NO142914B - ANALOGY PROCEDURE FOR THE PREPARATION OF THERAPEUTICALLY EFFECTIVE CEPHALOSPORINES - Google Patents

Description

The present invention relates to the production of therapeutically active cephalosporins with the formula:

where R is thienyl or phenyl and R 2 is a pyridinium group, optionally substituted with -CONH 2 , or a thiazolium group, optionally substituted with -CH 2 and/or -CI 2 CH 2 OH. The invention also relates to the preparation of pharmaceutically acceptable salts thereof.

Ever since the discovery of cephalosporin C, various derivatives of cephalosporin-type antibiotics have been developed which are substituted in the 7- and 3-position. However, compounds active at practical concentrations against Pseudomonas aeruginosa have not yet been described.

It has now been found that the new cephalosporins represented by the above formula I are not only effective in the therapy of various infectious diseases from Gram-positive and Gram-negative pathogenic bacteria, but also show effects at low concentrations against Pseudomonas aeruginosa . In the cephalosporins with the formula I, the sulfonic acid group in the substituents in the 7-position is bound directly to an asymmetric carbon atom. It is therefore obvious that the cephalosporins produced according to the invention comprise the D-type, the L-type and the DL-type of the cephalosporin compounds.

The cephalosporins I are produced by introducing the oc-sulfoacyl group in the 7-position and by converting the acetoxy group in the 3-position to the nitrogen-containing heterocyclic group. The turnover can take place first in position 3 or 7, then followed by turnover in the other position. The method according to the invention is characterized by what is stated in the characterizing part of the claim.

A) Procedure for first carrying out reaction in the 7-position and then in the 3-position: 7-aminocephalosporanic acid (hereafter called "7-ACA") is reacted with a cc-sulfocarboxylic acid with the formula: or with a functional derivative thereof, whereby a cephalosporanic acid with the formula can be obtained:

(see Belgian patent no. 762,725). As long as it does not have any adverse effect on the subsequent conversion reaction in the 3-position, the carboxyl group in the 4-position and/or the sulfo group in the side chain can be in the form of a salt, e.g. with sodium, potassium, magnesium, calcium, aluminum or triethylamine. In some cases, the carboxyl group in the 4-position can be protected with an ester group that can be easily removed, e.g. a benzyl, β-methylsulfonylethyl, benzhydryl or trimethylsilyl group.

The sulfocephalosporanic acid II is then reacted with a nitrogen-containing heterocyclic compound R~ with the above meaning.

The reaction between the sulfocephalosporanic acid II and the nitrogen-containing heterocyclic compound R2 is carried out according to methods known per se. Usually it is advantageous to carry out the reaction in water or a strong polar solvent. The reaction is carried out at approximately neutral pH, preferably pH 5 - 8. Usually, the nitrogenous compound is used in proportions of around 1-10 mol per moles of sulfocephalosporanic acid. Furthermore, the reaction can be carried out in the presence of a catalyst such as isocyanate, thioisocyanate or thiol compounds in a proportion of about 1-40 mol, preferably about 5-20 mol per moles of sulfocephalosporanic acid II, whereby the final product can be obtained in high yield. The above-mentioned catalyst reacts with the group in the 3-position of the sulfocephalosporanic acid and forms a functional derivative. This functional derivative may or may not be isolated and reacted with the nitrogen-containing heterocyclic compound R^. The reaction temperature and reaction time vary depending on the type of reaction reagent and the type of solvent. In most cases, however, the reaction is carried out in a temperature range from room temperature to 100°C, preferably 40 - 70°C, for 1 - 48 hours. The thus obtained reaction product I is purified and recovered according to methods known per se, such as solvent extraction, concentration, chromatography, freeze-drying and recrystallization. B) Procedure for first carrying out the conversion in the 3-position and then in the 7-position: The conversion of the acetoxy group in the 3-position in cephalosporin C can be carried out according to the methods which e.g. is described in U.S. Patent No. 3,225,038 or 3,217,000 or German Patent No. 1,817,121. The resulting cephalosporin with the nitrogen-containing heterocyclic group in the 3-position can be easily converted into a corresponding aminocephalosporanic acid derivative of the formula:

according to the procedure as e.g. is described in Dutch

Patent No. 6,401,421, British Patent No. 1,041,985 or U.S. Pat. Patent No. 3,575,970. Alternatively, aminocephalosporanic acid derivative IV can be prepared by deacylation of cephalosporin C and then substitution in the 3-position of the resulting 7-ACA. Aminocephalosporanic acid derivative IV can exist in the form of salts and esters, such as the previously mentioned sulfocephalosporanic acid II.

