i v i t y was r e p o r t e d . However, a c o l l a b o r a t i v e s t u d y of t h e modified procedure r e s u l t e d i n an ave r a g e r e c o v e r of 1 1 5 % w i t h a c o e f f i c i e n t of v a r i a t i o n of 20.4%3 7 4
.
An i n v e s t i g a t i o n of t h e a g a r d i f f u s i o n a s s a y of neomycin a t v e r y low l e v e l s ( 5 0 n g 1000ng) i n meat p r o d u c t s h a s been r e p o r t e d 2 8 0 . The p o i n t s on t h e dose-response graph c o v e r i n g t h e above c o n c e n t r a t i o n range w e r e s c a t t e r e d about t h e a v e r age s t r a i g h t l i n e . However, by j o i n i n g a l l t h e p o i n t s t o g e t h e r a complex c u r v e r e s u l t e d , t h e equat i o n of which was d e r i v e d .
6.5.
Automated Procedures
An a t t e m p t t o automate t h e t u r b i d i metric method f o r t h e d e t e r m i n a t i o n of neomycin w i t h K.pneurnaniae has been r e p o r t e d by Gerke e t a1281 who o b t a i n e d s a t i s f a c t o r y a s s a y s w i t h s o l An u t i o n s c o n t a i n i n g 150-1200 pg/ml of neomycin. automated r e s p i r o m e t r i c method, which measured t h e amount of C 0 2 produced by i n t e r a c t i o n of a n t i b i o t i c and t h e b a c t e r i a E.cali w a s a l s o r e p o r t e d w i t h a similar sensitivity. I n b o t h methods Auto Analyzer systems were employed.
The m o d i f i c a t i o n of t h e above r e s p i r o m e t r i c procedure t o i n c l u d e c o n t i n u o u s c u l t u r e of
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t h e t e s t o r g a n i s m E . c o L i h a s been d e s c r i b e d 2 8 2 . With t h e o r g a n i s m grown i n t h i s manner t h e s e n s i t i v i t y o f t h e a s s a y i s improved. G r e e l y e t a1283 have a p p l i e d t h e automated r e s p i r o m e t r i c method t o t h e d e t e r m i n a t i o n o f neomycin i n p h a r m a c e u t i c a l p r o d u c t s and compared t h e s e a s s a y s w i t h t h e r e s u l t s o b t a i n e d by t h e c y l i n d e r - p l a t e p r o c e d u r e on t h e same s a m p l e s . Good c o r r e l a t i o n between t h e t w o p r o c e d u r e s was d e m o n s t r a t e d . A n automated c o l o r i m e t r i c a s s a y f o r t h e q u a n t i t a t i o n of t h e s e p a r a t e components o f neom c i n ( B , C and neamine) h a s a l s o been r e p o r t The method u t i l i z e s a s e p a r a t i o n o f t h e ed148. components on a column o f c a r b o n and K i e s l g u h r G (4:l). The column e l u a t e i s reacted w i t h n i n h y d r i n t o d e t e r m i n e t h e amounts o f neomycin B , C and neamine.
6.6.
U s e as a n A n a l y t i c a l Reagent
Turbidimetric procedures f o r d e t e r mining r i b o n u c lease2 and d e o x y r i b o n u c l e a s e 85 u s i n g neomycin as t h e p r e c i p i t a n t h a v e been d e s c r i bed. The t u r b i d i t y w a s shown t o b e d e p e n d a n t on t h e r e l a t i v e c o n c e n t r a t i o n s o f r e a c t a n t s , t h e molec u l a r w e i g h t o f t h e RNA o r DNA and t h e i o n i c s t r e n g t h of t h e s o l u t i o n t h u s n e c e s s i t a t i n g t h e c a r e f u l c o n t r o l of assay conditions. Extraneous p r o t e i n s do n o t i n t e r f e r e e n a b l i n g t h e p r o c e d u r e t o be a p p l i e d d i r e c t l y t o blood serum. 6.7.
D e t e r m i n a t i o n i n Body F l u i d s and Tissues
An a g a r d i f f u s i o n a s s a y , based upon t h e method d e s c r i b e d by Groves and Randa11246, h a s been u t i l i s e d by t h e m a j o r i t y of w o r k e r s f o r det e r m i n i n g neomycin l e v e l s i n c l i n i c a l samples. T o compensate f o r t h e p r o t e i n - b i n d i n g e f f e c t e x h i b i t ed by neomycin, Kivman and Geitman309 recommended t h e a d d i t i o n of serum and 3 % KC1 t o t h e neomycin s t a n d a r d s o l u t i o n . D a n i e l ~ v a ~however, ~ ~ , pref e r r e d t o release t h e bound a n t i b i o t i c by enzymat i c h y d r o l y s i s p r i o r t o m i c r o b i o l o g i c a l a s s a y . An a g a r d i f f u s i o n method r e q u i r i n g o n l y 2 0 ~ 1o f serum sample h a s been d e s c r i b e d by A x l i n e e t a1311.
NEOMYCIN
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The a p p l i c a t i o n of a t u r b i d i m e t r i c method t o t h e e x a m i n a t i o n o f s e r u m s a m p l e s h a s been r e p o r t e d by Fe l s e n f e l d 3 l 2 . More r e c e n t l y a laser l i g h t s c a t t e r i n g b i o a s s a y f o r d e t e r m i n i n g t h e neomycin c o n t e n t of m i l k , s e r u m , u r i n e and b i l e h a s been r e p o r t e d 3 1 3 . The p r o c e d u r e u s e s a helium-neon l a s e r l i g h t s o u r c e and h a s a l i n e a r d o s e - r e s p o n s e g r a p h over t h e r a n g e 0.1 t o 1 0 u g / m l f o r serum. A n enzymic a s s a y i n v o l v i n g t h e r e a c t i o n of neomycin w i t h a m i n o g l y c o s i d e 4 ' a d e n y l t r a n s f e r a s e h a s b e e n d e s c r i b e d 3 1 4 . A l i n e a r r e s p o n s e f o r neomycin w a s o b s e r v e d over t h e r a n g e 2.5 t o 2Oug/ml serum.
The c o n c e n t r a t i o n of neomycin i n u r i n e h a s been d e t e r m i n e d w i t h a f l u o r i m e t r i c method315. I n t e r f e r i n g amines w e r e s e p a r a t e d by c h r o m a t o g r a p h y on SE Sephadex C-25 b e f o r e r e a c t i n g t h e i s o l a t e d neomycin w i t h f l u o r e s c a m i n e
.
B r a m m e r and Hemson182 employed a n e l e c t r o p h o r e t i c p r o c e d u r e t o s e p a r a t e neomycin from b l o o d - p r o t e i n s b e f o r e d e t e r m i n i n g t h e neomycin c o n c e n t r a t i o n c o l o r i m e t r i c a1l y
.
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Waksman S.A. a n d L e c h e v a l i e r H . A . , U.S. P a t e n t 2,799,620 (1957). Umezawa H . , T a k e u c h i T. a n d Yamagiwa S . , J a p a n . Med. J . , 3 , 25-30 ( 1 9 5 0 ) . A r a i T. a n d A i i s o K . , J a p a n e s e P a t e n t 5450 (1953). Game G.F., K o c h e t k o v a G . V . , P r o b r a z e n s k a y a T.P. a n d P e v z n e r N.S., A n t i b i o t i k i , 1 (51, 4-8 ( 1 9 5 6 ) . J a c k s o n F.L., K i t t i n g e r G.W. and K r a u s e F.P. , N u c l e o n i c s , 18 ( 8 ) ,102-5 ( 1 9 6 0 ) . S w a r t E.A. , H u t c h i n s o n D . a n d Waksman S.A. , A r c h . Biochem., 24, 92-103 ( 1 9 4 9 ) . L e a c h B.E., D e V r i e s W . H . , N e l s o n H.A., J a c k s o n W.G. a n d E v a n s J . S . , J.Am.Chem.Soc., 7 3 I 2797-2800 ( 1 9 5 0 ) Makino S. , H a y a s h i E . a n d Okamura K . , J a p a n . P a t e n t 6247 ( 1 9 6 0 ) . T a k e n a g a M. a n d Okada Am, G e r . P a t e n t 2,165,373 (1972). T a n a k a I . , Yoshizawa H., O t a n i S., N a k a y a s h i k i J. a n d Hara E . ,Y a k u z a i g a k u , 2 2 , 147-50 ( 1 9 6 2 ) . Simone R.M. a n d P o p i n o R.P., J.Am.Pharm. A S ~ O C .I 44, 275-80 ( 1 9 5 5 ) . Beyd A . , J . P h a r m . S c i . , 60 ( 9 ) ,1343-5 (1971). Gecgil S . , I s t a n b u l U n i v . E c z a c i l i k F a k . Mecmuasi , 2 (1),56-57 ( 1 9 6 8 ) Coates L . V T , P a s h l e y M.M. a n d T a t t e r s a l l K . , J.Pharm.Pharmaco1. , 13, 6 2 0 - 4 ( 1 9 6 1 ) . D a l e J . K . a n d Rundman S. J . , J.Am.Pharm. ASSOC., P r a c t . Pharm. E d . , 1 8 , 4 2 1 - 5 ( 1 9 5 7 ) . K u d a l k a r V.G., H a l l N . A . a n d R i s i n g L.W. , Am.J.Pharm., 1 3 1 , 166-73 ( 1 9 5 9 ) . M c G i n i t y J . W . a n d Brown R.L., J . P h a r m . S c i . , 64 ( 9 ) ,1528-30 ( 1 9 7 5 ) . E r n i c k R.C., P r o c . , Annu. P f i z e r R e s . C o n f . , 1 5 t h , 54-90 1 1 9 6 7 ) . Danti A . G . a n d G u t h E . P . , J.Am.Pharm.Assoc., S c i . E d . , 4 6 , 249-52 ( 1 9 5 7 ) . Hammouda Y T a n d S a l a k a w y S.A., P h a r m a z i e , 26 (10), 636-40 ( 1 9 7 1 ) . F l o r e s t a n o H . J . , B a h l e r M.E. a n d J e f f r i e s S . F . , J.Am.Pharm.Assoc. , 4 5 , 538-41 ( 1 9 5 6 ) . Kivman G. Y a . a n d G e i t m a n I. Y a . , A n t i b i o t i k i , 16 ( 4 ) ,331-5 ( 1 9 7 1 ) .
.
.
WILLIAM F. HEYES
488
310. 311. 312. 313. 314. 315.
