GB2146330A - Separating syn and anti oxime isomers - Google Patents

Separating syn and anti oxime isomers Download PDF

Info

Publication number
GB2146330A
GB2146330A GB08422611A GB8422611A GB2146330A GB 2146330 A GB2146330 A GB 2146330A GB 08422611 A GB08422611 A GB 08422611A GB 8422611 A GB8422611 A GB 8422611A GB 2146330 A GB2146330 A GB 2146330A
Authority
GB
United Kingdom
Prior art keywords
isomers
syn
group
groups
resin
Prior art date
Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.)
Granted
Application number
GB08422611A
Other versions
GB2146330B (en
GB8422611D0 (en
Inventor
Colin Robinson
David Thomas Eastlick
Audrey Joan Bownass
Current Assignee (The listed assignees may be inaccurate. Google has not performed a legal analysis and makes no representation or warranty as to the accuracy of the list.)
Glaxo Group Ltd
Original Assignee
Glaxo Group Ltd
Priority date (The priority date is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the date listed.)
Filing date
Publication date
Application filed by Glaxo Group Ltd filed Critical Glaxo Group Ltd
Publication of GB8422611D0 publication Critical patent/GB8422611D0/en
Publication of GB2146330A publication Critical patent/GB2146330A/en
Application granted granted Critical
Publication of GB2146330B publication Critical patent/GB2146330B/en
Expired legal-status Critical Current

Links

Classifications

    • CCHEMISTRY; METALLURGY
    • C07ORGANIC CHEMISTRY
    • C07DHETEROCYCLIC COMPOUNDS
    • C07D307/00Heterocyclic compounds containing five-membered rings having one oxygen atom as the only ring hetero atom
    • C07D307/02Heterocyclic compounds containing five-membered rings having one oxygen atom as the only ring hetero atom not condensed with other rings
    • C07D307/34Heterocyclic compounds containing five-membered rings having one oxygen atom as the only ring hetero atom not condensed with other rings having two or three double bonds between ring members or between ring members and non-ring members
    • C07D307/38Heterocyclic compounds containing five-membered rings having one oxygen atom as the only ring hetero atom not condensed with other rings having two or three double bonds between ring members or between ring members and non-ring members with substituted hydrocarbon radicals attached to ring carbon atoms
    • C07D307/54Radicals substituted by carbon atoms having three bonds to hetero atoms with at the most one bond to halogen, e.g. ester or nitrile radicals