The reaction of aminocephalosporanic acid deriv

IV with α-sulfocarboxylic acid V or a functional derivative thereof can also be carried out according to methods known per se. In the event that α-sulfocarboxylic acid V is used in free form, it is preferable to carry out the reaction in the presence of a condensing agent. The condensing agent can e.g. be N,N'-disubstituted carbodiimide, e.g. N,N'-dicyclohexylcarbodiimide; an azo lid compound, e.g. N,N'-thionylimidazole; N-ethoxy-carbonyl-2-ethoxy-1,2-dihydroquinoline, phosphorus oxychloride or alkoxyacetylene. As reactive ester of the acid V

carboxylic acid halides, anhydrides, azides and active esters can be used. The above-mentioned acylation reaction takes place advantageously and smoothly in a solvent. A normal solvent such as e.g. water, acetone, tetrahydrofuran, dioxane, acetonitrile, chloroform, dichloromethane, dichloroethylene, pyridine, dimethylaniline, dimethylformamide, dimethylacetamide or dimethylsulfoxide. The reaction temperature is not particularly limited. Usually, however, the reaction is carried out under cooling or at room temperature. The reaction product can be purified and recovered by exploiting the properties of the final product cephalosporin I, e.g. by column chromatography, extraction, precipitation at the isoelectric point, countercurrent distribution or recrystallization.

The cephalosporins I can be used in the same way as ordinary cephalosporins, although the use of these varies more or less depending on the type of nitrogenous heterocyclic group in the 3-position and/or the acyl group in the 7-position. The present compounds I are useful as pharmaceuticals as they have a strong antibacterial effect against a wide spectrum of pathogenic bacteria including Pseudomonas aeruginosa, against which they

similar cephalosporin preparations have essentially been ineffective.

The cephalosporins I produced according to the invention are usually administered in the same way as known cephalosporin preparations, but the dosage, dosage form etc. vary with the substituent groups in the 3-position and the acyl groups in the 7-position. E.g. the effective dose of sodium N-(α-sulfophenylacetamido)-cef-3-em-3-yl-methyl-7-pyridinium-4-carboxylate is about 0.25 g - 2.5 g every 4 to 6 .hour for an adult.

The compounds produced according to the present invention

was compared with typical compounds described in the widely available Norwegian soknad 471/71

These compounds were tested against the following microorganisms:

The microorganisms from (A) to (D) inclusive are Gram-positive bacteria; the microorganisms from (E) to (j) inclusive are Gram-negative bacteria.

The minimal inhibitory concentration, MIC, for each of the test compounds (DL form) was determined by the agar dilution method. Nutrient agar with a pH of 7.0 was used as the test medium. A lure of a cell suspension containing approx. 1 mg/ml of the sample microorganism was used as inoculum, and the sample microorganism was cultivated for 18 - 24 hours on the nutrient agar. The MIC values (mcg/ml) were determined after incubation at 37°C for 18 hours.

This superiority over Pseudomonas is unexpected to the person skilled in the art.

In the following examples, all temperatures are uncorrected.

Example 1

(1) Preparation of α-sulfobenzylcephalosporin:

A solution consisting of 2.5 ml of a 1N-NaOH solution and 5 ml of water is ice-cooled to 0 - 5°C after which 680 mg of 7-aminocephalosporanic acid was dissolved in the reading under thorough stirring. A solution of 585 mg of α-sulfophenylacetic acid chloride in 7 ml of diethyl ether was added dropwise to the resulting solution with stirring over the course of 15 minutes. Then the aqueous layer was separated, the pH value was adjusted to 1.5 by adding 1N-HCl and then it was extracted twice with 15 ml of n-butanol and the extract was washed twice with 5 ml each time of water and extra-hardened with a saturated aqueous NaHCO-^ solution. The resulting extract was adjusted to a pH value of 6.5, washed with ether and then subjected to lyophilization and 385 mg of the desired product in the form of the sodium salt was obtained.

