CA2159627C - Novel prednisolone derivatives - Google Patents
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- CA2159627C CA2159627C CA002159627A CA2159627A CA2159627C CA 2159627 C CA2159627 C CA 2159627C CA 002159627 A CA002159627 A CA 002159627A CA 2159627 A CA2159627 A CA 2159627A CA 2159627 C CA2159627 C CA 2159627C
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Abstract
Epimers of the compound having the formula (I) are disclosed, both in their pure form and mixed in any desired mix ratio.
Description
2159~~'~
_ BILE, P~-i~1 Tf~~J ~:~;~:.
- WO 94/22899 -TRANSLATION pCT/$p94/01015 Novel prednisolone derivatives Field of at~plication of the invention The invention relates to novel prednisolone derivatives which are used in the pharmaceutical industry for the production of medicaments.
Known technical background DE-OS 41 29 535 discloses pregna-1,4-diene-3,20-dione-16,17-acetal-21-esters which carry a butyl, iso-propyl, sec-butyl, cyclohexyl or phenyl radical on the cyclic acetal ring, and whose C-21 hydroxyl group is acylated by an acetyl or isobutyryl radical.
Description of the invention It has now been found that the following com pounds according to the invention, which differ from the compounds of DE-OS 41 29'535 by the missing acyl radical on the C-21 hydroxyl group, have surprising and advanta-geous properties.
The invention relates to the epimers of the compound of the formula I (see accompanying formula sheet) in pure form, and to mixtures of these epimers in any desired mixture ratio.
The epimers of the compound of the formula I can be characterized by the formulae Ia and Ib (see accom-panying formula sheets).
The invention further relates to a process for the preparation of the compounds according to the inven-tion. The process comprises reacting 16-hydroxyprednisol-one with cyclohexanecarboxaldehyde.
The reaction is carried out in a manner known per se to the person skilled in the art in suitable solvents such as ethers, e.g. dioxane, diisopropyl ether, esters, e.g. ethyl acetate, halogenated hydrocarbons, e.g.
methylene chloride, chloroform, nitrated hydrocarbons, e.g. nitromethane, or without solvents, with addition of catalytic or even larger amounts of acid, such as mineral acids, e.g. perchloric acid, hydrochloric acid, tetrafluoroboric acid, or sulfonic acids, e.g. methane-sulfonic acid, at temperatures of, preferably, 0 to 60°C.
Preferably, the reaction to give the epimer mixture (formula I) in dioxane or ethyl acetate is carried out using 70o strength perchloric acid or 85~ strength tetrafluoroboric acid at 0°C to room temperature.
The reaction of 16-hydroxyprednisolone with cyclohexanecarboxaldehyde as a rule yields an epimer mixture, it being possible by means of suitable variation of the reaction conditions to control the reaction in such a way that a specific epimer mainly results.
To prepare mainly the R epimer (formula Ia), the following conditions, for example, are preferred:
halogenated hydrocarbons or nitromethane with methane-sulfonic acid at room temperature to 40°C, or 35-70~
strength perchloric acid at 0°C to room temperature. A
further possibility of preparing mainly the R epimer consists in the treatment of the epimer mixture (formula I) with 70% strength perchloric acid in a suitable solvent, e.g. methylene chloride, at 0°C (epimerization).
Preparation mainly of the S epimer (formula Ib) is achieved with the aid of hydrogen chloride gas in a solvent such as, for example, dioxane at 0°C to room temperature.
If an epimer is desired in purer form than is achievable on the basis of the reaction conditions, suitable separation and purification steps, for example preparative HPLC can be added after the reaction.
The following examples serve to illustrate the invention in greater detail:
Examples 1. 500 mg (1.3 mmol) of 16-hydroxyprednisolone are suspended in 5 ml of nitromethane and treated with 33 ~.1 (0.38 mmol) of 70~ strength perchloric acid and 195 ~.1 (1.6 mmol) of cyclohexanecarboxaldehyde. After stirring at room temperature for 4.5 h (epimer ratio in the reaction mixture R/S - 55:45, HPLC content 95%), the 2I~962'~
reaction mixture is treated with sodium hydrogen carbon-ate solution, and the precipitate is filtered off with suction, washed with water and nitromethane and dried at 50°C in a high vacuum. Yield: 440 mg (70%), epimer ratio R:S - 57:43 (determined by means of HPLC, stationary phase ODS Hypersil, mobile phase water/ethanol = 60:40).