Description

1 GB 2 146 330A 1
SPECIFICATION
Chemical process This invention relates to a novel process for the separation of geometrical isomers of chemical compounds, and more particularly for the separation of geometrical isomers of oxime group-containing compounds. Many types of oxime group-containing compounds, that is, compounds containing a group of formula c 11 N 0 are known.
Especially important are cephalosporin com- pounds possessing an oxime grouping in a side chain in the 7,8-position, preferably a 90 side-chain having the formula 11 N ? 1 OR R-C-CON11- (where R and R' independently represent a hydrogen atom or an organic group) and the carboxylic acids used in the formation of such 40 side- chains.
Thus, particularly valuable oxime compounds are carboxylic acids of the formula R-C-C R 2 11 N 1 OR (1) (where R and R' have the above meanings and R 2 is a hydroxy group or the residue of a 7-aminocephem-4-carboxylic acid) and deriva- 120 tives thereof.
The most important of the above cephalos porin oxime compounds may be defined by the formula 7 B R - C ----CO. NH 3 R 3 N N 0 OR1 COOH (11) where each of R, R' and R 3 independently represents a hydrogen atom or an organic group, B is -S- or S->O / (a- or #-), and the dotted line indicates A2 or Z3 unsaturation.
If any of R, R' or R3 comprises a positively charged grouping, the compound of formula 1 or 11 may exist in the form of an internal salt formed between the said positively charged group and a carboxylate group -COT at the 4-position of the cephern nucleus.
It will be appreciated that alternative configurations of the oxime group in the above formulae 1 and 11 result in geometrical isomerism. Thus, compounds having the configuration R-C-CO 11 N OR, are designated syn-isomers, whilst compounds having the configuration R-C-CO11 N RIO are designated anffisomers.
Cephalosporin compounds possessing an oxime group in the 7p-side chain have generally been found to exhibit high stability to P- lactamases produced by many pathogenic organisms. However, it has been found that the syr-isomers of these cephalosporin compounds exhibit superior antibacterial activity to the corresponding antisomers, so that the oxime group-containing cephalosporin antibiotics are generally obtained and used in the form of their syr-isomers. The syri-isomers of the cephalosporin compounds may be prepared by employing an acid of formula 1 (where R' is a hydroxy group) substantially in the syn-isomer form, or a derivative thereof, in the 7-side chain coupling reaction and controlling the reaction conditions in this and any subsequent steps to avoid isomerisation to the anffisomer. However, in some circumstances 2 GB2146330A 2 mixtures of syn and anffisomers are formed and it is then necessary to separate them.
The separation of syn and anffisomers of oxime compounds by chromatography on sil ica gei is known. For example, British Patent Specification No. 1,576,625 describes the separation of syn and anffisomers of com pounds of formula 1 or derivatives thereof by this method. However, the separation achieved by this method depends to a large extent on the solvent system employed to elute the isomers and the separation of isom ers of different compounds often require quite different solvent systems. In general, such a procedure is not suitable for large scale oper ation.
A further method known in the art for the separation of syn and ant isomers of oxime compounds is fractional crystallisation whereby one of the isomers is crystallised from a solution of the mixed isomers while the other isomer is left in solution. However, it has been found that this technique does not achieve satisfactory separation of isomers of cephalosporin compounds.
Non-functional macroreticular adsorption re sins have found application in the purification of chemical compounds, for example in pro cesses where a cephalosporin compound is separated from other components of a fermen tation or reaction solution by loading the mixture onto the resin, washing to remove undesired components and eluting the desired compound. Thus, for example, the isolation of cephalosporin C from a fermentation solution using non-functional macroreticular adsorption resins is described in British Patent Specifica tion No. 1,303,728. Similarly, the purifica tion of semi-synthetic cephalosporin com pounds on such resins is exemplified, for example, in British Patent Specifications Nos.
1,600,735, 1,581,854 and 2,036,738 A.
However, there is no indication in this prior art that non-functional macroreticular adsorp tion resins may be used to separate geometrical isomers.
We have now surprisingly found that the geometrical isomers of osime group-contain ing compounds can be separated one from the other with high efficiency using aqueous elution from non-functional macroreticular ad sorption resins.
Thus, in one aspect the invention provides a process for the separation of a mixture of syn and antoxime isomers one from the other which comprises adsorbing said mixed oximes onto a non-functional macroreticular adsorp tion resin, and eluting said resin to yield at least one eluate fraction containing one of said isomers substantially free of the other.
In general, for efficient separation it is pre ferred that the oxime isomers should be in aqueous media, thus enabling their elution from the resin using aqueous eluants. In gen eral, the solubility of the isomers in pure 130 water at ambient temperature is desirably at least 0. 1 % by weight, more preferably at least 5%.
The aqueous eluant may conveniently be water or aqueous solutions containing salts and/or water-miscible organic solvents. Water is the preferred eluant. In general, such solutions may contain up to about 85% by volume of organic solvent but this figure may if desired be exceeded depending on the particular compounds to be separated. Solvent will normally be used to enhance the solubility of the oxume isomers in the eluant. In general, more efficient separation is to be expected if the quantity of solvent is close to the minimum required to provide sufficient solubility for elution from the resin. Examples of salts include those derived from acids such as formic, chloroacetic or acetic acid, with for example an alkali metal cation such as sodium or potassium. Examples of organic solvents include alcohols, e.g. methanol or isopropanol, or ketones e.g. acetone. The mixed isomers may be loaded onto the resin in solution.
This solution will generally be an aqueous solution but solutions in organic solvents may also be used.
A solution containing the isomers to be separated may be brought into contact with the non-functional macroreticular adsorption resin in any desired way, most suitably by loading it onto a column or bed of granular resin e.g. in conventional bead form.
Where the resin is used in the form of a column, the separation according to the invention may be essentially chromatographic. Thus, elution will tend to separate the isomers into bands which may be eluted as separate peaks. In our experience, the desired syn- isomers surprisingly always elute first, which is particularly advantageous in practice.