IR vmax (cm<-1>): 1755 (lactam, acetate), 1612 (-CO0"), 1680 (-CONH-), 1225 (-SO2-), 1046 (-SO3Na).

NMR (D 2 O) ppm: 2.09 (3H, singlet), 3.42

(2H, quartet, J-^18.0 c/s, J"2=18.0 c/s), 4.75 (2H), 5.09 (1H, singlet), 5.10 (1H, doublet , J=4.5 c/s), 5.70 (1H, doublet, J=4.5 c/s), 7.52 (5H, multiplet).

UV*max: 259 m/u (7.1 x 10<5>)

(2) Preparation of sodium N-(α-sulfophenylacetamido)-cef-3-em-3-ylmethyl 7pyridinium-4-carboxylate: 0.355 g (6.9 x 10"<4> mol) 7-(a -sulfophenyl-acetamido)-cephalosporanic acid (α-sulfobenzylcephalosporin), 0.34 g (3.5 x 10~<5> mol) potassium thiocyanate and 0.15 ml (1.88 x 10<-5> mol) pyridine were dissolved in 0.75 ml of water (pH 6.5). The resulting solution was heated to 60°C for 6 hours, purified chromatographically using a resin column ("Amberlite XAD-2", 16 x 700 mm, eluent : water, under the control of an ultraviolet spectrometer (240 nyu)).The fractions containing the desired cephalosporin were collected and then freeze-dried to obtain 126 mg of the desired product.

IR^Scs (dm<_1>): 5400 (OH), 3020 (CH), 1760 ((3-lactam), 1670 (-C0NH-), 1610 (-C00<->), 1525 (shoulder), 1490 , 1380, 1350 (SO 2 ), 1220 (-60 2- ), 1037 (-SOg-), 700 (no -SCN detected).

NMR (60Mc, D2O): 3.02, 3.48 (2H, doublet, <J>1<=J>2=18 c/s, C2 methylene), 5.28, 5.40 (2H J— CH2 ~),

5.05 (H, singlet, -C<g>-CO-), 5.07 (1H, doublet, J=5.3

S0-.H

3 c/s, Cg proton), 5.68 (1H, doublet, J=5.3 c/s, C^ proton), 7.32, 7.45 (5H, phenyl proton), 7.8 - 9.0 (5H, multiplet, pyridine proton).

Minimum inhibitory concentration:

Example 2

0.292 g N-(7-aminocef-3-em-3-ylmethyl)pyridinium-

4-carboxylate and 0.17 g of sodium bicarbonate were dissolved in 7 ml of water. To the resulting solution, while cooling, 3 ml of a chloroform solution containing 0.234 g of α-sulfophenylacetyl chloride was added dropwise. After complete dropwise addition, stirring was continued further under cooling for 40 minutes to terminate the reaction. After removal of the organic layer, the aqueous layer was adjusted to a pH value of 6 and subjected to chromatography using "Amberlite XAD-2", and the resulting desired product-containing fractions were freeze-dried to obtain sodium-N-/? -(α-sulfophenylacetamido)cef-3-em-3-ylmethyl)pyridinium-4-carboxylate.

Example 3

Preparation of sodium N-7-(α-sulfophenylacetamido)cef-3-em-3-ylmethyl-4'-carbamoyl-pyridini-um-4-carboxylate': 0.514 g (1 x 10"<3> mol ) 7-(α-sulfophenylacetamido)cephalosporanic acid, 0.366 g (3 x 10~<10> mol) of isonicotinamide and 2.0 g (2.06 x 10 mol) of calcium thiocyanate were dissolved in 2.5 ml of water. The resulting solution was set aside and heated for 20 hours in a thermostat maintained at 50°C, and then purified directly chromatographically using an "Amberlite XAD-2" column (16 x 880 mm). Thereafter, the cephalosporin-containing fractions were collected and subjected to freeze drying and 270 g of the desired product was obtained in the form of a pale yellowish white powder.

BWmax (cm<-1>): 3330 (CH, NH), 3200 (OH, broad), 1765 (C=0, (3-lactam), 1680 (-C0NH-), 1610 (-C00~), 1552 (-NH2, deformation), 1455, 1390 (C=C, SO2), 1200 (SO2, broad), 1120, 1040 (-SO3"), 850, 810, 700.