D a n i e l o v a L . T . , A n t i b i o t i k i , 1 9 (111, 1032-8 ( 1 9 7 4 ) . Axline S.G., Yaffe S . J . a n d Simon H . J . , P e d i a t r i c s , 39 ( 1 ) , 9 7 - 1 0 7 ( 1 9 6 7 ) . F e l s e n f e l d O . , V o l i n i I . F . , K a d i s o n E.R., Zimmermann E . a n d I s h i h a r a S . J . , Am.J. Clin.Path., 3 , 670-1 (1950). Wyatt P . J . , P h i l l i p s D . T . and A l l e n E . H . , J . A g r i c . F o o d Chem., 24 ( 5 ) ,984-8 ( 1 9 7 6 ) . Santanam P . a n d K a y s e r F.H., A n t i m i c r o b . A g e n t s C h e m o t h e r . , lo ( 4 ) ,664-7 ( 1 9 7 6 ) . K u s n i r J . a n d B a r n a K . , Cesk. Farm., 24 ( 6 ) ,253-5 ( 1 9 7 6 )
This p r o f i l e attempts t o cover t h e published l i t e r a t u r e on neomycin u p t o a n d i n c l u d i n g C h e m i c a l Abstracts, Volume 8 5 .
Analytical Profiles of Drug Substances, 8
PSEUDOEPHEDRINE HYDROCHLORIDE Steven A . Benezra and John W . McRae 1.
2.
3. 4. 5. 6.
Description 1.1 Name, Formula, Molecular Weight 1.2 Appearance, Color, Odor Physical Properties 2. I Infrared Spectrum 2.2 Nuclear Magnetic Resonance Spectrum 2.3 Ultraviolet Spectrum 2.4 Mass Spectrum 2.5 Melting Point 2.6 Specific Rotation 2.7 Solubility 2.8 Partition Coefficient 2.9 Differential Scanning Calorimetry 2.10 Crystal Structure 2.1 I Dissociation Constant Synthesis Stability Metabolism and Pharmacokinetics Methods of Analysis 6.1 Elemental Analysis 6.2 Nonaqueous Titration 6.3 Ultraviolet Spectrophotometric Analysis 6.4 Colorimetric Analysis 6.5 Chromatography 6.51 High Performance Liquid Chromatography 6.52 Thin-Layer Chromatography 6.53 Paper Chromatography 6.54 Gas Chromatography
489
Copyright @ 1979 by Academic Press, Inc. All rights of reproduction in any form reserved. ISBN 0-12-260808-9
490
1.
STEVEN A . BENEZRA AND
JOHN W. MCRAE
Description
1.1 Name, Formula, Molecular Weight d-Pseudoephedrine hydrochloride is (+)-threo-a-(1(methy1amino)ethyl)benzyl alcohol hydrochloride. Throughout this analytical profile, d-pseudoephedrine will be referred to as pseudoephedrine.
*o
C10H15NO*HC1
H
0
HCI
I
CH3
201.72
1.2 Appearance, Color, Odor Pseudoephedrine hydrochloride occurs as fine white t o off-white crystals o r as a powder having a faint odor1
2.
Physical Properties
2.1 Infrared Spectrum The infrared spectrum of pseudoephedrine hydrochloride is shown in Figure 1. It was obtained as a 0.2% dispersion of pseudoephedrine hydrochloride in KBr with a Nicolet Model 7199 FT-IR spectrophotometer.2 Table I gives the infrared assignments consistent with the structure of pseudoephedrine hydrochloride. Table I Infrared Spectral Assignments for Pseudoephedrine Hydrochloride Frequency (cm-l) Assignment OH stretch 3270 3010 Asym. C-H stretch
1
0
0
1
1
8
1
I
3
I
I
0 d
1
0 (u
STEVEN A. BENEZRA AND
492
Sym. C-H stretch
2930
+NH
2700
stretch
C=C aromatic stretch OH bend, secondary alcohol C-H bend, monosubst. benzene
1587, 1490 1430 762, 702 2.2
JOHNW. MCRAE
Nuclear Magnetic Resonance (NMR) Spectrum The NMR spectrum o f pseudoephedrine hydrochloride
is shown in Figure 2.
The spectrum was obtained with a
Varian model CFT-20 80 MHz NMR spectrometer. Deuterated DMSO was used as the solvent with tetramethylsilane as an internal standard. Table I1 gives the NMR assignments consistent with the structure of pseudoephedrine hydrochloride.
G9
8 H H HN-
OH H
@@
Table I1
NMR Assignments for Pseudoephedrine Hydrochloride Proton a
No. of Protons 3
Shift (ppm) 0.96
Multiplicity doublet
b
3
2.55
singlet
C
1
3.25
quartet (partially obscured by H20)
d
1
e
1
f
5
8
2
4.54 6.32 7.34 8.90
doublet of doublets doublet singlet broad singlet
493
PSEUDOEPHEDRINE HYDROCHLORIDE
J
1
1
I
8
9
7
6
5
4
3
S
I
2
'
I
!
I
1
I
1
I'
0
PPm
Figure 2
-
NMR Spectrum of Pseudoephedrine Hydrochloride
I.o
ae
0.6 U
4 [L
v 0 )
a 0.4
0.2
0.9
Figure 3
-
nrn
Ultraviolet Spectrum of Pseudoephedrine Hydrochloride
STEVEN A. BENEZRA A N D
494
JOHN W. MCRAE
2.3 Ultraviolet Spectrum The ultraviolet spectrum of pseudoephedrine hydrochloride in ethanol was obtained with a Beckman ACTA CIII ultraviolet spectrophotometer and is shown in Figure 3. Pseudoephedrine hydrochloride exhibits absorption maxima at 208, 251, 257, and 264 nm with extinction coefficients of 8300, 161, 201, and 161, respectively. 2.4. Mass Spectrum The low resolution mass spectrum of pseudoephedrine hydrochloride is shown in Figure 4.5 It was obtained with a Varian MAT CH5-DF mass spectrometer. Direct probe at 80'C into the ion source was used to obtain the mass spectrum. The electron energy was 70 eV. The assignments of the major ions formed in the mass spectrometer are shown below.
The
molecular ion is not observed.
H +HC/NzCH3 'CHq3 m/e 58 (100%) 2.5
0 +
m/e 77 (9%)
HCI
m/e 36 (10%)
+
HNCH3
m/e 30 (12%)
Melting Point Pseudoephedrine hydrochloride melts between 182'
and 185'C.
2.5 Specific Rotation The specific rotation, of d-pseudoephedrine hydrochloride in water is between +61.0' and +62.5'.l
[cy]iO,
2.7
Solubility The solubility of pseudoephedrine hydrochloride in
495
PSEUDOEPHEDRINE HYDROCHLORIDE
1001
I50
I00
200
m /e
Figure 4
1 I
178
-
Mass Spectrum of Pseudoephedrine Hydrochloride
1
1
1
180
179
I
181
I
I
182
1 1
183
TEMPERATURE
Figure 5
-
1
i
184
I
1
185
1 1
186
1 1
187
OC
DSC Curve of Pseudoephedrine Hydrochloride
STEVEN A. BENEZRA AND JOHN W. MCRAE
496
various solvents at 25OC is given in Table 111.' Table I11 Solubility of Pseudoephedrine Hydrochloride at 25OC Solvent
Solubility (gm/ml)
Water
2.0
Chloroform
0.011
E thano1
0.278
Ether
1.4
2.8 Partition Coefficient The partition coefficients of pseudoephedrine hydrochloride at 25OC in n-octanol/aq. pH 1.2 and n-octanol/ aq. pH 6.0 are 0.010 and 0.049 respectively.6 2.9 Differential Scanning Calorimetry (DSC) The DSC curve of pseudoephedrine hydrochloride obtained with a Perkin Elmer DSC-1B differential scanning calorimeter is shown in Figure 5 . ?
The heating rate was
5OC/min. The heat of fusion is 6.4 Kcal/mol. The melting point (uncorrected) is 184OC. 2.10 Crystal Structure The crystal properties of pseudoephedrine hydrochloride were determined with a GE model XRD-6 x-ray diffractometer using Zr filtered MoKa radiation on a crystal grown from water.
Pseudoephedrine hydrochloride has an ortho-
rhombic crystal system belonging to the P2 2 2 space group. 0 l a 1 0 The cell dimensions are a=25.358 A , bz6.428 A , ~ ~ 6 . 9 0A1 with each cell containing four molecules. 2.11 Dissociation Constant The pKa of pseudoephedrine hydrochloride determined
PSEUDOEPHEDRINE HYDROCHLORIDE
491
titrimetrically in 80% aqueous methylcellosolve is 9.22. 3.
Synthesis Pseudoephedrine hydrochloride is prepared by a
Welsh rearrangementl o of R-ephedrine hydrochloride with acetic anhydride followed by deacetylation with hydrochloric acid. l 1
2-Ephedrine can be resolved from dR-ephedrine with
2-mandelic acid. l2
R-Ephedrine occurs naturally in certain
plants of the Ma Huang species. 4.
Stability Pseudoephedrine hydrochloride can be considered a
stable compound in bulk and in formulations. After 4-weeks under fluorescent lights (2400 ft. candles) and ultraviolet light (190 pw/cm2) no discoloration or chemical degradation was observed. The bulk drug was stable for at least 6 months at 37OC and 3 months at 5OoC. Tablet and syrup formulations stored at 15-30°C for 5 years showed no appreciable degradation. l 3
5.
Metabolism and Pharmacokinetics The major biotransformations of pseudoephedrine
hydrochloride are parahydroxylation, N-demethylation, and oxidative deamination. l4
The proposed pathways for the
metabolism of pseudoephedrine are shown in Figure 6 . In a study with human subjects, whose urine pH was controlled with sodium bicarbonate and ammonium chloride, it was found that 10-25% of the administered pseudoephedrine hydrochloride was metabolized to norpseudoephedrine and the elimination of pseudoephedrine and norpseudoephedrine was related to urine pH.
As the urine pH increased, the serum
half-life o f pseudoephedrine and norpseudoephedrine increased.15
In another similar study it was found that a decrease
H
CH3
p-&-H++-Q OH NH
\ I
I
CH3 Pseudoephedr ine
OH NH, Nor pseudoephedrine
o + ( / OH
I/
CH3
I-Hydroxy-l-phenyl-2-proponone
OW,H OH OH
I -Phenyl-l,Z-propanediol
OH Benzoic acid Figure 6
-
Metabolism of Pseudoephedrine Hydrochloride
PSEUDOEPHEDRINE HYDROCHLORIDE
499
in urine pH caused a decrease in plasma half-life of pseudoephedrine. l6
Plasma half-lives measured in normal human
subjects were 5 . 2 - 8 . 0 hours.l6 In a rat study using 14C-labelled dQ-ephedrine, 85% of the i.p.-administered drug was eliminated in the first 40 hours.
Two major metabolic pathways were postulated after
analysis of the metabolites. The major metabolic pathway was ring para-hydroxylation forming para-hydroxyephedrine and para-hydroxynorephedrine.
The minor metabolic pathway was
oxidative deamination, giving acidic metabolites such as hippuric and benzoic acids. l7 The relative tissue distribution in mice 15 minutes after i.v.-administered l4C2ephedrine was kidney > lung, adrenal, spleen, liver > intestines, stomach > brain, heart > plasma. l7 The LDs0 in mice o f pseudoephedrine administered i.p. is 1.0 mmole/kg.18 6.