_ BILE, P~-i~1 Tf~~J ~:~;~:.
- WO 94/22899 -TRANSLATION pCT/$p94/01015 Novel prednisolone derivatives Field of at~plication of the invention The invention relates to novel prednisolone derivatives which are used in the pharmaceutical industry for the production of medicaments.
Known technical background DE-OS 41 29 535 discloses pregna-1,4-diene-3,20-dione-16,17-acetal-21-esters which carry a butyl, iso-propyl, sec-butyl, cyclohexyl or phenyl radical on the cyclic acetal ring, and whose C-21 hydroxyl group is acylated by an acetyl or isobutyryl radical.
Description of the invention It has now been found that the following com pounds according to the invention, which differ from the compounds of DE-OS 41 29'535 by the missing acyl radical on the C-21 hydroxyl group, have surprising and advanta-geous properties.
The invention relates to the epimers of the compound of the formula I (see accompanying formula sheet) in pure form, and to mixtures of these epimers in any desired mixture ratio.
The epimers of the compound of the formula I can be characterized by the formulae Ia and Ib (see accom-panying formula sheets).
The invention further relates to a process for the preparation of the compounds according to the inven-tion. The process comprises reacting 16-hydroxyprednisol-one with cyclohexanecarboxaldehyde.
The reaction is carried out in a manner known per se to the person skilled in the art in suitable solvents such as ethers, e.g. dioxane, diisopropyl ether, esters, e.g. ethyl acetate, halogenated hydrocarbons, e.g.
methylene chloride, chloroform, nitrated hydrocarbons, e.g. nitromethane, or without solvents, with addition of catalytic or even larger amounts of acid, such as mineral acids, e.g. perchloric acid, hydrochloric acid, tetrafluoroboric acid, or sulfonic acids, e.g. methane-sulfonic acid, at temperatures of, preferably, 0 to 60°C.
Preferably, the reaction to give the epimer mixture (formula I) in dioxane or ethyl acetate is carried out using 70o strength perchloric acid or 85~ strength tetrafluoroboric acid at 0°C to room temperature.
The reaction of 16-hydroxyprednisolone with cyclohexanecarboxaldehyde as a rule yields an epimer mixture, it being possible by means of suitable variation of the reaction conditions to control the reaction in such a way that a specific epimer mainly results.
To prepare mainly the R epimer (formula Ia), the following conditions, for example, are preferred:
halogenated hydrocarbons or nitromethane with methane-sulfonic acid at room temperature to 40°C, or 35-70~
strength perchloric acid at 0°C to room temperature. A
further possibility of preparing mainly the R epimer consists in the treatment of the epimer mixture (formula I) with 70% strength perchloric acid in a suitable solvent, e.g. methylene chloride, at 0°C (epimerization).
Preparation mainly of the S epimer (formula Ib) is achieved with the aid of hydrogen chloride gas in a solvent such as, for example, dioxane at 0°C to room temperature.
If an epimer is desired in purer form than is achievable on the basis of the reaction conditions, suitable separation and purification steps, for example preparative HPLC can be added after the reaction.
The following examples serve to illustrate the invention in greater detail:
Examples 1. 500 mg (1.3 mmol) of 16-hydroxyprednisolone are suspended in 5 ml of nitromethane and treated with 33 ~.1 (0.38 mmol) of 70~ strength perchloric acid and 195 ~.1 (1.6 mmol) of cyclohexanecarboxaldehyde. After stirring at room temperature for 4.5 h (epimer ratio in the reaction mixture R/S - 55:45, HPLC content 95%), the 2I~962'~
reaction mixture is treated with sodium hydrogen carbon-ate solution, and the precipitate is filtered off with suction, washed with water and nitromethane and dried at 50°C in a high vacuum. Yield: 440 mg (70%), epimer ratio R:S - 57:43 (determined by means of HPLC, stationary phase ODS Hypersil, mobile phase water/ethanol = 60:40).