The peaks containing the individual isomers may be eluted separately, in which case the syn isomer obtained will contain little or none of the anti isomers. However, more typically, the peaks will overlap slightly so that after initial fractions containing only syn isomer, fractions will be eluted which contain more and more of the anti isomer in addition to the syn isomer. It will be appreciated that if all such 'mixed' fractions are rejected, the syn isomer isolated from the preceding fractions will be of high purity with respect to the anti isomer, but there may be considerable losses of desired syn isomers. On the other hand, overall recovery of syn somers can be increased in such circumstances, if fractions are also collected which contain small quantities of the anti isomer from the overlapping peak.
The operator thus has the option, where the peaks overlap, of recovering syn isomers of very high purity but in reduced yield or at reduced purity with respect to antisomer but higher yield. However, in either case, the process of the invention enables the syn 3 GB 2 146 330A 3 isomer to be obtained substantially free from the anti isomer, i.e. free from anti isomer within the tolerance acceptable for the in tended use of the product. Where the oxime is a final pharmaceutical product, the percen tage of anti isomer present is preferably not more than 3% by weight, more preferably not more than 1.5%. Where the oxime is an intermediate, however, somewhat higher levels of anti-isomer may be acceptable, e.g.
up to 5% by weight, depending on the in tended further processing of the intermediate.
The eluate fraction collected may, if de sired, be reapplied to the resin to effect fur ther purification. It may be desirable to con centrate such an eluate fraction prior to re application.
Elution of the isomers from the non-func tional macroreticular resin may be monitored by conventional techniques, such as high per- 85 formance liquid chromatography (HPLQ.
The separated isomers may be isolated from the eluate fraction(s) containing them by con ventional techniques such as by solvent ex traction and/or crystal lisation.
Non-functional macroreticular adsorption re sins which may conveniently be employed according to the invention typically have a surface area of from 100 to 1300 M2. 9- 1, e.g. 140-950 M2.g - 1, and an average pore diameter of from 2-18 nm, e.g. 3-15 nm. The resin may be, for example, a copolymer of styrene cross- linked with divinylbenzene, examples of such resins which may be used include Amberlite XAD-2 and XAD-1 180 (Rohm and Haas), Diaion HP-20 and HP-21, and SP207 (Mitsubishi), Duolite S-861 and S 8602 (Rohm and Haas), and Kastell-Sl 12 (Montedison). Other suitable resins include acrylic ester polymers such as XAD-7 and XAD-8 of Rohm & Haas. The resins may be regenerated by conventional means and re used.
According to a preferred feature, the inven tion provides a process as defined above for the separation of syn and anti oxime isomers of compounds of formula (1) and derivatives thereof. Important cephalosphorin compounds of formula (1) are those of formula (11) as defined above. In formula 11, B is preferably -S-and the unsaturation represented by the dotted line is preferablyA3.
The group R in the above formulae repre sents, as indicated above, a hydrogen atom or an organic group. Thus, for example, R may 120 be selected from carbocyclic groups preferably containing 5-12 atoms and heterocyclic groups; these are preferably unsaturated or aromatic and the heterocyclic group preferably possess 5 or 6 ring members and contain from 1 to 4 heteroatoms selected from sul phur, nitrogen and oxygen; the above groups may be substituted, for example by one or more halogen atoms or by amino or hydroxy groups, which may be in protected form, or alkoxy groups. R may also represent a C,-, alkyl group which may be substituted, for example, by oxo and/or halogen. Examples of such groups include phenyl, thieny], furyl, aminothiazolyl and aminothiadiazoly] groups.
Of particular importance are compounds in which R represents a fur-2-y] group or a protected or unprotected 2-aminothiazol-4-yi group.
The group R' in the above formulae represents, as indicated above, a hydrogen atom or an organic group. When R' represents an organic group this will desirably be an etherifying monovalent organic group containing up to 16 carbon atoms and linked to the oxygen atom through a carbon atom.
Thus, for example, R' may be a hydrogen atom or an aliphatic group such as C,-, alkyl, C,-, cycloalkyl, C4-10 cycloalkylalkyl, C2, alkenyl or C4- 7 cycloalkenyl, or a C,-,, aryl (e.g. phenyl) or C,-,, aralkyl (e.g. benzyi) group, wherein any of the above groups may be optionally substituted by a halogen atom or a free or blocked carboxy (e.g. lower alkoxycar- bonyl) group, or by a carbamoyl, cyano or protected or unprotected amino group.
There may particularly be mentioned cornpounds in which R' represents a methyl group, a free or blocked 2-carboxyprop-2-oxy group or a cyclopropyl methyl group.
The group R 3 in the above formula 11 represents, as indicatedabove, a hydrogen atom or an organic group. When R3 represents an organic group, this may be a saturated or unsaturated, substituted or unsubstituted, organic group containing 1 -20 carbon atoms. Important saturated organic groups include methyl and ethyl; important unsaturated organic groups include vinyl and substituted vinyl groups.
Particularly important meanings for R 3 in the above formula 11 include a hydrogen atom; a vinyl group substituted by a heterocyclicthio group in which the heterocyclic portion corn- prises a 5- or 6-membered ring containing up to four nitrogen atoms and optionally one sulphur atom and substituted by one or more groups independently selected from methyl, protected or unprotected oxo, formyimethyi, protected or unprotected hydroxy and free or blocked carboxymethyl groups; or a group of formula -CH,Y (wherein Y represents a halogen atom, a hydroxy, acyloxy or carbamoyloxy group or the residue of a pyridine base e.g. of pyridine, 2,3- cyclopentenopyridine, nicotinamide or isonicotinamide or of a heterocyclicthiol comprising a 5- or 6-membered heterocyclic portion containing up to four nitrogen atoms and optionally one sulphur atom and substituted by one or more, e.g. 1 to 3, groups indepen- dently selected from methyl, protected or un- 4 GB 2 146 330A 4 protected oxo, formylmethyl, carbamoylmethyl, protected or unprotected hydroxy and free or blocked carboxymethyl groups).
The oxime isomers may also be derivatives of the compounds of formula 1. The carboxyi group formed when R 2 is a hydroxy group, or the 4-carboxy group, or the 4-carboxy group of a 7- aminocephem-4-carboxylic acid residue, may thus be present in the free acid form, as in the form of a salt with a base or in the form of a blocked carbonyl function such as an ester or amide grouping or a metabolically labile ester grouping. Such blocked carboxyl functions may thus be ester groups having 1 - 12 carbon atoms in the esterifying group, e.g. t-butyl or diphenylmethyl groups. Metabolically labile ester groups include, for example, acyloxyalkyl groups, such as an acetoxyethyl group.
As indicated above, it is preferred that the oxime isomers are soluble in aqueous eluants.
In general, there will be at least one hydro philic grouping in the molecule, e.g. a salt forming grouping such as a carboxyl or amino group or a quaternary ammonium group such as a pyridinium group.