NMR (60Mc, D90): 2.93 (1H, doublet, j=18 c/s,

, 3.52 (1H, doublet, J=18 c/s, , 5.08 (1H, singlet, 5.35 (1H,

CH2-), 5.50 (1H,

J=5 c/s, J_ CH2-), 5.09 (1H, doublet, J=6 c/s, 6-position proton), 5.71 (1H, -doublet, J=4.5 c/ s, 7-position proton), 7.25 - 7.6 (5H- multiplet, phenyl), 8.25 (2H, doublet, J=6.5 c/s, pyridine proton), 9.03

(2H, doublet, J=6.5 c/s, pyridine proton).

Minimum inhibitory concentration:

Example 4

Example 3 was repeated, except that nicotinamide was used instead of isonicotinamide. The minimum inhibitory concentration in yug/ml against Pseudomonas aeruginosa (Pd 1) for the resulting

connection with the group

was 1.

Example 5

Preparation of sodium 7-(α-sulfo-α-phenyl)-acetamido-3-(4'-methyl-5'-hydroxyethylthiazolium)cef-3-em-4-carboxylate: 500 mg (9.69 x 10_Zf mol) disodium 7-(α-sulfo-α-phenylacetamido)cephalosporanate, 1.68 g (1.73 x 10~<5> mol) KSCN and 415 mg (2.9 x 10 J mol) thiazole derivative were dissolved in 2 ml of water and allowed to react for 18 hours in a thermostat which was kept at 50°C. The solution thus obtained was subjected to chromatography using "Amberlite XAD-2" resin and frozen, and 264 mg of the above product was obtained in a yield of 42.8%.

IR\>5?L (cm<-1>)<:>3400, 3050, 1170, 1680,

1615, 1530, 1350, 1210, 1110, 1040, 700.

NMR (60Mc, D2O): 2.43 (3H, singlet,

Example 6

(1) While cooling and stirring, 1.84 g (0.0068 mol) of 7-ACA was suspended in 25 ml of water and to the suspension was added dropwise 6.8 ml of a 1N aqueous solution of sodium hydroxide to dissolve 7-ACA. On the other hand, it turned into a suspension of

1.5 g (0.0068 mol) of α-sulfo-3-thienylacetic acid in 10 ml of ether was added dropwise with 5.5 ml of thionyl chloride and 3 drops of dimethylformamide, and the resulting solution was stirred for 5 hours at room temperature. The reaction solution was subjected to evaporation to a tb'rr state under reduced pressure and α-sulfo-3-thienylacetyl chloride was obtained as a residue. The residue was dissolved in 10 ml of ethyl acetate and the solution was added dropwise to the 7-ACA solution mentioned above, followed by stirring for 30 minutes. The aqueous layer was separated from the reaction solution and adjusted to a pH value of 6.5 by addition of a saturated aqueous solution of NaHCO 3 . The resulting solution was purified by column chromatography using "Amberlite XAD-2" and 1.6 g (42%) of 7-(α-sulfo-3'-thienylacetamido)cephalosporanic acid was obtained.

1677 (-CONH-), 1605 (-COONa), 1225 (-SO^Na, -OAC), 1043 (SO,Na).

NMR δ(D 2 O): 2.13 (3H, singlet, -CO 2 CH ),

3.54 (2H, wide,

, 5.10 (1H, doublet, J=4.7, c/s,

in

5.24 (1H, singlet, -ChO, 5.70 (1H, dub-

IM

light, J=4.7 c/s,

), 7.38 - 7.67 (3H, multiplet, (2) 260 mg (0.5 x 10<-3> mol) 7-(α-sulfo-3-thienyl-acetamido)-cephalosporanic acid and 97 mg ( 1 x 10~<5> mol) KSCN was added to a solution of 240 mg (3 x 10~<5> mol) pyridine dissolved in 2 ml of water, and the resulting solution was allowed to stand for 24 hours at 40°C The reaction mixture was washed with ether. The aqueous layer was separated and purified by column chromatography using "Amberlite XAD-2" to obtain sodium N-[7-(α-sulfo-3-thienylacetamido)cef-3 -em-3-ylmethyl 7-pyridinium-4-carboxylate.