2. 2.0 g (5.3 mmol) of 16-hydroxyprednisolone are suspended in 20 ml of nitromethane and treated with 0.88 ml (10.2 mmol) of 70% strength perchloric acid and 0.78 ml (6.4 mmol) of cyclohexanecarboxaldehyde. After stirring at room temperature for 5 h (epimer ratio in the reaction mixture R:S - 73:27, HPLC content 95%), the reaction mixture is worked up as in Example 1. Yield:
1.96 g (78%), epimer ratio R:S = 76:24.
1.96 g (78%), epimer ratio R:S = 76:24.
3. 2.0 g (5.3 mmol) of 16-hydroxyprednisolone are suspended in 10 ml of nitromethane and 1.5 ml (17.4 mmol) of 70% strength perchloric acid and 0.8 ml (6.6 mmol) of cyclohexanecarboxaldehyde is subsequently added dropwise.
The mixture is stirred at room temperature for 2 h (epimer ratio in the reaction mixture R:S = 92:8, HPLC
content 98%) and worked up as in Example 1. Yield: 2.2 g (88%), epimer ratio R:S = 92:8.
The mixture is stirred at room temperature for 2 h (epimer ratio in the reaction mixture R:S = 92:8, HPLC
content 98%) and worked up as in Example 1. Yield: 2.2 g (88%), epimer ratio R:S = 92:8.
4. 2.0 g (5.3 mmol) of 16-hydroxyprednisolone are suspended in 20 ml of nitromethane and treated with 3.52 ml (41 mmol) of 70% strength perchloric acid and 0.78 ml (6.4 mmol) of cyclohexanecarboxaldehyde. After stirring at room temperature for 1 h, the mixture is added to sodium hydrogen carbonate solution, extracted with methylene chloride, and the organic phase is dried With sodium sulfate and concentrated in vacuo. The residue is chromatographed on silica gel using methylene chloride/ethyl acetate - 1:1 (Rf=0.5). Yield: 1.0 g (40%), epimer ratio R:S = 89:11.
5. 20 g (53 mmol) of 16-hydroxyprednisolone are suspended in 300 ml of chloroform, treated with 8.0 ml 2~59fi~~
WO 94/22899 - 4 - PCT/$P94/01015 (66 mmol) of cyclohexanecarboxaldehyde, and 17.6 ml (205 mmol) of 70% strength perchloric acid are added dropwise with cooling in an ice bath. After stirring at room temperature for 2.5 h, the reaction mixture is added to sodium carbonate solution, and the organic phase is extracted with water, dried using sodium sulfate and concentrated in vacuo (epimer ratio in the crude product R:S = 85:15). The residue is dissolved in warm ethanol, the solution is treated with water until it becomes turbid and cooled in the ice bath, and the precipitate is filtered off With suction and dried. Yield: 20.2 g (81%), epimer ratio R:S = 85:15.
WO 94/22899 - 4 - PCT/$P94/01015 (66 mmol) of cyclohexanecarboxaldehyde, and 17.6 ml (205 mmol) of 70% strength perchloric acid are added dropwise with cooling in an ice bath. After stirring at room temperature for 2.5 h, the reaction mixture is added to sodium carbonate solution, and the organic phase is extracted with water, dried using sodium sulfate and concentrated in vacuo (epimer ratio in the crude product R:S = 85:15). The residue is dissolved in warm ethanol, the solution is treated with water until it becomes turbid and cooled in the ice bath, and the precipitate is filtered off With suction and dried. Yield: 20.2 g (81%), epimer ratio R:S = 85:15.
6. 5.0 g (13.3 mmol) of 16-hydroxyprednisolone are suspended in 100 ml of methylene chloride, treated with 4.4 ml (51.2 mmol) of 70% strength perchloric acid and 2.1 ml (17.3 mmol) of cyclohexanecarboxaldehyde. After 1.25 h, the reaction mixture is added to sodium carbonate solution, and the organic phase is washed with water, dried using magnesium sulfate and concentrated in vacuo.
z Crude yield quantitative, HPLC content 96%, epimer ratio R:S = 89:11.
z Crude yield quantitative, HPLC content 96%, epimer ratio R:S = 89:11.