Methods of Analysis Elemental Analysis
6.1
The results of the elemental analysis o f pseudoephedrine hydrochloride are given in Table IV.6 The analysis was performed on a NF Reference Standard. Table IV Elemental Analysis of Pseudoephedrine Hydrochloride Element
Theory (%)
Found ( X )
C
59.55
59.54
H
8.00
8.11
N
6.95
6.81
STEVEN A. BENEZRA AND
500
6.2
JOHN W.M C W E
Nonaqueous Titration Pseudoephedrine hydrochloride is dissolved in a
mixture of glacial acetic acid and mercuric acetate test solution. A standardized solution of 0 . 1 N perchloric acid is used to titrate the solution to a blue-green end point with crystal violet indicator. Each ml of 0.1N perchloric acid is equivalent to 0.1 mmole of pseudoephedrine hydrochloride. 6.3
Ultraviolet Spectrophotometric Analysis An ultraviolet spectrophotometric analysis is used
to assay pseudoephedrine hydrochloride in tablets. A portion of finely powdered tablets equivalent to approximately 30 mg of pseudoephedrine hydrochloride is placed in a distilling flask which is part of a micro-steam distillation apparatus. Sodium chloride, water, and concentrated sodium hydroxide are added. A minimum of 30 ml of distillate is collected in a volumetric flask containing dilute hydrochloric acid.
The
flask is made to volume with distilled water and the absorbance of the solution is determined at 257 nm in 1 cm cells and compared to a solution of known concentration of NF Pseudoephedrine Hydrochloride Reference Standard. An ultraviolet spectrophotometric method based on the absorbance of a periodate oxidation product o f pseudoephedrine hydrochloride will be the official method of analysis in the USP XX.19,20 A portion of tablets or syrup in water is placed in a separatory funne.1. Sodium bicarbonate and sodium metaperiodate are added. After standing for 15 minutes, 1 N HC1 is added. The solution is extracted with hexane. The hexane extract is filtered and its absorbance determined at 242 nm in 1 cm cells. The amount of the oxidation product of pseudoephedrine hydrochloride is determined by comparison of the sample absorbance against the absorbance of a Pseudoephedrine Hydrochloride Reference Standard treated in the same manner.
50 1
PSEUDOEPHEDRINE HYDROCHLORIDE
6.4 Colorimetric Analysis Pseudoephedrine hydrochloride in syrup formulations has been analyzed by colorimetry. Pseudoephedrine forms a stable blue-colored chelate with cupric sulfate at pH 12.5. The complex has a maximum absorbance at 500 nm. The complex is extracted from an aqueous layer with 1-pentanol. Interfering substances such as glycerine and sugars normally found in syrup formulations, which form complexes with cupric aulfate, are not extracted into l-pentanol.*l 6.5
Chromatography 6.51 High Performance Liquid Chromatography (HPLC) High performance liquid chromatography has been
used to analyze pseudoephedrine hydrochloride and dosage forms containing pseudoephedrine hydrochloride.
Table V
gives the HPLC conditions used for separations. Table V HPLC Conditions €or Pseudoephedrine Hydrochloride Column Corasil@/Phenyl
Mobile Phase Rention Time (min) 1.8 (phenyl) acetonitrile:
Corasil@/C18
0.1% ammonium
Reference 22
1.9 (C18)
carbonate (9:l) pH 8.9
Corasil@/Phenyl Corasil@/C18
acetonitrile: 1% ammonium
carbonate (6:4) pH 7.4
22
STEVEN A. BENEZRA AND JOHN W.M C M E
502
Zipax@/SCX
0.02 M dibasic ammonium phosphate:dioxane
7
23
6
24
8
25
(64:36) Nucleosil@/
methanol:0.5M
silica gel
sodium dihydrogen phosphate: phosphoric acid (195:50:2)
Spherisorb@/
ethanol:0.4%
silica gel
ammonium acetate (85: 15)
6.52 Thin Layer Chromatography (TLC) Table VI lists the various TLC systems used for pseudoephedrine hydrochloride. Table VI TLC Systems for Pseudoephedrine Hydrochloride
Rf
Reference
silica gel
0.25
26
silica gel
0.46
Mobile Phase
Adsorbent
ethyl acetate: cyclohexane: methano1:conc. M140H(70:15:10:5) n-butano1:ethanol: water:acetic acid (60:30:10:0.2)
27 0.18 (free base)
503
PSEUDOEPHEDRINE HYDROCHLORIDE
chlorof o rni:
silica gel
0.33
28
methanol : acetone (7:3:5) ethyl ether:
0.10 (free base) silica gel
benzene (1:l)
0.35 (as 4-chloro-
29
7-nitrobenzo-2,1,3oxadiazole derivative) chloroform :
alumina
0.70 (as
water:acetic
acetylated
acid (20:75:20:1)
product)
16
(lower phase) 6.53 Paper Chromatography Paper chromatography has been used to separate and detect pseudoephedrine hydrochloride from other pharmacologically active amines. Whatman No. 1 paper developed in n-butanol:water:95% acetic acid (4:5:1), n-butano1:toluene: water:95% acetic acid (10:10:5:5), ethyl acetate:water:95% acetic acid (3:3:1), o r chloroform:water:95% acetic acid (10:5:4) gave Rf values of 0.73, 0.35, 0.57, and 0.52 for pseudoephedrine hydrochloride respectively. Visualization of pseudoephedrine hydrochloride was done by spraying the chromatogram with 0.5% bromcresol green in methanol or 0.2% ninhydrin in acetic acid:butanol 5 :95.30 6.54 Gas Chromatography Pseudoephedrine hydrochloride has been separated from other arnines by gas chromatography. The oxazolidine
504
STEVEN A. BENEZRA AND JOHN
w.MCRAE
derivative has been prepared by the reaction of pseudoephedrine with anhydrous acetone. On a 1.15% SE-30, glass column, 2.4 m x 3 mm i.d. at 104OC the oxazolidine derivative has a retention time of 16.4 minutes.31
On a 15% PEG 6000, glass column 2 m x 4 mm i.d. at 175OC the oxazolidine derivative had a retention time of 10.1 minutes.32 The N-trifluroacetyl-L-prolylchloride derivative of pseudoephedrine has retention time of 105 minutes on a 3% SE-30, stainless steel column, 2 m x 3 mm i.d. at 170°C.33 An on-column acetic anhydride derivatization technique has been described for pseudoephedrine hydrochloride. Immediately after injection of a solution of pseudoephedrine onto a 20% SE-30, 1.8 m x 7 mm i.d. glass column at 125OC, an injection of acetic anhydride was made. The pseudoephedrine derivative formed on column has a retention time of 55.5 minutes as compared to a retention time of 8.7 minutes for underivatized pseudoephedrine.34 A variety of methods have been used to determine pseudoephedrine hydrochloride levels in plasma and urine by ~~ basefied gas chromatography. Bye and c o - w o r k e r ~extracted plasma or urine with diethyl ether. The ether extract concentrate was chromatographed on a 1.2 m x 2mm i.d. glass column packed with 2% Carbowax 20 M +5% KOH. The column was maintained at 187OC for plasma samples and 15OoC for urine samples. The heptafluorobutyric anhydride derivative of pseudoephedrine and electron capture detector have been used to enhance the sensitivity of the gas chromatographic method. Lin and c o - ~ o r k e r sand ~ ~ Cummins and Fourier37 extracted basefied urine or serum with benzene. Heptafluorobutyric anhydride is added to the benzene extract. The heptafluoroibutyric anhydride derivative extracted was chromatographed
505
PSEUDOEPHEDRINE HYDROCHLORIDE
on a 3% OV-17, 1.82 m x 2 mm i.d. glass column at 150°C36 or a 5% ethylene glycol succinate, 1.82 m x 2 mm i.d. stainless steel column at 140°C. 37 Pseudoephedrine in urine was analyzed by gas chromatography using a 2% polyethylene glycol 600 + 5% KOH,
2 m x 2 mm i.d. stainless steel column at 165OC. The urine was extracted with diethyl ether and then made basic with 5N NaOH. The pseudoephedrine was extracted with diethyl ether, concentrated, and injected directly into the gas chromatograph, or derivatized with acetone and then chromatographed.38 Pseudoephedrine was determined after acidification, precipitation, and acetic anhydride derivatization. The ester derivative was injected onto a 2.5% SE-30, 1.8 m x 4 mm i.d. column at 190°C.39 References 1.
N . F . XIV, Mack Printing Co., 1975
2. W. Martin, Burroughs Wellcome Co., personal communication 3 . R . Crouch, Burroughs Wellcome Co., personal communication 4.
J.W. McRae, unpublished data
5. D. Brent, Burroughs Wellcome Co., personal communication
6. B.S. Hurlbert, Burroughs Wellcome Co., personal communication 7. J. Ebron, Burroughs Wellcome, personal communication 8. M. Mathew, G.J. Palenik, Acta. Cryst., E, 1016 (1977)
9. V. Prelog, P. Haflinger, Helv. Chim. Acta., 33, 2021 (1950) 10. L.H. Welsh, J. h e r . Chem. SOC., 3500 (1949) 11. R. Seaman, Burroughs Wellcome Co., personal communication
c,
STEVEN A. BENEZRA AND JOHN W.MCRAE
506
12.
R.H. Manski, T.B. Johnson, J. h e r . Chem. SOC., 51,
1906
(1929) 13.
T. Morgan, Burroughs Wellcome Co., personal communication
14.
D.R. Feller, P. Basu, W. Mellon, J. Curott, L. Malspeis, Arch. Int. Pharmacodyn.,
15. 16.
17.
203,
187 (1973)
D.C. Brater, L.Z. Benet, E. Lin, R.C. Morris, Jr.,
K.L. Melmon, Clin. Res., 24, 252A (1976) R.G. Kuntzman, I. Tsai, L. Brand, L. Mark, Clin. Pharmacol. Ther., 12, 62 (1971) J. Bralet, Y. Cohen, G . Valette, Biochem. Pharm.,
11
2319 (1968) 18.
M.D. Fairchild, G.A. Alles, J. Pharmacol. Exp. Ther.
19. 20.
158, 135 (1967) J.E. Wallace, J. Pharm. S c i . , g ,1489 (1969) L. Chafetz, J. Pharm. Sci., 60, 291 (1971)
21.
J.A. McCrerie, Wellcome Foundation Ltd., personal communication
22.
I.L. Honigberg, J.T. Stewart, A.P. Smith, J. Pharm. Sci.,
3,766
(1974)
23.
T.L. Spriek, J. Pharm. Sci., 64, 5 9 1 (1974)
24.
G.T. Hill, Wellcome Foundation Ltd., personal communication
25.
M.L. Blackmon, Burroughs Wellcome Co., personal communication
26.
K.K. Kaistha, R. Tadrus, R. Janda, J. Chromatog.,
107,
359 (1975) 27. 28
29. 30.