It should be appreciated that protecting groups are commonly employed in the cephal osporin art to protect any sensitive groups in the molecule in question to avoid undesirable side reactions. Thus, for example, amino, hy droxy, carboxy or oxo groups may be pro tected using known protecting groups by con ventional methods. Thus, for example an am ino group may be protected by tritylation, acylation (e.g. chloroacetylation or formyla tion) or protonation. Suitable protecting groups and techniques are fully described in textbooks such as "Protective Groups in Or ganic Chemistry" Ed. J.F.W. McOmie, 105 Plenum Press (1973), or "Protective Groups in Organic Synthesis" by T.W. Greene, Wiley Interscience (1981). Any protecting groups may thereafter be removed in any convenient way which does not cause breakdown of the desired compound. Such groups may thus in some cases be present at the stage of cephal osporin synthesis at which the separation ac cording to the invention is effected.
It will be appreciated that various tautomeric and isomeric (e.g. optical, geometric or structural isomeric) forms of any of the above groups or compounds may exist, and the definitions given herein include within their scope where appropriate all such tautomeric and isomeric forms.
Examples of cephalosporin antibiotics whose isomers may be separated by the process of the present invention include particu- larly the compounds cefuroxime: (6R, 7R)-7[((Z)-2-(fur-2-yl)-2methoxyiminoacetamido]-3carbamoyloxymethylceph-3-em-4-carboxylic acid and the 3-acetoxymethyl and 3-hydroxymethyl analogues thereof; ceftazidime: (6R, 7R)-7-[(Z)-2-(2-aminothiazol-4-yi)-2-(2-carboxyprop-2-oxyimino)acetamido]-3-(l -pyridiniummethyl)ceph-3-em-4-carboxylate; ceftizoxime: (6R, 7R)-7-[(Z)-2-(2-aminothiazol-4-yi)-2methoxyiminoacetamido]-ceph-3-em-4-carboxylic acid; ceftriaxone: (613, 7R)-7-[(Z)-2-(2-aminothiazol4-yi)-2-methoxyiminoacetamido]-3-[(2,5dihydro-6-hydroxy-2-methyi-5-oxo-as-triazin-3-yi)thiomethyl]-ceph-3-em-4carboxylic acid diso- diurn salt; cefotaxime: (6R, 7R)-3-acetoxymethyI-7-[(Z)-2(2-aminothiazol4-yi)-2-methoxyiminoacetamido]ceph-3-em-4-carboxylic acid; cefmenoxime: (6R, 7R)-7-[(Z)-2-(2-aminothia80 zol-4-yi)-2-methoxyiminoacetamido]-3-[(1 -methyl-1 H-tetrazol-5-yl)thiomethyi]ceph-3-em-4carboxylic acid; cefodizime: (613, 7R)-7-[(Z)-2-(2-aminothiazol4-yl)-2methoxyiminoacetamido]-3-[(5-carboxy85 methyl-4-methyl-1,3-thiazol-2yl)thiomethyllceph-3-em-4-carboxylic acid; (6R, 7R)-7-[(Z)-2-(2aminothiazol-4-yi)-2-methoxyiminoacetamido]-3-[2-(5,6-dioxo-4formylmethyl-1,4,5,6-tetrahydro-1,2,4-triazin90 3yl)thiovinyl]ceph-3-em-4carboxylic acid; (6R, 7R)-7-[(Z)-2-(2-aminothiazol-4-yi)-2(carboxymethoxyimino)acetamido]-3-vinyi-ceph-3em-4-carboxylic acid; cefirompe: (6R, 7R)-7-[(Z)-2-(2-aminothiazoI-4yl)-2methoxyiminoacetamido]-3-[(2,3-cyclopentenopyridinium)methyl ceph-3-em-4carboxylate; (6R, 7R)-7-[(Z)-2-(2-aminothiazol-4-yi)-2cyclopropylmethoxyiminoacetamido]-3-pyridiniummethyl-ceph-3-em-4-carboxylate; and (613, 7R)-7-[(Z)-2-(2-aminothiazol-4yi)-2-methoxyiminoacetamido]-3-[(l-methyl-l-pyrrolidinium)-methyl]-ceph-3em-4-carboxylate.
Salts of the compounds of formula I which may be used, include: (a) inorganic base salts such as ammonium, alkali metal (e.g. potassium and sodium) or alkaline earth metal (e.g. calcium) salts, amino acid salts (e. g. lysine and arginine salts), and organic base salts such as procaine, phenylethylbenzylamine, dibenzylethylenediamine, ethanolamine, diethanolamine and N- methylglucosamine salts, and (b) acid addition salts formed with, for example, hydrochloric, hydrobromic, sulphuric, nitric, phosphoric, formic, trifluoroacetic, p-toluenesulphonic and methanesulphonic acids.
Important solvates include the hydrates.
The process according to the invention thus enables the efficient and simple separation of geometrical isomers of oxime group-containing compounds to be achieved by a-method capable of large-scale operation.
The following Examples serve to illustrate the invention. All temperatures are in C.
Example 1 Separation of isomers of Sodium (6R, 7R)-3carbamoyloxymethyl-7-[2-(fur-2-yi)-2-methoxyiminoacetamido]ceph-3-em-4-carboxylate A mixture of sodium (6R, 711)-3-carbamoy- loxymethyi-7-[2-)fur-2-yi)-2-methoxyiminoacetamido]ceph-3-em-4-carboxylate, syt--isomer (27.81 g) (added as the tetrahydrofuran sol- 70 vate) and its corresponding antisomer (6.03 g) was dissolved in water (300 mi). The solution was loaded at 500 ml/hour on a column containing Amberlite XAD-1 180 resin (500 mi). All the cephalosporin was retained 75 on the resin, none being detected in the percolate, which was discarded. The resin was then eluted with water at 500 ml/hour and the eluate collected in fractions. Each fraction was examined using HPLC for the presence of 80 the syn and anffisomers. The early eluate fractions were combined together (total volume 750 mi); methyl acetate (750 mi) and sodium chloride (150 g) were added with stirring. Whilst continuing stirring, 15% v/v sulphuric acid was added to pH 2.0. After stirring for a further 10 minutes at pH 2.0, the lower aqueous phase was separated and extracted with a second portion of methyl acetate (100 ml). The methyl acetate fractions 90 were combined and sodium 2-ethythexanoate solution was added to pH 5.5 The resultant slurry was filtered. The filter cake was washed with methyl acetate and dried overnight in vacuo at 40. The dry product (24.33 g) was 95 found to contain 22.0 g of sodium (611, 7R) 3-carbamoyloxymethyl-7-[2-(fur-2-yi)-2-methoxyiminoacetamido]ceph-3-em-4-carboxyi- ate, syn-isomer and 0. 1 g of the correspond- ing anti isomer.
Example 2 Separation of isomers of (6R, 7R)-7-[2-(fur-2yl)-2methoxyiminoacetamido]-3-hydroxyme- thylceph-3-em-4-carboxylic acid.
A sample of (6R, 7R)-7-[2-(fur-2-yi)-2-methoxyiminoacetamido]-3hydroxymethylceph3-em-4-carboxylic acid containing the syn isomer (33.2 g) and the anti isomer (3.72 g) was dissolved in water (about 500 mi) by adding sodium bicarbonate to pH 7.0 with stirring. The hazy solution was filtered and adjusted to pH 5.0 using sulphuric acid. This solution (about 600 mi) was loaded at 500 ml/hour on a column containing Amberlite XAD-1 180 resin (500 mi). All the cephalosporin was retained on the resin, none being detected in the percolate, which was discarded. The resin was efuted with water at 500 ml/hour and the eluate collected in fractions. Each fraction was examined using HPLC for the presence of the syn and anti isomers. The early eluate fractions were combined together (total volume 1300 mi) and cooled with stirring to 5'. Ethyl acetate (180 mi) was added followed by 20% v/v sulphuric acid to pH 2.3. The resulting slurry was stirred at 50 for 40 minutes, filtered, washed with chilled water (6 X 50 mi) and transferred to an open tray for drying overnight in vacuo at 40. The GB 2 146 330A 5 dry product (28.38 g) was found to contain 28.01 g of (611, 7R)-7-[2-(fur2-yl)-2-methoxyiminoacetamido]-3-hydroxymethylceph-3-em4-carboxylic acid, syn isomer and 0.09 g of the corresponding anti isomer.
Example 3 Separation of Isomers of Sodium (6R, 7R)-3carbamoyloxymethyi- 7[2-fur-2-yl)-2-methoxyiminoacetamido]ceph-3-em-4-carboxylate.