7. 300 g (797 mmol) of 16-hydroxyprednisolone are suspended in 3.0 1 of ethyl acetate, treated with 120 ml (991 X01) of cyclohexanecarboxaldehyde and 150 ml (1.75 mol) of 70% strength perchloric acid are added dropwise in the course of 20 min. After stirring for 1 h the solution is treated with 250 g of sodium carbonate and stirred with 1.5 1 of water. The aqueous phase is extracted with ethyl acetate, and the collected organic phases with saturated sodium chloride solution. After drying the organic phase with sodium sulfate, the mixture is slowly concentrated in vacuo, and the resulting solid is filtered off with suction, washed with diethyl ether and dried. Yield: 282 g (75%), epimer ratio R:S = 58:42.
8. 10.0 g (26.6 mmol) of 16-hydroxyprednisolone are suspended in 100 ml of dioxane while cooling in an ice 21~96~r bath, treated with 8.8 ml (102.4 mmol) of 70~ strength perchloric acid and 3.7 ml (30.5 mmol) of cyclohexane-carboxaldehyde are added dropwise in the course of 45 min. The mixture is stirred at room temperature for 2 h, neutralized with sodium carbonate solution and extracted with methylene chloride. The organic phase is washed with water, dried using sodium sulfate and concentrated in vacuo (epimer ratio in the crude product R: S - 49 : 51) .
The residue is taken up in warm ethanol and fractionally crystallized by adding water and cooling in an ice bath.
1st fraction: 8.5 g, epimer ratio R:S - 60:40. 2nd fraction: 2.5 g, epimer ratio R:S - 27:73. Total yield:
11 g (88~).
9. 0.5 g (1.3 mmol) of 16-hydroxyprednisolone is suspended in 20 ml of diisopropyl ether at room temperature and treated with 190 ~C1 (1.56 mmol) of cyclohexanecarboxaldehyde and 440 ~,1 (5.1 mmol) of 70%
strength perchloric acid. After 45 min, the reaction mixture is treated with ethyl acetate and extracted with sodium hydrogen carbonate solution and water. The organic Y phase is dried using magnesium sulfate and concentrated in vacuo. Crude yield quantitative; HPLC content 95~, epimer ratio R:S = 57:43.
The residue is taken up in warm ethanol and fractionally crystallized by adding water and cooling in an ice bath.
1st fraction: 8.5 g, epimer ratio R:S - 60:40. 2nd fraction: 2.5 g, epimer ratio R:S - 27:73. Total yield:
11 g (88~).
9. 0.5 g (1.3 mmol) of 16-hydroxyprednisolone is suspended in 20 ml of diisopropyl ether at room temperature and treated with 190 ~C1 (1.56 mmol) of cyclohexanecarboxaldehyde and 440 ~,1 (5.1 mmol) of 70%
strength perchloric acid. After 45 min, the reaction mixture is treated with ethyl acetate and extracted with sodium hydrogen carbonate solution and water. The organic Y phase is dried using magnesium sulfate and concentrated in vacuo. Crude yield quantitative; HPLC content 95~, epimer ratio R:S = 57:43.
10. 2.0 g (5.3 mmol) of 16-hydroxyprednisolone are suspended in 20 ml of nitromethane at room temperature and treated with 1.4 ml (21.5 mmol) of methanesulfonic acid and 0.78 ml (6.4 mmol) of cyclohexanecarboxaldehyde.
The solution is stirred at 40°C for 3 h and diluted with methylene chloride after cooling. The reaction mixture is extracted with sodium hydrogen carbonate solution and water, and the organic phase is dried using sodium sulfate and concentrated in vacuo. The residue is chromatographed as in Example 4. Yield: 1.7 g (680), epimer ratio R:S = 85:15.
The solution is stirred at 40°C for 3 h and diluted with methylene chloride after cooling. The reaction mixture is extracted with sodium hydrogen carbonate solution and water, and the organic phase is dried using sodium sulfate and concentrated in vacuo. The residue is chromatographed as in Example 4. Yield: 1.7 g (680), epimer ratio R:S = 85:15.