Y. Hashimoto, Y. Ikeshiro, T. Higashiyama, T. Ando, M. Endo, Yakugaku Zasshi, 97, 1594 (1977) L.N. Mikhailova, M.N. Preobrazhenskaya, G.M. Kadatskii, S.D. Sokolov, Khim.-Farm. Zh., 2, 49 (1975) J.C. Hudson, W.P. Rice, J. Chromatog., 117, 449 (1976) A. WickstrZim, B. Salvesen, J. Pharm. Pharmacol., 4, 631 (1952)
PSEUDOEPHEDRINE HYDROCHLORIDE
31.
507
E.B.-Hanssen, A.B. Svendsen, J. Pharm. Sci.,
51,
938
(1962) 32.
K. Yamasaki, K. Fujia, M. Sakamoto, M. Okeda, M. Yoshida, 0. Tanaka, Chem. Pharm. Bull.,
33.
22,
2898 (1974)
A.H. Beckett, B. Testa, J. Pharm. Pharmacol., 9, 382 (1973)
34. 35.
M.W. Anders, G.J. Mannering, Anal. Chem., 34, 730 (1962) C. Bye, H.M. Hill, D.T.D. Hughes, A.W. Peck, Eur. J. Clin. Pharmacol., 8, 47 (1974)
36.
E.T. Lin, D.C. Brater, L.Z. Benet, J. Chromatog., 140, 273 (1977)
2,
37.
L.M. Cummins, M.J. Fourier, Anal. Lett.,
38.
A.H. Beckett, G.R. Wilkinson, J. Pharm. Pharmacol.,
39.
Suppl. 1 7 , 104s (1965) P. Leblish, B . S . Finkle, J . W . Chem.,
16,195
(1970)
403 (1969)
Brackett, Jr., Clin.
Analytical Profiles of Drug Substances, 8
TRIPROLIDINE HYDROCHLORIDE Steven A . Benezra and Chen-Hwa Yang I. 2.
3. 4. 5. 6.
Description I. I Name, Formula, Molecular Weight I .2 Appearance, Color, Odor Physical Properties 2. I Infrared Spectrum 2.2 Nuclear Magnetic Resonance Spectrum 2.3 Ultraviolet Spectrum 2.4 Mass Spectrum 2.5 Fluorescence Spectrum 2.6 Crystal and Molecular Structure 2:7 Melting Point 2.8 Solubility 2.9 Partition Coefficient 2.10 Dissociation Constant Synthesis Stability Drug Metabolic Products and Pharmacokinetics Methods of Analysis 6. I Elemental Analysis 6.2 Nonaqueous Titration 6.3 Ultraviolet Spectrophotometric Analysis 6.4 Quantitative Infrared Analysis 6.5 Chromatography 6.5 I High Performance Liquid Chromatography 6.52 Thin-Layer Chromatography 6.53 Quantitative Thin-Layer Chromatography 6.54 Gas Chromatography 6.6 Fluorimetric Analysis
509
Copy-t @ 1979 by Academic F’ress, Inc. AU rights of reproduction in any form reserved.
ISBN 0-12-2608089
5 10
1.
STEVEN A. BENEZRA AND CHEN-HWA YANG
Description 1.1
Name, Formula, Molecular Weight Triprolidine hydrochloride is E-2-[3-(l-pyrroli-
diny1)-1-p-tolylpropenyllpyridine,
monohydrochloride;
E-l-(2-pyridyl)-3-pyrrolidino-l-p-tolylprop-l-ene,
monohydro-
chloride. J
M.W. 314.85 1.2 Appearance, Color, Odor Triprolidine hydrochloride occurs as a white, crystalline powder, with no more than a slight unpleasant odor.
2.
Phvsical ProDerties 2.1
Infrared Spectrum (IR) The infrared spectrum of triprolidine hydrochloride
is shown in Figure 1.
The IR spectrum was recorded with a
Nicolet model 7199 FT-IR spectrophotometer as a 0.2% dispersion of triprolidine hydrochloride in KBr.2
Table I gives
the infrared assignments consistent with the structure of triprolidine hydrochloride.
511
TRIPROLIDINE HYDROCHLORIDE
Table I Infrared Spectral Assignments €or Triprolidine Hydrochloride Monohydrate Assignment
Band (em-')
3480 2958 2690 1630 1582 1562
OH stretch (hydrate) CH stretch (-CH3) NH' stretch C=C stretch (conj. diene) C=C stretch (aromatic) C=C stretch (pyridine)
1462 1386 1358 846
-CH a s p . bend 3 -CH3 sym. bend C-N stretch (tert. amine) =C-H rock
824 776
para subst. benzene 1-subst. pyridine
2.2 Nuclear Magnetic Resonance (NMR) Spectrum The NMR spectrum of triprolidine hydrochloride is shown in Figure 2. It was obtained with a Varian XL-100 100 MHz NMR spectrometer. Deuterated DMSO was used as the solvent with tetramethylsilane as an internal standard. The interpretation of the NMR spectrum is given in Table 11.
i 9
H3cQ
e
b
c I'
1
8
1
1
?=====-
c P
r-
{
1
8
I
8
I
33NVlllWSNVU
I
P
0
I
1
I
1
STEVEN A. BENEZRA AND CHEN-HWA YANG
5 I4
Table I1
NMR Assignments for Triprolidine Hydrochloride Chemical Shift (ppm) No. of Protons Multiplicity Assignments 1 1 11.55 j a 1 multiplet 8.63 b 6 1 7.74 multiplet C 1 7.35 d multiplet 7.00 1 4 4 benzene ring 7.12-7.38 e 1 3 6.95 f 2 2 3.78 h 1 (broad) 2 3.49 h 1 (broad) 2 2.94 1 i 2.37 3 mu1tiplet 1.88 4 lz =8, Jc,d=1.2, Jaf=7 J =4.7, Ja,d=0.9, Ja,b=2.0, J b,c
a,c
2.3 Ultraviolet (W)Spectrum The ultraviolet spectrum of triprolidine hydrochloride in 0.1N HC1 was taken with a Beckman ACTA CIII W spectrophotometer and is shown in Figure 3.4 Table I11 gives the W data for triprolidine hydrochloride in various solvents. Table I11 W Spectral Data for Triprolidine Hydrochloride Solvent h a x (NO)
EmaX
0.1N NaOH
0.1N HC1 Methanol
234 275 232 290 235 282
17000 8000 13000 9900 15000 7200
5 15
TRIPROLIDINE HYDROCHLORIDE
I-
0.6 W
0 Z
a m cr
0 cn
m
a
220 Figure 3
260
- Ultraviolet
300 340 nm
380
Spectrum of Triprolidine Hydrochloride
250 m /e
Figure 4
-
Mass Spectrum of Triprolidine Hydrochloride
300
STEVEN A. BENEZRA AND CHEN-HWA YANG
516
2.4 Mass Spectrum The mass spectrum of triprolidine hydrochloride is shown in Figure 4. It was obtained with a Varian MAT CH5-DF mass spectrometer. The electron energy was 70 eV and the sample was introduced via direct probe at 120°C.5 The characteristic fragments are in agreement with those found by Kuntzman and co-workers.6 The major fragments characteristic of triprolidine are shown in Figure 5. 2.5 Fluorescence Spectrum Triprolidine hydrochloride in 0.1M sulfuric acid has an excitation maximum at 305 nm and an emission maximum at 445 nm. The fluorescence is much diminished in hydrochloric acid and almost non-existent in distilled water. The addition of halide ions to 0.1M sulfuric acid solutions of triprolidine hydrochloride has a quenching effect on the fluorescent intensity. The degree of quenching is I- > BrZC1 > F-. A concentration of 10-3M C1- has little effect on the fluorescent intensity, while 0.1M C1- reduces the
s
intensity by a proximately 75% of the chloride-free sulfuric acid solution.
2.6 Crystal and Molecular Structure James and Williams have determined that triprolidine hydrochloride monohydrate crystals belong to the P2 /c 1 space group.8 There are 4 molecules per unit cell. The cell parameters are a = 14.777 b = 9.5785 c = 13.099 0 A, and f? = 90.48O. The 2-pyridyl ring and p-tolyl group make dihedral angles of 29.7O and 55.3O respectively with the double bond plane. The inter-aryl dihedral angle is 106.5O. The data was obtained on crystals grown from a solution of the compound in anisole. A Picker FACS-1 diffractometer with CuK01 radiation was used for the measurements.
i,
i,
R2,
r c=c
RI’
, c=c
R l?
R2 \
3
‘H
RI’
/-R3
R2,
+c=c
‘H
m/e 200 ( 10%)
c=c+
R,’ H ‘ m/e 194 ( 18 %)
R2=QCH
Figure 5
c=c R,’
‘H
m/e 209 (90%)
m/e 278 ( 33%)
R2,
+CH2 /
CH’;
- Major
‘H
m/e 208 (100%)
R2\+
/
CH
+CHz-R,
Rl m/e 182 (7%)
R3=-N
m/e 84 (15 %)
3
Ions in Mass Spectrum of Triprolidine Hydrochloride
STEVEN A. BENEZRA AND CHEN-HWA YANG
518
2.7 Melting Point Triprolidine hydrochloride melts at 115-12OoC in a sealed capillary tube.
2.8 Solubility The solubility of triprolidine hydrochloride, as the monohydrate, in various solvents at 25OC is given in Table IV.9 Table IV Solubility of Triprolidine Hydrochloride at 25OC Solvent
Solubility (mg/ml)
Water
316
0.1N HC1
319
95% Ethanol
374
n-Octanol
75
Chloroform
480 237 <1
Propylene Glycol Diethyl Ether 2.9 Partition Coefficients
The partition coefficients of triprolidine hydrochloride in n-octanol/aqueous pH 1.2 and n-octanol/aqueous pH 7.4 are 0.041 and 7.0 respectively.9 2.10 Dissociation Constant The pKal and pKa2 of triprolidine are 3.6 and 9.3 respectively.9 3.
Synthesis The synthesis of triprolidine hydrochloride is
shown in Figure 6.l o
The 4-methyl-w-pyrrolidinopropiophenone used in the first step is prepared by the Mannich
b
+
c-3 z O
0
AI
X
+
+ m I
0
I
i
I
/
I
T
I
m z a
520
STEVEN A. BENEZRA AND CHEN-HWA YANG
reaction of 4-methylacetophenone and pyrrolidine. With proper dehydration conditions of the carbinol, a product almost pure in the desired E-conformation is obtained. 4. Stability Ultraviolet light will convert the E-form of triprolidine hydrochloride to the Z-form. After 2 years at 37OC, triprolidine hydrochloride in a syrup formulation does
not decompose more than 10%. After 3 years at 37OC triprolidine hydrochloride in tablet formulations does not decompose more than 10%. The formulations are kept in light resistant containers since triprolidine hydrochloride discolors on exposure to light.' Drug Metabolic Products and Pharmacokinetics Figure 7 shows the major metabolic pathway of triprolidine hydrochloride as determined in a study of 14C labelled triprolidine hydrochloride in guinea pigs. Triprolidine is converted to metabolite I by liver microsomes. Metabolite I is converted to metabolite I1 which is the major metabolite found in guinea pig urine. The plasma levels of triprolidine hydrochloride were determined in 16 normal male subjects.12 When administered orally at a concentration of 3.75 mg triprolidine hydrochloride in 15 ml of syrup, peak plasma levels of 8 . 2 ng/ml were achieved in 2 hours with a drug half-life of 5 hours. The low plasma levels found indicate a large volume of tissue distribution which was consistent with data obtained from rat studies. 5.