A mixture of sodium (6R, 7R)-3-carbamoyloxymethyi-7-[2-(fur-2-y])-2methoxyiminoacetamido]ceph-3-em-4-carboxylate, syn isomer (27.81 g) and the corresponding anti isomer (6.03 g) (added as the tetrahydrofuran solvate) was dissolved in water (300 mi). The solution was loaded at 500 ml/hour on a column containing Diaion HP-20 resin (500 mi). All the cephalosporin was retained on the resin, none being detected in the percolate, which was discarded. The resin was eluted with water at 500 m]/hour and the eluate collected in fractions. Each fraction was examined using HPLC for the presence of the syn and anti isomers. The early eluate fractions were combined together (total volume 610 mi); methyl acetate (750 m]) and sodium chloride (120 g) were added with stirring. Whilst continuing stirring, 15% v/v sulphuric acid was added to pH 2.0. After stirring for 10 minutes at pH 2. 0, the lower aqueous phase was separated and extracted with a second portion of methyl acetate (100 ml). The methyl acetate fractions were combined and sodium 2-ethy[hexanoate solution was added to pH 5.5. The resultant slurry was filtered. The filter cake was washed with methyl acetate and dried overnight in vacuo at 40'. The dry product (23.99 9) was found to contain 21.9 9 of sodium (6R, 711)-3-carbamoyloxymethyi-7-[2-(fur-2-yi)-2methoxyiminoacetamido]ceph-3-em-4-carboxylate, syn isomer and 0.41 g of the corresponding anti isomer.
Example 4 Separation of Isomers of sodium (617, 7R)-3carbamoyloxy-methyl7-[2-(fur-2-yl)-2-methoxyiminoacetamidolceph-3-em-4-carboxylate A mixture of sodium (611, 7R)-3-carbamoy- foxy methyl-7-[2-(fu r-2-yi)-2-methoxyi m in oacetamido]ceph-3-em-4- carboxylate, syn-isomer (27.59 9) and the corresponding anffisomer (5.38 g) as the tetrahydrofuran solvate was dissolved in water (300 mi). The solution was loaded at 250 ml/hour to a column containing Mitsubishi SP 207 resin (250 mi). All the cephalosporin was retained on the resin, none being detected in the percolate, which was discarded. The resin was eluted with water at 250 ml/hour and the eluate collected in fractions. Each fraction was examined using HPLC for the presence of the syn and anffisomers. The early eluate fractions were combined to- gether (total volume 400 mi); methyl acetate 6 GB 2 146 330A 6 (750 mi) and sodium chloride (80 g) were added with stirring. Whilst continuing stirring, 15% v/v sulphuric acid was added to pH 2.0. After stirring for 10 minutes at pH 2.0, the lower aqueous phase was separated and extracted with a second portion of methyl acetate (100 m[). The methyl acetate fractions were combined and sodium 2-ethyl hexanoate solution was added to pH 5.5. The resultant slurry was filtered, washed with methyl acetate and dried overnight in vacuo at 4WC. The dry product (20.24 9) was found to contain 18.09 9 of sodium (611, 7R)-3-carbamoyloxymethyi-7-[2-(fur-2-y])-2-methoxyiminoacetamido]ceph-3-em-4-carboxylate, syri.. isomer and 0.43 g of the corresponding ant isomer.
Example 5
Separation of Isomers of sodium (617, 7R)-7[2-(fur-2-yi)-2-methoxyiminoacetamido]-3-acetoxymethylceph-3-em-4-carboxylate A mixture of sodium (6R, 7R)-3-acetoxymethyl-7-[2-(fur-2-yi)-2- methoxyimino-acetamido]ceph-3-em-4-carboxylate, syn-isomer (added as the dioxan solvate) (21.9 g) and the corresponding antisomer (3.2 g) was prepared in water (250 ml) at pH 6.0. The solution was loaded at 1,000 ml/hour to a column con- taining Rohm and Haas XAD 1180 resin (500 ml). All of the cephalosporin was retained on the resin, none being detected in the percolate, which was discarded. The resin was eluted with water at 1,000 mi/hour and the eluate collected in fractions. Each fraction was examined using H PLC for the presence of the syn and anti isomers. The early eluate frac tions were combined together (total volume 1,735 ml) and found to contain 17.5 g of the syn isomer and 0.2 g of the anti isomer. This 105 fraction (1684 ml) was concentrated in vacuo to give a solution that was about 10% w/v cephalosporin compound.
The concentrated solution (10 w/v) was extracted into dichloromethane (2 X 150 m1s) 110 at pH 2.0. The organic extract was then evaporated to a solid which was redissolved using industrial methylate spirits (I IVIS) (180 MIS).
A solution of sodium 2-ethyl hexanoate (8.4 115 g) was added to the solution of cephalosporin acid and the mixture was stirred for 18 hours.The solid was filtered, washed with IMS, and dried in vacuo at 40C. The dried solution (75.5% yield from the aqueous col- 120 umn eluate) was pure sodium (6R, 7R)-7-[2 (fur-2-yl)-2-methoxyiminoacetamido]-3-acetoxymethylceph-3-em-4-carboxylate syn isomer containing 0.7% w/w anti isomer.
Example 6
Separation of Isomers of Sodium (6R, 717)-7 [2-(fur-2-yi)-2-methoxyiminoacetamidol3-acetoxymethylceph-3-em-4-carboxylate A mixture of sodium (6R, 7R)-3-acetoxyme-130 thyl-7-[2-(fur-2-yi)-2-methoxyiminoacetamido]ceph-3-em-4-carboxylate syn isomer (added as the dioxan solvate) (21.9 g) and the corresponding anti isomer (3.2 g) was prepared in water (250 ml) at pH 6.0. The solution was loaded at 1,000 mi/hour to a column containing Rohm and Haas XAD 1180 resin (500 mi). All of the cephalosporin was retained on the resin, none being detected in the percolate, which was discarded. The resin was eluted with 6% v/w methanol water at 1,000 ml/hr and the eluate collected in fractions. Each fraction was examined using HPLC for the presence of the syn and anti isomers. The early eluate fractions were combined together (total volume 1480 ml) and found to contain 18.2 g of the syn isomer and 0.2 g of the anti isomer. This fraction (1428 ml) was concentrated in vacuo to give a solution that was about 10% w/v cephalosporin compound.
The concentrated solution (10 w/v) was extracted into dichloromethane (2 X 150 mls) at pH 2.0. The organic extract was then evaporated to a solid which was redissolved using IMS (180 m1s).
A solution of sodium 2-ethyl hexanoate (8.4 g) was added to the solution of cephalosporin acid and the mixture was stirred for 18 hours. The solid was filtered, washed with IMS, and dried in vacuo at 40C. The dried solution (79.3% yield from the aqueous column eluate) was pure sodium (613, 7R)-7-[2-(fur-2-yI)2-methoxyi m inoaceta m ido]-3-acetoxym ethylceph-3-em-4-carboxylate syn isomer contain- ing 1.0% w/w anti isomer. Example 7 Separation of Isomers of (617, 7R)-7-2-(2-aminothiazol-4-yi)-2-
(2-carboxyprop-2-oxyimino)acetamido-3-(l-pyridiniummethyl)ceph-3-em4carboxylate A mixture of (613, 7R)-[2-(2-aminothiazol-4yi)-2-(2-carboxyprop-2- oxyimino)acetamido]-3(1 -pyridinium-methyl)ceph-3-em-4-carboxylate, syn isomer (21.1 g) and the corresponding anti isomer (0.8 g) was dissolved in water (250 ml) at pH 6.0. The solution was loaded at 500 ml/hour to a column containing Rohm and Haas XAD 1180 resin (500 ml). All the cephalosporin was retained on the resin, none being detected in the percolate, which was discarded. The resin was eluted with water at 500 mi/hour and the eluate collected in fractions. Each fraction was examined using HPLC for the presence of syn and anti isomers. The early eluate fractions were combined together (total volume 590 mi) and contained 81. 7% of the input syn Isomer. A portion of the eluate (500 ml) was adjusted to pH 6.0 with phsophoric acid and freeze-dried to a solid of 99.98% syn, 0.2% anti geometric isomer composition.
Example 8 Separation of Isomers of 2-(Fur-2yl)-2-me- 7 GB 2 146 330A 7 thoxyimino-acetic acid A mixture of ammonium 2-(fur-2-yi)-2-methoxyiminoacetate, syn isomer (5.50 9) and 2 (fur-2-yi)-2-methoxyiminoacetic acid, anti isomer (0.50 g) were dissolved in water and the pH of the solution adjusted to 3.0 to give 81 m] of solution. The solution was passed at mi/hour down a column containing Am berlite XAD-1 180 resin (100 mi). The column was then eluted with water at 100 ml/hour. 75 The eluate from the column was collected in fractions and each fraction examined using H PLC for the presence of the syn and anti isomers. The early eluate fraction (183 mi) contained 82% of the syn isomer originally present (contaminated with 3% of anti isomer). The 2-(fur-2-yi)-2-methoxyiminoacetic acid syn isomer was recovered from these early fractions by extraction into dichlorometh ane at pH 0.2. Evaporation of the dried 85 organic extract yielded a solid which was contaminated with 2% of the anti isomer.