11. 5.0 g (13.3 mmol) of 16-hydroxyprednisolone are suspended in 50 ml of methylene chloride, treated with 21~962~~
WO 94/22899 - 6 - PCT/$P94/01015 3.45 ml (53.1 mmol) of methanesulfonic acid while cooling in an ice bath, and 1.95 ml (16.1 mmol) of cyclohe-xanecarboxaldehyde are added dropwise in the course of min. The mixture is allowed to come to room 5 temperature and is then stirred at 40°C for 3 h. The solution is extracted with water, dried using sodium sulfate and concentrated in vacuo. Crude yield quanti-tative, HPLC content 96~, epimer ratio R:S = 85:15.
WO 94/22899 - 6 - PCT/$P94/01015 3.45 ml (53.1 mmol) of methanesulfonic acid while cooling in an ice bath, and 1.95 ml (16.1 mmol) of cyclohe-xanecarboxaldehyde are added dropwise in the course of min. The mixture is allowed to come to room 5 temperature and is then stirred at 40°C for 3 h. The solution is extracted with water, dried using sodium sulfate and concentrated in vacuo. Crude yield quanti-tative, HPLC content 96~, epimer ratio R:S = 85:15.
12. 10.0 g (26.6 a~ol) of 16-hydroxyprednisolone are 10 suspended in 60 ml of 70~ strength perchloric acid while cooling in an ice bath and treated with 3.7 ml (30.5 amnol) of cyclohexanecarboxaldehyde in the course of 10 min. After stirring for 30 minutes with ice-cooling, the mixture is added to ice-cooled sodium hydrogen carbonate solution and extracted with ethyl acetate. The organic phase is washed with sodium hydrogen carbonate solution and water, dried using sodium sulfate and concentrated in vacuo (epimer ratio in the crude product R:S = 93:7). The residue is purified as in Example 8. 1st fraction: 2.1 g, epimer ratio R:S - 94.5:5.5, 2nd frac-tion: 6.56 g, epimer ratio R:S - 96:4, 3rd fraction:
1.29 g, epimer ratio R:S = 91.5:8.5. Total yield: 9.95 g (79.50 .
In the case of corresponding reaction of the starting materials in 50 or 35~ strength perchloric acid, an epimer ratio of R:S = 95:5 or 81:19 is obtained in the crude product.
1.29 g, epimer ratio R:S = 91.5:8.5. Total yield: 9.95 g (79.50 .
In the case of corresponding reaction of the starting materials in 50 or 35~ strength perchloric acid, an epimer ratio of R:S = 95:5 or 81:19 is obtained in the crude product.
13. 5.0 g (13.3 mmol) of 16-hydroxyprednisolone are suspended in 80 ml of dioxane while cooling in an ice bath, treated with 2.5 ml of 85~ strength tetrafluoro-boric acid in diethyl ether, and 1.95 ml (16.1 mmol) of cyclohexanecarboxaldehyde are added in the course of 10 min. The mixture is stirred at room temperature for 1 h, then poured into sodium hydrogen carbonate solution and extracted with ethyl acetate. The organic phase is extracted with water, dried using sodium sulfate and concentrated in vacuo. The residue is chromatographed as 215962' WO 94/22899 - 7 - PCT/$P94/01015 in Example 4. Yield: 4.0 g (64%), epimer ratio R:S -47:53.
14. 100 mg (0.27 mmol) of 16-hydroxyprednisolone are suspended in 5 ml of nitromethane, treated with 50 ~.1 of 85% strength tetrafluoroboric acid in diethyl ether and 35 ~.l (0.29 mmol) of cyclohexanecarboxaldehyde, and stirred at room temperature for 15 h. Epimer ratio of the reaction mixture R:S - 80:20, HPLC content 96%. The adjustment of the epimer ratio can also be achieved by heating the reaction solution at 60°C for 30 min.