Methods of Analysis 6.1 Elemental Analysis The results of the elemental analysis of triprolidine hydrochloride are given in Table V.3 The theoretical
6.
0=0 I
I
I zI
$1 I zI
H W
-I
k 0
m
e I
W
H
W
k J
0
a
m
z
k W
01
Q
0
&
4
0
W
VJ
aJ
STEVEN A. BENEZRA AND CHEN-HWA YANG
522
figures are based on the monohydrate. Table V Elemental Analysis of Triprolidine Hydrochloride Element Theory (%) Found (%>* 58.50
58.59
H 7.51 N 8.41 *N.F. Reference Standard
7.58
C
8.39
6.2 Nonaoueous Titration
Triprolidine hydrochlor-Je -s dissolved, w th warming if necessary, in glacial acetic acid. Mercuric acetate test solution is added and the solution titrated with 0.1N perchloric acid, the end-point being determined potentiometrically. Each ml. of 0.1N perchloric acid is equivalent to 0.05 m o l e of triprolidine hydrochloride. 6.3 Ultraviolet Spectrophotometric Analysis
An ultraviolet spectrophotometric analysis is used to determine content uniformity of triprolidine hydrochloride in tablet formulations.
The triprolidine hydro-
chloride is extracted from finely powdered tablets with dilute hydrochloric acid. The solution is filtered and diluted to a concentration of approximately 10 pg triprolidine hydrochloride per ml.
The absorbance at 290 nm of
the extracted triprolidine hydrochloride solution in 1 cm cells is compared against NF Triprolidine Hydrochloride Reference Standard prepared in dilute hydrochloric acid at the 10 pg/ml level. 6.4 Quantitative Infrared Analysis
Quantitative infrared analysis is used as an assay
TRIPROLIDINE HYDROCHLORIDE
523
procedure for triprolidine hydrochloride in syrup and tablets.
’
A portion of syrup or tablets equivalent to 20 mg
and 12.5 m g triprolidine hydrochloride, respectively, is placed in a separatory funnel or glass-stoppered test tube. Distilled water is added to dilute the sample followed by concentrated NaOH solution to liberate triprolidine free base.
The triprolidine free base is extracted into cyclo-
hexane. The infrared absorbance of the cyclohexane extract is determined at 824 cm
-1
in 1 mm thick cells. A base line
is drawn between 840 cm-’ and 806 cm-’.
The absorbance of
the sample is compared against the absorbance of a NF Triprolidine Hydrochloride Reference Standard treated in the same manner as the sample. 6.5
Chromatography
6.51 High Performance Liquid Chromatography (HPLC) Separation of the E and 2 isomers of triprolidine hydrochloride has been performed with HPLC. A DuPont SAX column (lm x 2 mm i.d.) with a mobile phase of 0.04M NaN03 and 0.01M Na HP04 at a pressure of 1500 psi gave retention 2 times of 4 minutes and 9 minutes for the E and 2 isomers re~pective1y.l~A 0.45m x 4 mm i.d.
Partisil@ silica gel
column with a mobile phase of acetonitri1e:concentrated
NH40H:H20 (1000:5:45) at 2 ml/min gave retention times of 15 and 22 minutes for E and 2 isomers respectively.’* A mixture of triprolidine hydrochlaride with other drugs normally found
in combination with triprolidine hydrochloride was separated with a 1.22m x 2.3 mm i.d. column containing a chemically bonded diphenyldichlorosilane pellicular packing. A mobile phase consisting of 6 0 : 4 0 acetonitrile:l% aqueous ammonium acetate (pH 7.4) with a flow rate of 1.4 ml/min gave a retention time of 310 seconds for triprolidine.15 Syrup and
524
STEVEN A. BENEZRA AND CHEN-HWA YANG
tablet formulations of triprolidine hydrochloride can be analyzed by HPLC using a SpherisorbG3 lop C18 reversed phase column eluted with ethanol:0.5% aqueous ammonium acetate (4:l) at 2 ml/min. In this system triprolidine hydrochloride has a retention time of 22 minutes. l6 6.52 Thin Layer Chromatography (TLC) Various TLC systems for triprolidine hydrochloride are given in Table VI. Table VI Thin Layer Chromatography Systems for Triprolidine Hydrochloride Mobile Phase ch1oroform:methanol:ammonia 80:20:1 ch1oroform:diethylamine 95:5 2-butanone:dimethylformamide 1:1 n-buty1acetate:acetone: n-butano1:methanol:lOX aq. ammonia 4:2:2:1:1 2-butanone:toluene: methano1:diethylamine 60:40:7:3 cyc1ohexane:benzene: diethylamine 75:15:10 methano1
Adsorbant Silica gel F
Rf Reference 0.60 17
Silica gel F
0.44
17
Silica gel F
0.60
17
Silica gel F
0.60
17
Silica gel F
0.40
17
Silica gel G
0.41
18
Silica gel G 0.40 pre-coated with
18
525
TRIPROLIDINE HYDROCHLORIDE
0.1M NaOH
acetone
Silica gel G
0.13
19
0.17
18
0.02
19
Silica gel G
0.40
20
ethano1:acetic acid:water
Silica gel G
0.48
20
5:3:2 methano1:n-butanol
Silica gel G
0.26
20
Alumina
0.81
20
pre-coated with 0.1M NaOH methano1
Silica gel G pre-coated with 0.1M KHS04
95% ethanol
Silica gel G pre-coated with 0.1M KHS04
benzene:dioxane:amonia 60:35: 35
6:4 n-butano1:n-butyl ether: acetic acid 4:8:1 6.53 Quantitative Thin Layer Chromatography Quantitative TLC has been used to determine triprolidine hydrochloride in human plasma. l 2 Plasma was extracted with dichloroethane at physiological pH (7.4). The organic phase was evaporated and the residue dissolved in chloroform. A portion of the chloroform solution was spotted on silica gel plates which were then developed in ch1oroform:methanol:anunonia
(89:lO:l). After development,
the plate was air dried and sprayed with a 2M aqueous solution of ammonium bisulfate. After the plate was air dried for 1 hour, the fluorescent spot representing triprolidine was
quantitated with a spectrodensitometer in the reflectance mode with 300 nm excitation and emission above 405 nm.
With
STEVEN A. BENEZRA AND CHEN-HWA YANG
526
this technique it was possible to quantitate as little as 0.4 ng triprolidine spotted on the plate.
6.54 Gas Chromatography Triprolidine hydrochloride has been separated from other antihistamines with a 1.52111x 2 . 4 m m i.d. column packed with 2% carbowax 20M + 10% KOH on 60180 mesh Chromosorb W. Retention time of 32 minutes was obtained with a column temperature of 190OC. Triprolidine hydrochloride was probably eluted as the free base.21
6.6 Fluorimetric Analysis Triprolidine hydrochloride in syrups and tablets can be analyzed by fluorimetry. A portion of the tablets or syrup is made basic with 1N NaOH and extracted with ethylene chloride. The organic phase is then extracted with 0.1N H2S04.
The fluorescence of the acid extract is determined
with a fluorometer using a UGll filter for excitation and a Wratten 2A filter for emission. The fluorescence of the sample preparation is compared against a Reference Standard prepared in the same manner22.
527
TRIPROLIDINE HYDROCHLORIDE
References 1.
N.F. XIV, Mack Printing Co.,
2.
W. Martin, Burroughs Wellcome Co., personal
1975
communication 3.
B.S. Hurlbert, Burroughs Wellcome Co., personal communication
4.
C-H. Yang, Burroughs Wellcome Co., unpublished data
5.
D. Brent, Burroughs Wellcome
Co.,
personal
communication 6.
R. Kuntzman, E. Sernatinger, I. Tsai, A. Klutch, Importance Fundam. Princ. Drug Eval. Proc. Symp., 87 (1968)
7.
J. McCrerie, Wellcome Foundation Ltd., personal communication
8.
M.N.G. James, G.J.B. Williams, Can. J. Chem.,
52,
1880
(1974) 9.
T.A. Morgan, Burroughs Wellcome Co., personal communication
U.S. Patent 2,712,023 11. D. Adamson, J. Billinghurst, J. Chem. SOC., 1039 (1950) 12. R.L. DeAngelis, M.F. Kearney, R.M. Welch, J. Pharm. Sci., 66, 841 (1977) 13. K. Holmes, Burroughs Wellcome Co., personal communication 14. G.T. Hill, Wellcome Foundation Ltd., personal communication 15. I.L. Honigberg, J.T. Stewart, A.P. Smith, J. Pharm. Sci., 63, 766 (1974) 16. R. Jones, Wellcome Foundation Ltd., personal communication 17. A.C. Caws, Wellcome Foundation Ltd., personal communication 18. W.W. Fike, I. Sunshine, Anal. Chem., 37, 127 (1965) 10.
STEVEN A. BENEZRA AND CHEN-HWA YANG
528
19. W.W. Fike, Anal Chem.,
38, 1697
(1966)
20. J. Cochin, J.W. Daly, J. Pharm. Exptl. Therap.,
139, 160
(1963) 21. C.R. Fontan, W.C. Smith, P.L. Kirk, Anal. Chem.,
(1963) 22. C. Skinner, Burroughs Wellcome Co., personal
communication
35, 591
Analytical Profiles of Drug Substances, 8
SODIUM VALPROATE AND VALPROIC ACID Zui L . Chang I.
2.
3. 4. 5. 6.
7. 8. 9.
Description 1. I Nomenclature 1.1 I Chemical Names I . 12 Trade Names 1.2 Formulas and Molecular Weights 1.3 Appearance, Color, Odor Physical Properties 2.1 Infrared Spectra 2.2 Nuclear Magnetic Resonance Spectra 2.3 Mass Spectrum 2.4 Raman Spectra 2.5 Ultraviolet Spectrum 2.6 Solubility 2.7 Crystal Properties 2.8 Dissociation Constants 2.9 Hygroscopic Behavior 2.10 Sublimation 2. I 1 Melting Range 2.12 Boiling Point 2.13 Differential Thermal Analysis 2.14 Specific Gravity 2.15 Refractive Index Synthesis Stability-Degradation Drug Metabolism and Pharmacokinetics Methods of Analysis 6. I Identification 6.2 Elemental Analysis 6.3 Chromatographic Analysis 6.3 1 Thin-Layer Chromatography 6.32 Gas-Liquid Chromatography 6.4 Titrimetry Determination of Valproic Acid and Its Metabolites in Biological Fluids References Acknowledgments
529
Copyright @ 1979 by Academic Rcss, Inc. All rights of reproduction in any form reserved.