Minimum inhibitory concentration:

), 8.08 (2H, wide, ), 8.54 (1H, wide, , 8.91 (2H, wide,

Example 7

213 mg (2.5 x 10<-5> mol) thiazole, 97 mg (1 x 10"<5 >mol) KSCN and 260 mg (0.5 x 10"<3> mol) 7-(α-sulfo -3-thienylacetamido)cephalosporanic acid was completely dissolved in 0.8 ml of water. The solution was set at 50°C for 20 hours and then purified by column chromatography using "Amberlite XAD-2" and 80 mg of sodium N-[7-(α-sulfo-3'-thienylacetamido) was obtained. cef-3-em-3-ylmethyl7thiazolium-4-carboxylate.

i<R>^max (cm<-1>): 1757 (p-lactam), 1670 (-C0NH-, -N=C), 1617 (-COONa), 1038 (-SO^Na).

NMR δ (D 2 O): 3.5 (2H,

T T

), 5.1 (1H,

), 5.25 (1H, singlet, -CH< ), 5.3 (2H,

SO^Na

-CH2-N), 5.7 (1H, ), 7.37 - 7.6 (3H, thiophene), 8.15, 8.35, 10.0 (1H, each,

Example 8

420 mg (3 x 10~<3> mol) 4-(3-hydroxy-ethyl-5-methylthiazole, 485 mg (5 x 10~<5> mol) KSCN and 260 mg (0.5 x 10 _ - z mol) 7-(α-sulfo-3-thienylacetamido)-cephalosporanic acid was dissolved in 1 ml of water and the solution obtained in this way was placed at 50° C. for 10 hours. The reaction solution was purified by column chromatography

fi using "Amberlite XAD-2" and sodium-N-[7-(a-sulfo-3'-thienylacetamido)cef-3-em-yl-methyl7-4"-(3-hydroxyethyl-5 "-methyl-thiazolium-4-carboxylate.

IR^max (cm<_1>): 1760 (P-lactam), 1675

+

(-CONH-, -N=C), 1615 (-COONa), 1040 (-SO^Na).

NMR J(D 2 O): 2.43 (3H, singlet,

3.2 - 3.5 (4H, ), 3.84 (2H, triplet, J=4.5 c/s, , 5.1 (1H, doublet, J=4.9 c/s, , 5, 20 (1H, singlet, , 5.3 (2H, I CH2-N®), 5.70 (1H, doublet, J=4.9 c/s, 7.3 - 7.6 (3H, thiophene), 9.12 (1H, singlet.

Example 9

558 mg (2 x 10 mol) sodium 7-aminocephalosporanate, 790 mg (1 x 10~^ mol) pyridine and 1.94 g

(2 x 10~<5> mol) KSCN was dissolved in 2 ml of water and the resulting solution was placed at 50°C for 8 hours. The reaction solution was purified by column chromatography using "Amberlite XAD-2" to obtain pyridinium 7-aminocephalosporanate which was dissolved in 10 ml of water after which the solution was reacted with 235 mg of α-sulfo-3-thienyl-acetyl chloride to obtain sodium- N-/?-(α-sulfo-3'-thienyl-acetamido)cef-3-em-3-yl-methyl-7-pyridinium-4-carboxylate. This compound was identical to the product obtained in Example 6, as determined by IR and NMR spectroscopy.

Claims (1)

Analogy method for the production of terra therapeutically active cephalosporins of the general formula I where R is thienyl or phenyl and R2 is a pyridinium group which is optionally substituted with -CONH2, or a thiazolium group which is optionally substituted with -CFLj and/or -CH2CH2OH, or a pharmaceutically acceptable salt thereof, characterized in that ( 1) a sulfocephalosporanic acid with the general formula where R has the above meaning, or a salt • or an easily decomposable ester thereof, is reacted with a compound R2 with the above meaning; or (2) an aminocephalosporanic acid of the general formula where Rg has the meaning given above, or a salt or an easily decomposable ester thereof, is reacted with an α-sulfocarboxylic acid, or a functional derivative thereof, with the formula where R has the above meaning, after which any ester group is cleaved off, and, if desired, the compounds obtained are converted into a pharmaceutically acceptable salt.