15. 2.0 g (5.3 mmol) of 16-hydroxyprednisolone are suspended in 40 ml of dioxane, treated with 760 ~,1 (6.3 mmol) of cyclohexanecarboxaldehyde while cooling in an ice bath, and 15 ml of 14.8% strength hydrogen chloride gas/dioxane solution are added dropwise in the course of 20 min. After stirring at 0°C for 2 h and at room temperature for 2 h, tfie mixture is added to sodium hydrogen carbonate solution and extracted with ethyl acetate. The organic phase is washed with water, dried z using sodium sulfate and concentrated in vacuo. The residue is chromatographed as in Example 4. Yield: 620 mg (25%), epimer ratio R:S = 25:75.
16. 12.0 g (25.5 mmol) of l6a,17-cyclohexylmethylene-dioxy-11(3,21-dihydroxypregna-1,4-diene-3,20-dione (compound I, epimer ratio R:S - 60:40) are dissolved in 240 ml of methylene chloride at 0°C, treated with 8.7 ml (101.1 mmol) of 70% strength perchloric acid and added to sodium hydrogen carbonate solution after stirring for 40 min. The aqueous phase is extracted with methylene chloride, and the collected organic phases are extracted with water and dried using magnesium sulfate. After concentrating the solvent in vacuo, the compound I is quantitatively recovered With an epimer ratio of R:S -90:10 (HPLC content 98%) .
17. Separation of the epimers (starting from any desired i epimer mixture) can be achieved with the aid of HPLC, for example as follows:
Equipment: HP 10848 liquid chromatograph, HP 79850E LC
terminal and UV detector; column material: Hypersih C18, 12 jcm, 250 x 20 mm; eluent: water (59%) /ethanol (41%) ;
detector wavelength: 242 am; sample concentration: 220 mg in 600 ~Cl of DMSO + 3800 ~Cl of ethanol; application volume: 200 ~C1 - 10 mg of epimer mixture; flow rate:
ml/min; oven temperature: 40°C; purity achieved: R
10 epimer 99.6%, S epimer 99.4%.
Industrial utility The compounds according to the invention have useful pharmacological properties, Which make them industrially utilizable. They are generally suitable for I5 the treatment of those disease conditions which can be treated by steroidal antiinflammatories. These primarily include disorders of the skin and of the respiratory tract, but also inflammatory bowel disorders and allergic rhinitis/conjunctivitis.
In the skin area, the compounds according to the invention are suitable on account of their antiinflam-matory, antiproliferative, immunosuppressive, antipruri-ginous and vasoconstrictory properties for the (in particular topical) treatment of dermatoses of varying origin. Examples which may be mentioned are: allergic contact eczema, atopic eczema, seborrhoeic eczema, lichen simplex, psoriasis (vulgaris), sunburn, pruritus in the anogenital area, alopecia areata, hypertrophic scars and discoid lupus erythematosus.
In the respiratory tract area, the compounds according to the invention suppress nearly all inflamma-tory reactions occurring in the wall of the airways by inhibiting the proliferation, differentiation, migration and activation of the inflammatory cells and also the formation of prostaglandins, leukotrienes and PAF. As a result, the compounds according to the invention reduce bronchial hyperreactivity, decrease mucus formation, .- 2159627 - WO 94/22899 - 9 - PCT/$P94/01015 improve mucociliary clearance and potentiate (partly by increased expression of ~B-adrenoreceptors) the action of ~B-sympathomimetics. As a result of these properties, the compounds according to the invention are primarily suitable (topically applied in inhalant form) for the (long-term) therapy of bronchial asthma.
The compounds according to the invention are distinguished by a low toxicity, an essentially topical activity, a wide therapeutic spectrum, a long-lasting action and the absence of significant side effects. The activity of the compounds according to the invention makes possible their use in human and veterinary medicine.
The invention therefore further relates to a .
process for the treatment of mammals, including humans, who are affected by one of the abovementioned diseases.
The process comprises administering to the affected mammal a therapeutically active and pharmacologically tolerable amount of one or more of the compounds accord ing to the invention.
The invention further relates to the compounds according to the invention for use in the treatment and/or prophylaxis of said diseases.
The invention likewise relates to the use of the compounds according to the invention for the production of medicaments which are employed for the treatment and/or prophylaxis of said diseases.