ISBN 0-12-2€!48W-9
ZUI L. CHANG
530
1. Description 1.1 Nomenclature 1.11 Chemical Names Sodium valproate is sodium 2-propylpentanoate. It is also known as sodium dipropylacetic acid, sodium 2-propylvalerate, sodium dipropylacetate, sodium di-n-propylacetate, and by many slight variations of the particular nomenclature. Valproic acid is also known propylvaleric variations of
is 2-propylpentanoic acid. It as n-dipropylacetic acid, 2acid, DPA, and by many slight the particular nomenclature.
1.12 Trade Names DepakeneB, Depakinea, EurekeneB, Epilim, ErgenylB, and LabazeneB. 1.2 Formulas and,MolecularWeights CH3CH2CH2,
CHCOONa
CH3CH2CH2/ C8H1502Na
M.W.
CH3CH2CH2,
CHCOOH
~
CH3CH2CH2 C8H1602
166.19
M.W.
144.21
1.3 Appearance, Color, Odor Sodium valproate is a white crystalline powder with a very slight characteristic odor of valproic acid. Valproic acid is a colorless slightly viscous liquid, and it has a characteristic odor of valproic acid.
SODIUM VALPROATE A N D VALPROIC ACID
2.
531
Physical Properties 2.1
Infrared Spectra The infrared spectrum of sodium valproate is presented in Figure 1. The spectrum was measured in the solid state as a potassium bromide dispersion. The following bands (cm-1) have been assigned for Figure 1 (1). a.
3000-2800 cm-l
Complex of strong bands due to the overlapping C-H stretching vibrations of the various methyl and methylene groups.
b.
1560 and 1412 cm-1
Strong bands due to the antisymmetrical and symmetrical stretching vibrations of the COO- grouping.
The infrared spectrum of valproic acid is presented in Figure 2. The spectrum was measured using the capillary method. The following bands (cm-1) have been assigned for Figure 2 (1). a.
3400-2300 cm-l
Broad and diffuse absorption due to the OH stretching vibration of the carboxylic acid.
b.
3000-2800 cm-1
Complex of strong bands due to the overlapping C-H stretching vibrations of the various methyl and methylene groups.
c. 1700 cm-'
d.
930 cm-l
Strong band due to the C=O stretching vibration of the carboxylic acid. Broad band due to the OH bending vibration of the carboxylic acid.
2.2
The nuclear magnetic resonance spectrum of sodium valproate as shown in Figure 3 was obtained on a Varian Associates T-60 N M R Spectrometer in deuterium oxide containing tetramethylsilane as the internal standard. The spectral peak assignments (2) are presented in Table I.
FIGURE 1
4000
3500
- INFRARED SPECTRUM O F SODIUM VALPROATE
3000
2500
2000
FREQUENCY ( C M - l )
1500
1000
700
FIGURE 2
- INFRARED SPECTRUM OF VALPROIC ACID WAVELENGTH (MICRONS) 4
3
2.5
5
6
7
8
9 10
12
15
VI
w W
4000
3500
3000
2 500
2000
FREQUENCY (CM-')
1500
1000
700
FIGURE 3 I
I
-
NUCLEAR MAGNETIC RESONANCE SPECTRUM OF SODIUM VALPROATE I
I
I
1
I
I
ii VI W P
I
I
I
I
I
I
I
I
8
7
6
5
4
3
2
1
0
SODIUM VALPROATE A N D VALPROIC ACID
535
Table I
NMR Spectral Assignments for Sodium Valproate Proton Assignment
.
\
CH-CO
CH3-
Chemical Shift (ppm)
Mu1tiplicity
1.9-2.5
Mu1tiplet
1.1-1.8
Complex
0.5-1.1
Complex
The nuclear magnetic resonance spectrum of valproic acid as shown in Figure 4 was obtained on a Varian Associates T-60 NMR Spectrometer as a 10% w/v solution in a solvent of deuterated chloroform. The spectral peak assignments ( 2 ) are presented in Table 11. Table I1
NMR Spectral Assignments for Valproic Acid Proton Assignment
Chemical Shift (ppm)
Multiplicity
C02H
11.3-11.6
Singlet
CHCO
1.9-2.5
Multiplet
-CH2CH2
1.1-1.8
Complex
CH3-
0.5-1.1
Complex
2.3 Mass Spectrum Sodium valproate was not sufficiently volatile for mass spectral analysis. The mass spectrum of valproic acid as shown in Figure 5 was obtained using an Associated Electrical Industries Model MS-902 Mass Spectrometer with the ionization electron beam energy at 70 eV. High resolution data were compiled and tabulated with the aid of an on-line PDP11 Computer.
ZUI L. CHANG
536
Valproic acid was quite volatile and vaporized as soon as it was admitted to the source of the mass spectrometer. Only a very weak ion was detectable in the molecular ion region at m/e 145. This would correspond to (M+H)+, but exact mass measurement was not possible because of the peak's small size and the short lifetime of the sample in the mass spectrometer. The mass spectrum assignments of the prominent ions and subsequent fragments are shown in Table I11 and Figure 6 (3). Table I11 High Resolution Mass Spectrum of Valproic Acid Measured Mass (m/e)
Calculated Mass
Formula
126.1044
126.1045
C8H140
102.0690
102.0681
CgH1002
73.0295
73.0290
C3H502
2.4
Raman Spectra The Raman spectrum of sodium valproate as shown in Figure 7 was obtained in the solid state on a Cary Model 83 Spectrometer. The following bands (cm-l) have been assigned for Figure 7 (1). a.
3000-2800 cm-'
Complex of strong bands due to the overlapping C-H stretching vibrations of the various methyl and methylene groups.
b.
1450 cm-l
Due to the superimposing C-H bending vibrations of the various methyl and methylene groups.
The Raman spectrum of valproic acid as shown in Figure 8, was obtained in the undiluted liquid state on a Cary Model 83 Spectrometer. The following bands (cm-1) have been assigned for Figure 8 (1).
FIGURE 4
- NUCLEAR MAGNETIC RESONANCE SPECTRUM OF VALPROIC ACID
I
I
I
I
1
I
I
I
I
I
FIGURE 5
=
MASS SPECTRUM O F VALPROIC ACID
Em z c z Lu
Y
>
0
100
130
539
m
2 Y
0
4 a > E 2
g
cn
5 L
3
e P
cn
z
a E a
0
el
0 0
0 0 d
0 0 9
0 a0
0
0
0
2 0 0
-
v)
1
E
-
U
Z ' r 0 0
-P g f o
w
U
2 5
-5 0 0 0
0
N
0 0 0 t
m
9
0
0
(Y
0 0 m
(Y
a0
0 0
P
0
Y
z 3 E
N
N
0
I
O P
AlISN31NI
h
0 9
540
~
I
0
I
0
I
I
(Y
I
I
I
0
1
w
>
I
AllSN31NI
0
I
9
0
m
S4 I
0
0 0 (Y
0 0 d
0 0 9 0
2 0 0
P 0 0
2
8 5 0
B 0
0
z
0 0
8 0 N
0 0
aD
N
0
0 0
5
0
0
3
ZUI L. CHANG
542
-
FIGURE 9 ULTRAVIOLET SPECTRUM O F VALPROIC ACID
0.6
0.5
0.4
ez
2 SI
0.3
9
0.2
0.1
0 200
2 50
300 WAVELENGTH (nm)
350
543
SODIUM VALPROATE AND VALPROIC ACID
2.5
a.
3000-2800 cm-1
Complex of strong bands due to the overlapping C-H stretching vibrations of the various methyl and methylene groups.
b.
1660 cm-l
Weak band due to C=O stretching vibration of the carboxylic acid.
c.
1450 cm-l
Due to the superimposing C-H bending vibrations of the various methyl and methylene groups.
Ultraviolet Spectrum (UV) Sodium valproate in methanol solution has no W maximum between 400 and 205 nm. When the UV spectrum of 0.1% solution of valproic acid in methanol solution was scanned from 400,to205 nm, one maximum at 213 nm ( E = 86) was observed (Figure 9 ) . The spectrum was obtained with a Beckman Acta V Spectrophotometer.
2.6
Solubility Approximate solubility data have been determined for sodium valproate at room temperature. One gram of sodium valproate is soluble in 0 . 4 ml of water and also in 1.5 ml of ethanol. It is freely soluble in methanol (1 in 5 ) . It is practically insoluble in common organic solvents such as ether, chloroform, benzene, n-heptane, etc. The following solubility data have been determined for valproic acid at room temperature: n-Heptane Chloroform Ethyl Acetate Methanol 100% Ethanol Acetone Diethyl Ether Benzene 1 N Aqueous NaOH 0.1 N Aqueous HCl Water
Greater than Greater than Greater than Greater than Greater than Greater than Greater than Greater than Greater than 1.15 mg/ml 1 . 2 7 mg/ml
lo%, v/v lo%, v/v
v/v v/v v/v v/v lo%, v/v lo%, v/v lo%, v/v lo%, lo%, lo%, lo%,
ZUI L. CHANG
544
2.7
Crystal Properties The X-ray powder diffraction pattern of sodium valproate was determined by visual observation of a film obtained with a 143.2 mm Debye-Scherrer Powder Camera (Table IV). An Enraf-Nonius Difractis 6 0 1 Generator; 38 KV and 1 8 MA with nikel filtered copper radiation; A = 1.5418, was employed ( 4 ) . Table IV X-Ray Powder Diffraction Pattern d-Spacings and Intensities
2.8
dA -
111 1
dA
16.0 13.4 7.7 6.7 5.8 5.25 4.9 4.77 4.42 4.21 4.09 3.95 3.85 3.64 3.40 3.20 3.13 3.02 2.87 2.84
60 100 50 3 5 20 5 2 5 30 35 5 1 15 20 1 3 4 5 5
2.80 2.66 2.61 2.57 2.46 2.42 2.37 2.23 2.20 2.06 2.01 1.97 1.93 1.90 1.86 1.81 1.75 1.69 1.66
1/11 5 2
1 1
1 1 2 2 2 2
1 1 2
1 1 5 1 1 1
Dissociation Constants Sodium valproate exhibits basic properties. Titration of an aqueous solution of sodium valproate with aqueous hydrochloric acid gave a pKa value of 4.8 (proton gained). Titration of valproic acid with aqueous sodium hydroxide using acetone-water as the sample solvent and extrapolated to pure water gave a pKa value of 4.6 (proton lost).
SODIUM VALPROATE AND VALPROIC ACID
2.9
545
Hygroscopic Behavior Sodium valproate is hygroscopic. The rate of moisture absorption was tested in a humidity chamber using a Cahn Electro Balance and the results are shown in Table V (5). Table V Rate of Moisture Absorption of Sodium Valproate
Relative Time, min. 10 20 30 40 50 60 Overnight Humidity No gain
12, 22 33, 43% 53%
1.76
3.17 4.39
5.61
6.78 7.80
42.9%*
*Sample was completely liquified. Expressed as precent weight gain. 2.10
Sublimation Sodium valproate did not sublime when it was stored at 105°C for 10 days.