Example 9
Separation of Isomers of (6R, 7R)-7-[(2-aminothiazol-4-yl)-2-cyclopropyimethoxyiminoacetamido]-3-(1-pyridiniummethyl)ceph-3-em-4- carboxylate A mixture of (611, 7R)-[2-(2-aminothiazol-4- yi)-2-eyclopropyimethoxyiminoacetamido]-3(1 -pyri d in i u m methyl)-cep h-3-em-4-ca rboxyl ate syn isomer (added as the bis-ethylene glycol solvate) (9.07 g) and the corresponding anti isomer (1.56 g) was prepared in water (102 mi) at pH 4.2. The solution was loaded at 200 ml/hour to a column containing Rohm and Haas XAD 1180 resin (200 mi). All of the cephalosporin was retained on the resin, none being detected in the percolate, which was discarded. The resin was washed with water (200 mi) at 200 mi/hour and then eluted with 30% methanol-water at 200 ml/hour and the eluate collected in fractions. Each fraction was examined using HPLC for the presence of the syn and anti isomers. The early eluate fractions were combined together (total volume 450 mi) and found to contain 7.37 g of the syn isomer and no anti isomer. This bulked fraction was evaporated in vacuo to remove methanol and freeze-dried to a solid that contained no anti isomer.
Example 10 Separation of Isomers of (R, S)- 1 -Acetoxye- thyl, 3-carbamoyloxymethyl-7-[2-(fur-2-yl)-2- methoxyimi ' noacetamido]-ceph-3-em-4-car boxylate A mixture of (R,S)-1-acetoxyethyi,3-carbamoyloxymethyi-7-[2-(fur-2-yi)-2- methoxyiminoacetamido]ceph-3-em-4-carboxylate syn isomer (20.13 g) and the corresponding anti isomer (1.08 9) was prepared in N,N-dimethylacetamide (40 mi). The solution was loaded at 500 mi/hr to a column containing Rohm and Haas XAD 1180 resin (500 mi). Water (750 mi) was passed down the column at 500 mi/hr to remove the N,N- dimethylacetamide. All the cephalosporin was retained on the column, none being detected in the perco- late, which was discarded. The resin was eluted with 60% v/v methanol/water at 500 mi/hour and the eluate collected in fractions. Each fraction was examined using HPLC for the presence of syn and anti isomers. Fractions totalling 1,800 mi rich in syn isomer were combined and evaporated in vacuo to a volume of 500 mi. this was then extracted twice with ethyl acetate (1 X 250 mi, 1 X 100 m]). The combined ethyl acetate ex- tracts were evaporated to 100 mi in vacuo and the concentrate seeded and stirred vigorously for 30 minutes. IMS (90 mi) was added followed by demineralised water (180 m]) and the mixture concentrated in vacuo to 240 mi. The suspension was stirred at 25'C for 30 minutes before filtering off the solid and washing with a mixture of water (117 mi) and IMS (17 mi). The product was dried in vacuo at 6WC. The solid was found to contain 6.16 9 (R,SJ-1 -acetoxylethyi,3-carbamoyloxymethyi-7-[2-(fur-2yi)-2-methoxyiminoaceta m i dolceph-3-em-4-ca rboxy late syn isomer and none of the corresponding anti isomer.
Example 11 Separation of Isomers of (R,S,)-l-acetoxyethyl 3carbamoyloxymethyl- 7-[2-(fur-2-y1)-2-methoxyiminoacetamido]-ceph-3-em-4carboxylate A mixture of (R,S)-l-acetoxyethyl 3-carbamoyloxymethyl-7-[2-(fur-2-yl)-2- methoxyiminoaceta m ido]ceph-3-e m-4-ca rboxyl ate syn isomer (20.93 g) and the corresponding anti isomer (2.15 g) was prepared in N,N-dimethy- lacetamide (40 ml). The solution was loaded at 500 ml/hour to a column containing Rohm and Haas XAD 1180 resin (500 ml). Water (750 ml) was passed down the column at 500 ml/hr to remove the N,N-dimethylace- tamide. All the cephalosporin was retained on the column, none being detected in the percolate, which was discarded. The resin was eluted with 60% v/v methanol water at 500 ml/hr and the eluate collected in fractions.
Each fraction was examed using HPLC for the presence of syn and anti isomers. Fractions rich in syn isomer totalling 1,700 mi were combined and evaporated in vacuo to a volume of 500 mi. This was then extracted twice with ethyl acetate (1 X 250 mi, 1 X 100 ml). The combined ethyl acetate extracts were evaporated to 100 mi in vacuo and the concentrate seeded and stirred vogorously for 1 hour. The resulting suspension was stored overnight. IMS (90 ml) was added followed by water (180 ml) and the mixture concentrated in vacuo to 240 mi. The suspension was stirred at 25C for 30 minutes before filtering off the solid and washing with a mixture of water (117 mi) and IMS (17 mi).
8 GB 2 146 330A 8 The product was dried in vacuo at WC. The solid was found to contain 8.50 g (R,S)-1 acetoxyethyl 3-carbamoyloxymethyi-7-[2-(fur 2-yi)-2-methoxyiminoacetamido]ceph-3-em-4carboxylate syn isomer and the corresponding 70 anti isomer (0. 16 g).
Example 12
Separation of isomers of (617, 7R)-7-[2-(2 aminothiazol-4-yl)-2-cyclopropyimethoxyiminoacetamidol-3-(1-pyridinium-methyl)-ceph-3- em-4-carboxylate A mixture of (611, 7R)-7-[2-(2-aminothiazol 4-yi)-2-cyclopropyimethoxyiminoacetamido]-3- (1 -pyrid in i u m methyl)-ceph-3-e m-4-ca rboxyl ate, 80 syn isomer (added as the bis-ethylene glycol solvate) (9.22 g) and the corresponding anti isomer (1.29 g) was prepared in water 104 mi) at pH 4. 1. The solution was loaded at 20 200 mi/hr to a column containing Rohm and 85 Haas XAD 7 resin (200 mi). All the cephalosporin was retained on the resin, none being detected in the percolate, which was discarded. The resin was eluted with water at 200 mi/hr and the eluate collected in frac tions. Additional fractions were also collected using 10% v/v methanol-water eluant at a rate of 400 ml/hr. Each fraction was exam ined using HPLC for the presence of syn and anti isomers. The eluate fractions were com- 95 bined together (total volume 1364 mi) and found to contain 6.28 9 of the desired syn isomer and no detected anti isomer.
Example 13 Separation of isomers of sodium (617, 7R)-7[2-(2-aminothiazol4-yl)-2-methoxyiminoacetamidol-3-acetoxymethyf-ceph-3-em-4-carboxylate A mixture of sodium (6R, 7R)-7-[2-(2-ami nothiazol-4-yi)-2-methoxyiminoacetamido]-3acetoxymethylceph-3-em-4-carboxylate syn isomer (5.15 9) and the corresponding anti isomer (0.40 g) was prepared in water (106 m[) at pH 5.5. The solution was loaded at 240 m[/hr to a column containing Rohm and Haas XAD 1180 resin (120 mi). All of the cephalosporin was retained on the resin, none being detected in the percolate, which was discarded. The Resin was eluted with water at 240 mi/hr and the eluate collected in fractions. Each fraction was examined using HPLC for the presence of syn and anti isomers. The early eluate fractions were combined together (total volume 420 mi) and found to contain 4.44 g of the syn isomer and not more than 0.02 9 of the anti isomer.
Example 14
Separation of isomers of sodium (6R, 7R)-7[2-(2-aminothiazol-4-yi)-2-methoxyiminoace- tamido]ceph-3-em-4-carboxylate A mixture of sodium (6R, 7R)-7-[2-(2-ami nothiazol-4-yi)-2-methoxyiminoacetamido]- ceph-3-em-4-carboxylate syn isomer (5.73 g) and the corresponding anti isomer (0.28 9) was prepared in water (153 ml) at pH 6.0. The solution was loaded at 240 m]/hr to a column containing Rohm and Haas XAD 1180 resin (120 mi). All the cephalosporin was retained on the resin, none being detected in the percolate which was discarded. The resin was eluted with water at 240 mi/hr and the eluate collected in fractions. Each fraction was examined, using HPLC, for the presence of the syn and anti isomers. The early eluate fractions were combined together (total volume 360 mi) and found to contain 5.69 g of syn isomer and no detected anti isomer.