The invention furthermore relates to medicaments for the treatment and/or prophylaxis of said diseases, which contain one or more of the compounds according to the invention.
For the treatment of dermatoses, the administra-tion of the compounds according to the invention is carried out. in particular, in the form of those medica-ments which are suitable for topical application. For the production of the medicaments, the compounds according to the invention (= active compounds) are preferably mixed with suitable pharmaceutical auxiliaries and additionally processed to give suitable pharmaceutical formulations.
2~~962'~
Examples of suitable pharmaceutical formulations which may be mentioned are powders, emulsions, suspensions, sprays, oils, ointments, fatty ointments, creams, pastes, gels or solutions.
On account of his expert knowledge, the person skilled in the art is familiar with the auxiliaries which are suitable for the desired pharmaceutical formulations.
In addition to solvents, gel-forming agents, ointment bases and other active compound excigients, antioxidants, dispersants, emulsifiers, preservatives, solubilizers or permeation promoters can be used.
For the treatment of disorders of the respiratory tract, the compounds according to the invention are preferably applied in inhalant form. For this purpose, the latter are either administered directly as powders, (preferably in micronized form) or by atomizing solutions or suspensions which contain them. With respect to the preparations and administration forms, reference is made, for example, to the embodiments in European Patent 163 965.
The medicaments according to the invention are prepared by processes known per se. The active compounds are administered in the quantity customary for highly active glucocorticoids. Topical application forms (e. g.
ointments) for the treatment of dermatoses thus contain the active compounds in a concentration of, for example, 0.1-l0. The dose for application in inhalant form is customarily between 0.2 and 2 mg per day. The customary (maintenance) dose in systemic therapy is approximately 10 mg per day, it being possible in the case of severe asthma attacks and in particular in status asthmaticus for significantly higher doses. (e. g. 250-500 mg i.v.) also to be used.
Pharmacolo Experimental procedure for recording the local and systemic action of the compounds to be tested on granulation tissue formation after cotton pellet implan-tation in the rat (cotton pellet method):
Male Sprague-Dawley rats (in each case 8-16 21~9~27 A
- WO 94/22899 - 11 - PCT/$P94/01015 animals per dose; weight per animal: 180-230 g) are each given one cotton ball (manufacturer: Hartmann, Heidenheim; cotton balls Size 2, No. 4865/2) of 13.0 ~ 0.5 mg, subcutaneously implanted bilaterallv in the shoulder blade area under isofluorane anesthesia and under sterile conditions. Before the start of the experiment, alcoholic solutions (0.05 ml/pellet; 96%
strength alcohol) of the compounds to be tested are in each case instilled into the cotton balls intended for implantation in the left side of the body. At the time of implantation, the pellets are dry, i.e. the substances have been deposited on the cotton fibers. The pellets on the right side of the body are implanted untreated.
In the course of 7 days, granulomas are formed as a result of foreign body irritation. On the 8th day, these are carefully excised from the sacrificed animals, i.e. with protection of the connective tissue capsule, dried (15 h at 120°C) and weighed. By subtraction of the proportion by weight of the cotton balls, the amount of the newly formed granulation tissue is obtained.
The percentage reduction of the mean granuloma dry weight of a treated group compared with the control group (= 100%) is used as a measure of the antiprolifer-ative action of a compound.
The local action of a compound is recorded on the left granulomas, and the systemic action on the right.
For recording the systemic corticoid action, the fresh weights of thymus and adrenal were also determined.
Table Antiproliferative action of the compounds according to the invention after local administration in the chronic inflammation model (measured by the effect on granulation tissue formation after s.c. cotton pellet implantation (so-called cotton pellet test)) 21~~~27 - WO 94/22899 - 12 - PCT/$P94/01015 Compound Dose Inhibition of n 1 x granulation tissue (number of formation animals) (mg per % p animal) (signifi Local* cance) Ia 0.2 69 < 0.001 8 Ib 0.2 32 < 0.001 8 * Instilled into the left pellet
Equipment: HP 10848 liquid chromatograph, HP 79850E LC
terminal and UV detector; column material: Hypersih C18, 12 jcm, 250 x 20 mm; eluent: water (59%) /ethanol (41%) ;
detector wavelength: 242 am; sample concentration: 220 mg in 600 ~Cl of DMSO + 3800 ~Cl of ethanol; application volume: 200 ~C1 - 10 mg of epimer mixture; flow rate:
ml/min; oven temperature: 40°C; purity achieved: R
10 epimer 99.6%, S epimer 99.4%.