2.11 Melting Range Sodium valproate does not melt, decompose, or physically change form in the normal working range of the Thomas-Hoover Capillary Melting Point apparatus. 2.12
Boiling Point The following boiling points have been reported for valproic acid: bpi4 120-121°C (6), bp20 128-13OoC (6) and bp760 221-222"C (7).
2.13
Differential Thermal Analysis Differential thermal analysis of sodium valproate shows a large endotherm beginning at 100°C and ending at 118°C which is possible due to the loss of water. A sharp endothermic peak at 450°C is indicative of the melting point of sodium valproate. Differential thermal analysis of valproic acid shows. a sharp endothermic response at 225°C indicative of the boiling point of valproic acid.
FIGURE 10 I
I
- DIFFERENTIAL THERMAL ANALYSIS CURVE OF SODIUM VALPROATE I
I
I
I
I
I
I
0
I
I
I
I
50
100
150
200
T,
O C
I
250
I
I
I
300 350 400 (CORRECTED FOR CHROME1 ALUMEL THERMOCOUPLES)
I
450
500
FIGURE 11
- DIFFERENTIAL THERMAL ANALYSIS CURVE OF VALPROIC ACID
0
50
100
150
200
250
300
350
400
1, O C (CORRECTED FOR CHROME1 ALUMEL THERMOCOUPLES)
450
500
548
ZUI L. CHANG
2.14
Specific Gravity The specific gravity of valproic acid was determined It has a in a calibrated 25 ml pycnometer at 25'C. value of 0.904 g/ml (8).
2.15
Refractive Index Valproic acid has a refractive index of N D ~ ~ - ~ 1.425 (6).
3.
Synthesis The synthesis of valproic acid was first described in the literature by Oberreit (9) in 1896. The sodium valproate is preferably formed from valproic acid by the interaction of sodium hydroxide in an aqueous solution. The synthetic pathways are shown in Figure 12.
4. Stability-Degradation Sodium valproate was found to be extremely stable when refluxed in water, 1.0 N hydrochloric acid, or 1.0 sodium hydroxide for 3 Kours. Also, it was very stable when it was subjected to heat at llO°C for 10 days and to natural sunlight for 30 days in the dry state. Valproic acid is a very stable compound. No degradation has been observed by the action of heat, light, and strong aqueous alkali, or acid. 5. Drug Metabolism and Pharmacokinetics In 1971, Eymard et. al. (10) studied the distribution and the absorption of carbon-14 labeled sodium valproate in rats by oral administration. The metabolites and metabolic pathway of a new anticonvulsant drug, sodium valproate, in rats were investigated using carbon-14 labeled sodium valproate. Most of the metabolites in urine and bile were a glucuronide conjugate of ValprOic acid. Free sodium valproate was as little as one-seventh of the total metabolites. In feces, only free sodium valproate was detected, and the possibility of enterohepatic circulation of sodium valproate was presumed. A part of dosed sodium valproate was excreted in expired air in the form of C02. This degradative reaction took place in liter mitochondria and required CoA and oxygen. It was stimulated by ATP
FIGURE 12
- SYNTHETIC PATHWAYS OF VALPROIC ACID AND SODIUM VALPROATE
/ CH2
C02C2H5
\ C02C2H5
Diethyl Malonate
+
2CI-CH2CH
= CH2
c02r
CH2= CHCH2 * C ’‘
(or NaOCzHS) CHjOH
(or C,H,OH)
CH2= CHCH2
/ \ C02R
Esters of Diallyl Malonic Acid
Ally1 Chloride
R=CHs and/or C2H5
Pd/C H
CH3CH2CH2
\ / CH3CH2CH2/ c \
Co2R
CO2R
-
CH3CH2C H2
CH3CH2CH2
CHsCH2CH2
/ CH-C02H
2-Propylpentonoic Acid (Valproic Acid)
/ \ C02H
Dipropyl Malonic Acid
CH3CH2CH2
\
C02H
C ’‘
c
2) HCI
Esters of Dipropyl Malonic Acid
-c02
CH3CH2CH2
1) KOH, H 2 0
N aOH H2O
c
CH3CH2CH2
\
/ CH-c02No
Sodium 2-propylpentanoate (Sodium Valproate)
ZUI L. CHANG
550
and EDTA, and inhibited by various enzyme reaction inhibitors such as malonate, Antimycin-A, chloropromazine, p-chloromercuribenzoate (PCMB) and 2,4-dinitrophenol. Therefore, this degradation is not a one-step reaction, decarboxylation, but must be @-oxidation of a fatty acid. Thin-layer chromatography and gas-liquid chromatography were used for assay of metabolites (11). The pharmacokinetics of distribution and elimination of sodium valproate in mice and dogs has been reported by Schobben and van der Kleijn (12). The omega-oxidation of sodium valproate in rats has been reported by Kuhara, et. al. (13). The absorption, excretion, and biotransformation of valproic acid were studied by Kukino and Matsumoto (14). A preliminary pharmacokinetic profile of sodium valproate in monkey has been written by Levig, et. al. (15). The pharmacokinetics of sodium valproate have been studied in 7 patients by Schobben, et. al. (16). The plasma concentrations were determined by gas-liquid chromatography during and following subchronic treatment. Elimination of the drug appeared to follow a monophasic exponential course; biological half lives were 8 to 15 hours. The drug appeared to have a relatively restricted distribution: calculated relative distribution volumes ranged from 0.15 to 0.40 llkg. There were large interindividual differences in clearance rate. The therapeutic range was considered to be between 50 and 100 mg/l of plasma. In 1976, Matsumoto, et. al. (17, 18) discovered several new metabolites of sodium valproate in rat urine, which support the hypothesis that the drug is also metabolized by a B-oxidation mechanism. One of the metabolites, 2n-propyl 3-0x0-pentanoic acid, was recently found by Gompertz, et. al. (19) and Kochen, et. al. (20) to be a major constituent in urine of children who were receiving sodium valproate. The urinary 3-0x0 derivative of valproate was reported to account €or 20% of the administered dose. 6.
Methods of Analysis
6.1 Identification The presence of sodium cation may be identified by
55 1
SODIUM VALPROATE AND VALPROIC ACID
a flame test. A positive test for sodium is produced in a non-luminous flame imparting a yellow color. The presence of carboxylic anion may be ider!.tified by the following two tests:
6.2
A.
A 5% aqueous solution gives a violet precipitate with a 5% aqueous solution of cobalt nitrate.
B.
A 5% aqueous solution gives a violet precipitate with potassium iodobismuthite.
Elemental Analysis A typical elemental analysis of a sample of sodium valproate is present in Table VI (21).
Table VI Elemental Analysis of Sodium Valproate Element C
H 0
Na
% Theory 57.82 9.10 19.25 13.83
% Found
57.82 9.38
-----* -----*
*The oxygen value cannot be determined due to presence of sodium.
A typical elemental analysis of a sample of valproic acid is present in Table VII (22). Table VII Elemental Analysis of Valproic Acid Element C
H 0
6.3
% Theory
66.63 11.18 22.19
% Found
66.39 11.32 22.43
Chromatographic Analysis 6.31
Thin-Layer Chromatography A number of thin-layer chromatographic systems
552
ZUI L. CHANG
on silica gel have been found to induce the migration of the compound. However, no system has been found which gives resolution equivalent to the gas-liquid chromatographic system detailed in section 6.32. Thin-layer chromatography is not the preferred method for determining the impurities. The following systems have been studied : 1. Ch1oroform:Methanol:Glacial Acetic Acid (17:2 :1) 2.
Ethyl Acetate:Formic Acid:Water (5:l:l)
3.
Benzene:Methanol:Acetone:Ammonium Hydrox-
ide (2:2:5:1)
4. Ch1oroform:Methanol:Ammonium Hydroxide (20:15 :3)
5. n-Butanol Saturated with 10% Ammonium Hydroxide Solution (Aqueous) 6.32 Gas-Liquid Chromatography The author has found the following GLC procedure to be suitable to determine the purity of sodium valproate and valproic acid. Preparatory to chromatography, the sodium valproate was acidified with a strong aqueous hydrochloric acid solution, and the valproic acid which is practically insoluble in water was separated. The separated free acid was then analyzed. The following is the typical chromatographic condition for the GLC determination of valproic acid: Column: 10% DEGS-PS on Supelcoport 80/100 mesh, Two 6 ft x 114 in 0.d. stainless steel. Detection: Thermal Conductivity Detector. Temperature: Inj. Port Column Detector Flow Rate:
225OC 160°C 300°C -20 ml/min helium
SODIUM VALPROATE AND VALPROIC ACID
553
Attenuation: 2 x 4 Slope Sensitivity: 0.03 or adjust for proper sensitivity Sample Size:
2 1.11
Impurities as low as 0.01% could be detected using the above conditions. 6.4
Titrimetry Sodium valproate exhibits basic properties. It can be titrated with 0.1 N hydrochloric acid. In addition, sodium valproate can be potentiometrically titrated with standardized 0.1 perchloric acid using a modified glass-calomel electrode system, in which 0.1 N lithium perchlorate in acetic acid has been substituted for potassium chloride, and employing glacial acetic acid as the sample solvent
.
Valproic acid can be potentiometrically titrated with standardized 0.1 N tetra-n-butylammonium hydroxide in chlorobenzene using a modified glasscalomel electrode system, in which 1.0 aqueous tetra-n-butylammonium chloride has been substituted for potassium chloride, and employing acetone as the sample solvent. 7.
Determination of Valproic Acid and Its Metabolites in Biological Fluids Many gas-liquid chromatographic methods for determination of valproic acid in biological fluids have been reported. Early methods required derivatization of valproic acid ( 2 3 , 24, 25, 2 6 ) .
Although Meijer and Hessing-Brand in 1973 (27) developed a micro diffusion method without derivatization, it required special equipment. Recently, most of the methods which have been used for the analysis of valproic acid in plasma, serum, cerebral spinal fluid, saliva, breast milk, and urine involve acidification of the biological sample, extraction into an organic solvent, and direct injection onto a gasliquid chromatographic column (28, 29, 16, 30, 31, 3 2 ,
554
ZUI L. CHANG
33, 34, 35, 36, 37, 38, 39). Most of the methods employ an internal standard, and all are reported as accurate and reproducible. However, Schmidt, et. al. (40) recently reported great interlaboratory variation in the analysis of such biological samples. 8. References 1. W. Washburn, Abbott Laboratories, Personal Communication.
2. M. Cirovic and R. Egan, Abbott Laboratories, Personal Communication. 3. S. Mueller, Abbott Laboratories, Personal Communication. 4.