Claims (10)

1. A process for the separation of a mixture of syn and anti oxime isomers one from the other which comprises adsorbing said mixed oxime isomers onto a non-functional macroreticular adsorption resin, and eluting said resin to yield at least one eluate fraction containing one of said isomers substantially 90 free of the other of said isomers.
2. A process as claimed in claim 1, wherein the syn and anti oxime are isomers of a cephalosporin compound possessing an oxime grouping in a side-chain in the 713-position thereof.
3. A process as claimed in claim 1, wherein the syn and anti oximes are isomers of a compound of general formula R-C-COR 2 11 N ? 1 OR (1) (wherein each of R and R' independently represents a hydrogen atom or an organic group and R 2 represents a hydroxy group or the residue of a 7-aminocephem-4-carboxylic acid) or a derivative thereof.
4. A process as claimed in any preceding claim, wherein the syn and anti oximes are isomers of a water-soluble cephalosporin compound of general formula R - C 0. NH 11 1 R' 3 3 N --N R COOH (where each of R, R' and R 3 independently represents a hydrogen atom or an organic group, B is -S- or 9 GB 2 146 330A 9 S->0 (a- or P-) and the dotted line indicates A2 or A 3 unsaturation) or of an ester, salt or solvate thereof.
5. A process as claimed in claim 3 on claim 4 for the separation of syn and anti oxime isomers of a compound of formula I or formula 11 or an ester, salt or solvate thereof wherein R is selected from carbocyclic groups and heterocyclic groups; these being unsatu- rated or aromatic and any heterocyclic groups possessing 5 to 6 ring members and containing from 1 to 4 heteroatoms selected from sulphur nitrogen and oxygen, the above groups optionally being substituted, or R is selected from optionally substitutedCl-6 alkyl groups.
6. A process as claimed in claim 3 on claim 4 for the separation of syn and anti oxime isomers of a compound of formual I or formula 11 or an ester, salt or solvate thereof wherein RI represents a hydrogen atom, a C5-10 aryl or C5-,, aralkyl group or an aliphatic group selected from C,-, alkyl, C3-1 cycloalkyl, C,-,, cycloalkylalkyl, C2-, alkenyl and C4-1 CY_ cloalkenyl group, wherein each of the above groups may be optionally substituted be a free or blocked carboxy, carbamoyl, cyano or protected or unprotected amino group.
7. A process as claimed in claim 4 for the separation of syn and anti oxime isomers of a compound of formula 11 or an ester, salt or solvate thereof wherein R 3 represents a hydrogen atom; a vinyl group substituted by a heterocyclicthio group in which the heterocy- clic portion comprises a 5- or 6-membered ring containing up to four nitrogen atoms and optionally one sulphur atom and substituted by one or more groups independently selected from methyl- protected or unprotected oxo, formylmethyl, protected or unprotected hydroxy and free or blocked carboxymethyl groups; or a group of formula -CH,Y (wherein Y represents a halogen atom, a hydroxy, acyloxy or carbarnoyloxy group or the residue of pyridine, 2,3-cyclopentenopyridine, nicotinamide or isonicotinamide or of a heterocyclicthiol comprising a 5- or 6- membered heterocyclic portion containing up to four nitrogen atoms and optionally one sulphur atom and substituted by one or more groups independently selected from methyl, protected or unprotected oxo, formylmethyl, carbamoyimethyl protected or unprotected hydroxy and free or blocked carboxymethyl groups).
8. A process as claimed in any preceding claim for the separation of syn and anti oxime isomers of a compound selected from the following: cefuroxime and its 3-acetoxymethyl and 3-hydroxymethyl analogues; ceftazidime; ceftizoxime; ceftriaxone; cefotaxime; cefmenoxime; cefodizime; cefpirome; (611, 7R)-7[(Z)-2-(2-aminothiazol-4-yi)-2-methoxyiminoacetamidol-3-[2-(5,6-dioxo-4formylmethyl1,4,5,6-tetrahydro-1,2,4-triazin-3-yl)thiovinyl]ceph-3-em-4carboxylic acid; (613, 7R)-7-[(Z)-2(2-aminothiazol-4-yl)-2(carboxymethoxyimi- no)acetamido]-3-vinyl-ceph-3-em-4-carboxylic acid; (611, 7R)-7-[(Z)-2-(2aminothiazol-4-yi)-2cyclopropylmethoxyiminoacetamido]-3-pyridinium-methylceph-3-em-4-carboxylate; and (613, 7R)-7-[(Z)-2-(2-aminothiazol-4-yl)-2me- thoxyiminoacetamido]-3-[(l-methyl-l-pyrrolidinium)methyl]-ceph-3-em-4-carboxylate or an acid corresponding to the 7-side chain thereof or of a salt of said compound or side chain acid.
9. A process as claimed in any preceding claim wherein the non-functional macroreticu lar resin a copolymer of styrene cross linked with divinyl benzene or an acrylic ester poly mer.
10. A process as claimed in any preceding claim wherein the oxime isomers are soluble in aqueous media and elution is effected us ing an aqueous eluant.
Printed in the United Kingdom for Her Majesty's Stationery Office, Dd 8818935, 1985, 4235. Published at The Patent Office. 25 Southampton Buildings, London, WC2A lAY, from which copies may be obtained.
GB08422611A 1983-09-09 1984-09-07 Separating syn and anti oxime isomers Expired GB2146330B (en)