J. Quick, Abbott Laboratories, Personal Communication.
5. M. Yunker, Abbott Laboratories, Personal Communication. 6. The Merck Index, 9th Edition, 9574, Merck ti Co., Inc., Rahway, N.J., 1976. 7. Dictionary of Organic Compounds, Vol. 5, p. 2799, Oxford University Press, New York, (1965).
8. J. Fornnarino, Abbott Laboratories, Perwnal Communication. 9. E. Oberreit, Berichte der Deutschen Chemischen Gesellschaft, 3,1998 (1896).
10. P. Eymad, et. al., J. Pharmacol. (Paris), 2 (2), 251 (1971)
.
11. K. Kukino, K. Mineura, T. Deguchi, A. Ishii and H. Takahira. Yaku-Gaku Zasshi, 92 (71, 896 (1972). 12. F. Schobben and E. van der Kleijn, Pharm. Weekbl., 109 (2), 33 (1974). 13. T. Kuhara, et. al., Biomed. Mass Spectrom., 291 (1974).
1. ( 4 ) ,
SODIUM VALPROATE AND VALPROIC ACID
555
14. K. Kukino and I. Matsumoto, J. of Kurukome Med. ASSOC., 34 (41, 369 (1975). 15. R.H. Levig, et. al., Epilepsia 16 (l), 202 (1975). 16.
F. Schobben, E. van der Kleijn and F.J. M. Gabreels, Europ. J. Clin. Pharmacol., 8, 98 (1975).
17.
I. Matsumoto, T. Kuhara and M. Yoshino, Advances in Mass Spectrometry in Biochemistry and Medicine, 1, 17-26, (1976).
18. I. Matsumoto, T. Kuhara and M. Yoshino, Biomedical Mass Spectrometry, 3 (5), 235-240, (1976). 19. D. Gompertz, P. Tippett, K. Bartlett, and T. Baillie, Clinica Chimica Acta, 74, 153-160, (1977). 20. W. Kochen, H. Imbeck and C. Jakobs, ArzneimittelForschung, 27 (I) No. 5, 1090-1099, (1977). 21.
Galbraith Laboratories, Inc., Knoxville, TN.
22. J. Hood, Abbott Laboratories, Personal Communication. 23. J. Alary, D. Cantin, A. Coeur and G. Carraz, Trav. SOC. Pharm. Lyon., 16 (2), 53 (1972).
u.
24. B. Ferrands, P. Eymard and C. Gautier, Ann. Pharm. 5, 31 (4), 279 (1973). 25. J.M.H.G. Cremers and Ing. P.E. Verheesen, Pharm. Weekbl. , 109 (22), 522 (1974). 26. F.N. Ijdenberg, Pharm, Weekbl.,
110 (2),
21 (1975).
27. J.W.A. Meijer and L. Hessing-Brand, Clin. Chim. , .Acta 43 ( 2 ) , 215 (1973). 28.
I.C. Dijkhuis and E. Vervloet, Pharm. Weekbl., (2), 42 (1974).
109
29. F. Schobben, E. van der Kleijn and Neth. Nijmegen, Pharm. Weekbl, 109 (2), 30 (1974). 30. C.R. Chard, N.J. Legg, Ed., Clinical and Pharmacological Aspects of Sodium Valproate in the Treatment of Epilepsy, pp. 89-91 (1975).
ZUI L. CHANG
556
31. P.N. Patsalos, V.C. Goldberg and P.T. Lascelles, Proc. Analyt. Div. Chem. SOC., 12 (lo), 270 (1975). 32. M.C. Pfaff and G. Mahuzier, Ann. Pharm. Fr., (1975).
33, 355
33. T.B. Vree, E. van der Kleijn and H.J. Knop, J. Chromatography, 121 (l), 150 (1976). 34. N.H. Wood, D.C. Sampson and W.J. Hensley, Clinica Chimica Acta, 77, 343 (1977). 35. L.J. Dusci and L.P. Hackett, J. of Chromatography, 132, 145 (1977). 36. L.J. Dusci and L.P. Hackett, J. Chromatography, 132 (l), 145 (1977). 37. C.J. Jensen and R. Gugler, J. Chromatography, 137, 188 (1977). 38. W. Loescher, Epilepsia 18 (2), 225 (1977). 39. A. Sengupta and M.A. Peat, J. Chromatography, 137 206 (1977). 40.
D. Schmidt, B. Ferrandes, D. Grandjean, R. Gugler, C. Jakobs, S . Johannessen, U. Klotz, W. Kochen, H.J. Kupferberg, J.M.A. Meijer, A. Richens, H. Schaefer, H.U. Schulz and.A. Windorfer, Arzneim-ForschIDrug 27 (l), 1078 (1977).
w,
9. Acknowledgements The author wishes to thank Mr. V.E. Papendick and Mr. J. B. Martin for their review of the manuscript, and Miss Diane Penza for typing the manuscript.
CUMULATIVE INDEX Italic numerals refer to volume numbers Acetaminophen, 3, I Acetohexamide, I , 1 ;2,573 Allopurinal, 7, 1 Alpha-tocopheryl acetate, 3, 11 1 Amitriptyline hydrochloride, 3, 127 Amoxicillin, 7, 19 AmphotericinB,6, 1;7,502 Ampicillin,2, I ; # , 517 Aspirin, 8, 1 Bendroflumethiazide, 5 , I ;6,597 Betamethasone dipropionate, 6,43 Bromocriptine methanesulfonate, 8 , 4 7 Calcitriol, 8,83 Cefazolin*; 4, I Cephalexin, 4,21 Cephalothin sodium, I , 319 Cephradine*, 5 , 2 1 Chloral hydrate, 2,85 Chloramphenicol, 4,47,517 Chlordiazepoxide, I , I5 Chlordiazepoxide hydrochloride, I , 39; 4,517 Chloroquine phosphate, J , 6 1 Chlorpheniramine maleate, 7,43 Chloroprothixene, 2,63 Chlortetracycline hydrochloride, 8; 101 Clidinium bromide, 2, 145 Clonazepam, 6 , 6 1 Clorazepate dipotassium, 4,91 Cloxacillin sodium, 4,113 Cyclizine, 6,83; 7, 502 Cycloserine, I , 53 Cyclothiazide, I , 66 Dapsone, 5 , 8 7 Dexamethasone, 2, 163; 4,518 Diatrizoic acid, 4,137; 5,556 Diazepam,1,79;4,517
Digitoxin, 3, 149 Dihydroergotoxine methane sulfonate, 7,8 1 Dioctyl sodium sulfosuccinate, 2, 199 Diperodon, 6.99 Diphenhydramine hydrochloride, 3, 173 Diphenoxylate hydrochloride, 7, 149 Disulfram, 4,168 Dobutamine hydrochloride, 8 , 139 Droperidol, 7,171 Echothiophate iodide, 3,233 Epinephrine, 7, 193 Ergotamine tartrate, 6, 113 Erythromycin, 8 , 139 Erythromycin estolate, 1, 101; 2, 573 Estradiol valerate, 4,192 Ethambutol hydrochloride, 7,231 Ethynodiol diacetate, 3,253 Fenoprofencalcium*, 6, 161 Flucytosine, 5 , 115 Fludrocortisone acetate, 3,281 Fluorouracil, 2,221 Fluoxymesterone, 7,251 Fluphenazine enanthate, 2,245; 4,523 Fluphenazine hydrochloride, 2,263; 4,518 Gluthethimide,S, 139 Gramicidin, 8 , 179 Griseofulvin, 8,219 Halcinonide, 8,251 Halothane, I , 119;2,573 Hexetidine, 7,277 Hydralazine hydrochloride, 8,283 Hydroflumethiazide, 7,297 Hydroxyprogesterone caproate, 4,209 Hydroxyzine dihydrochloride, 7,319 Iodipamide, 3,333 Isocarboxazid, 2,295
*Monographs in “Pharmacological and Biochemical Properties of Drug Substances: M. E. Goldberg, D. Sc., Editor American Pharmaceutical Association.
558
Isoniazide, 6,183 Isopropamide, 2,315 Isosorbide dinitrate, 4,225;5,556 Kanamycin sulfate, 6,259 Ketamine, 6,297 Leucovonn Calcium, 8,3 I5 Levarterenol bitartrate, I , 49;2,573 Levallorphan tartrate, 2,339 Levodopa, 5,189 Levothyroxine sodium, 5,225 Meperidine hydrochloride, I, 175 Meprobamate, I, 209;4,519 &Mercaptopurine, 7,343 Methadone hydrochloride, 3,365;4,519 Methaqualone, 4,245,519 Methimazole, 8,351 Methotrexate, 5,283 Methyclothiazide, 5,307 Methyprylon, 2,363 Metronidazole, 5,327 Minocycline, 6,323 Nalidixic Acid, 8.371 Neomycin, 8,399 Nitrohrantoin, 5 , 345 Norethindrone, 4,268 Norgestrel, 4,294 Nortriptyline hydrochloride, I, 233;2,573 Nystatin, 6,341 Oxazepam, 3,441 Phenazopyridine hydrochloride, 3,465 Phenelzine sulfate, 2,383 Phenformin hydrochloride, 4,319;5,429 Phenobarbital, 7,359 Phenoxymethyl penicillin potassium, I, 249 Phenylephrine hydrochloride, 3,483 Piperazine estrone sulfate, 5,375 Primidone, 2,409 Procainamide hydrochloride, 4,333 Procarbazine hydrochloride, 5,403 Prornethazine hydrochloride, 5,429
CUMULATIVE INDEX
Proparacaine hydrochloride, 6,423 Propiomazine hydrochloride, 2,439 Propoxyphene hydrochloride, I, 301 ;4 , 5 19; 6,598 Propylthiouracil, 6,457 Pseudoephedrine hydrochloride, 8,489 Reserpine, 4,384;5,557 Rifampin, 5,467 Secobarbital sodium, I, 343 Spironolactone, 4,431 Sodium nitroprusside, 6,487 Sulphamerazine, 6,515 Sulfamethazine, 7,401 Sulfamethoxazole, 2,467;4,520 Sulfasalazine,5,515 Sulfisoxazole, 2,487 Testolactone,S, 533 Testosterone enanthate, 4,452 Theophylline, 4,466 Thiostrepton, 7,423 Tolbutamide,3,513;5,557 Triamcinolone, 1,367;2,571;4,520,523 Triamcinolone acetonide, I, 397,416;2,571; 4,520;7 Triamcinolone diacetate, I , 423 Triamcinolone hexacetonide, 6,579 Triclobisonium chloride, 2,507 Triflupromazine hydrochloride, 2,523;4,520; 5,557 Trimethaphan camsylate, 3,545 Trimethobenzamide hydrochloride, 2,551 Trimethoprim, 7,445 Triprolidine hydrochloride, 8,509 Tropicamide, 3,565 Tubocurarine chloride, 7,477 Tybamate, 4,494 Valproate Sodium and valproic acid*, 8, 529 Vinblastine sulfate, I, 443 Vincristine sulfate, I , 463