Applications Claiming Priority (1)

Application Number Priority Date Filing Date Title
GB838324152A GB8324152D0 (en) 1983-09-09 1983-09-09 Chemical process

Publications (3)

Publication Number Publication Date
GB8422611D0 GB8422611D0 (en) 1984-10-10
GB2146330A true GB2146330A (en) 1985-04-17
GB2146330B GB2146330B (en) 1986-10-08

Family

ID=10548522

Family Applications (2)

Application Number Title Priority Date Filing Date
GB838324152A Pending GB8324152D0 (en) 1983-09-09 1983-09-09 Chemical process
GB08422611A Expired GB2146330B (en) 1983-09-09 1984-09-07 Separating syn and anti oxime isomers

Family Applications Before (1)

Application Number Title Priority Date Filing Date
GB838324152A Pending GB8324152D0 (en) 1983-09-09 1983-09-09 Chemical process

Country Status (9)

Country Link
US (2) US4717768A (en)
JP (1) JPS60190782A (en)
BE (1) BE900544A (en)
CH (1) CH662560A5 (en)
DE (1) DE3432984A1 (en)
FR (1) FR2551749B1 (en)
GB (2) GB8324152D0 (en)
IT (1) IT1178418B (en)
NL (1) NL8402738A (en)

Families Citing this family (8)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
GB8324152D0 (en) * 1983-09-09 1983-10-12 Glaxo Group Ltd Chemical process
DE3650526T2 (en) * 1985-08-12 1996-10-31 Upjohn Co CONVERSION OF THE CEPHALOSPORINE HYDROHALIDE SALT TO AN ALKALINE METAL SALT
GB8524001D0 (en) * 1985-09-30 1985-11-06 Glaxo Group Ltd Pharmaceutical composition
EP0658558B1 (en) 1993-11-17 2001-01-24 Biochemie Gesellschaft M.B.H. Separation of cephalosporin isomers
CN109553629B (en) * 2018-12-26 2020-06-23 浙江永宁药业股份有限公司 Preparation method of cefuroxime sodium intermediate E-type impurity compound
CN110627813A (en) * 2019-09-27 2019-12-31 广州白云山天心制药股份有限公司 Preparation method of cefuroxime axetil methoxyimino isomer
CN110627814A (en) * 2019-09-27 2019-12-31 广州白云山天心制药股份有限公司 Preparation method of cefuroxime sodium methoxyimino isomer
CN112574232B (en) * 2020-12-29 2022-04-15 山东金城昆仑药业有限公司 Method for recovering cefuroxime acid from cefuroxime acid waste residue liquid

Family Cites Families (7)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US4028355A (en) * 1974-01-23 1977-06-07 Smithkline Corporation Cephalosporin purification process
CA1046052A (en) * 1974-03-28 1979-01-09 Masaru Kurita Process for the purification of fr-1923 substance
DK162391C (en) * 1976-04-12 1992-03-09 Fujisawa Pharmaceutical Co ANALOGY PROCEDURE FOR PREPARING SYN-ISOMERS OF 3,7-DISUBSTITUTED 3-CEPHEM-4-CARBOXYLIC ACID COMPOUNDS
JPS5829079B2 (en) * 1976-04-20 1983-06-20 藤沢薬品工業株式会社 Separation and purification method of cephalosporin compounds
US4339390A (en) * 1979-09-18 1982-07-13 Abbott Laboratories Preferential immunoreactivity of syn-isomer of cortisol derivative
US4399274A (en) * 1981-07-02 1983-08-16 Merck & Co., Inc. Isolation of non-ionic lipophilic materials on macroreticular polymeric absorbents
GB8324152D0 (en) * 1983-09-09 1983-10-12 Glaxo Group Ltd Chemical process

Also Published As

Publication number Publication date
US4717768A (en) 1988-01-05
FR2551749B1 (en) 1986-10-31
GB8324152D0 (en) 1983-10-12
US4876351A (en) 1989-10-24
JPS60190782A (en) 1985-09-28
GB2146330B (en) 1986-10-08
IT8448814A0 (en) 1984-09-07
GB8422611D0 (en) 1984-10-10
BE900544A (en) 1985-03-11
NL8402738A (en) 1985-04-01
FR2551749A1 (en) 1985-03-15
DE3432984A1 (en) 1985-03-28
IT1178418B (en) 1987-09-09
IT8448814A1 (en) 1986-03-07
CH662560A5 (en) 1987-10-15

Similar Documents

Publication Publication Date Title
JPH0567632B2 (en)
CA1213883A (en) Cephalosporin derivatives
JPS5946954B2 (en) Antibiotic manufacturing method
GB2146330A (en) Separating syn and anti oxime isomers
JPH0262557B2 (en)
JPH07188250A (en) Separation of cephalosporin isomer
KR100515273B1 (en) Process for the selective preparation of z-isomers of 3-(2-substituted vinyl)cephalosporins
NZ203312A (en) Cephalosporin derivatives and pharmaceutical compositions
US3167549A (en) Derivatives of 7-aminocephalosporanic acid
KR930007416B1 (en) Process for preparing 3-(substituted) propenylaminothiazolyl cephalosporanic acids
US5869649A (en) Process for producing cephalosporin antibiotics
JP3547141B2 (en) Purification method
AU690482B2 (en) Process for producing cephalosporin antibiotics
US3644347A (en) 3-aminomethyl cephalosporin compounds
US4028355A (en) Cephalosporin purification process
JPH0240676B2 (en)
US3928333A (en) Process for the preparation of 3 cephalosporin esters
US4145539A (en) Process for isolation and purification of cephalosporin compound
US4168375A (en) Process for the recovery of cephalosporin C and derivatives thereof
EP0186586B1 (en) Cephem compounds and the production thereof
KR840002046B1 (en) Process for preparing cepharosporins
GB2218095A (en) Cepholosporin isomerisation
BE882359A (en) CEPHALOSPORIN TYPE ANTIBIOTICS AND PROCESS FOR THE PREPARATION
US2980700A (en) Process of gibberellic acid purification
SU814279A3 (en) Method of preparing 7-/2-oxyimino-2-(2-aminothiazol-4-yl)-acetamido/-2-methyl-3-cepheme-4-carboxlic acid derivatives in the form of sin-isomers or their salts

Legal Events

Date Code Title Description
PCNP Patent ceased through non-payment of renewal fee