Industrial utility The compounds according to the invention have useful pharmacological properties, Which make them industrially utilizable. They are generally suitable for I5 the treatment of those disease conditions which can be treated by steroidal antiinflammatories. These primarily include disorders of the skin and of the respiratory tract, but also inflammatory bowel disorders and allergic rhinitis/conjunctivitis.
In the skin area, the compounds according to the invention are suitable on account of their antiinflam-matory, antiproliferative, immunosuppressive, antipruri-ginous and vasoconstrictory properties for the (in particular topical) treatment of dermatoses of varying origin. Examples which may be mentioned are: allergic contact eczema, atopic eczema, seborrhoeic eczema, lichen simplex, psoriasis (vulgaris), sunburn, pruritus in the anogenital area, alopecia areata, hypertrophic scars and discoid lupus erythematosus.
In the respiratory tract area, the compounds according to the invention suppress nearly all inflamma-tory reactions occurring in the wall of the airways by inhibiting the proliferation, differentiation, migration and activation of the inflammatory cells and also the formation of prostaglandins, leukotrienes and PAF. As a result, the compounds according to the invention reduce bronchial hyperreactivity, decrease mucus formation, .- 2159627 - WO 94/22899 - 9 - PCT/$P94/01015 improve mucociliary clearance and potentiate (partly by increased expression of ~B-adrenoreceptors) the action of ~B-sympathomimetics. As a result of these properties, the compounds according to the invention are primarily suitable (topically applied in inhalant form) for the (long-term) therapy of bronchial asthma.
The compounds according to the invention are distinguished by a low toxicity, an essentially topical activity, a wide therapeutic spectrum, a long-lasting action and the absence of significant side effects. The activity of the compounds according to the invention makes possible their use in human and veterinary medicine.
The invention therefore further relates to a .
process for the treatment of mammals, including humans, who are affected by one of the abovementioned diseases.
The process comprises administering to the affected mammal a therapeutically active and pharmacologically tolerable amount of one or more of the compounds accord ing to the invention.
The invention further relates to the compounds according to the invention for use in the treatment and/or prophylaxis of said diseases.
The invention likewise relates to the use of the compounds according to the invention for the production of medicaments which are employed for the treatment and/or prophylaxis of said diseases.
The invention furthermore relates to medicaments for the treatment and/or prophylaxis of said diseases, which contain one or more of the compounds according to the invention.
For the treatment of dermatoses, the administra-tion of the compounds according to the invention is carried out. in particular, in the form of those medica-ments which are suitable for topical application. For the production of the medicaments, the compounds according to the invention (= active compounds) are preferably mixed with suitable pharmaceutical auxiliaries and additionally processed to give suitable pharmaceutical formulations.
2~~962'~
Examples of suitable pharmaceutical formulations which may be mentioned are powders, emulsions, suspensions, sprays, oils, ointments, fatty ointments, creams, pastes, gels or solutions.
On account of his expert knowledge, the person skilled in the art is familiar with the auxiliaries which are suitable for the desired pharmaceutical formulations.
In addition to solvents, gel-forming agents, ointment bases and other active compound excigients, antioxidants, dispersants, emulsifiers, preservatives, solubilizers or permeation promoters can be used.
For the treatment of disorders of the respiratory tract, the compounds according to the invention are preferably applied in inhalant form. For this purpose, the latter are either administered directly as powders, (preferably in micronized form) or by atomizing solutions or suspensions which contain them. With respect to the preparations and administration forms, reference is made, for example, to the embodiments in European Patent 163 965.
The medicaments according to the invention are prepared by processes known per se. The active compounds are administered in the quantity customary for highly active glucocorticoids. Topical application forms (e. g.
ointments) for the treatment of dermatoses thus contain the active compounds in a concentration of, for example, 0.1-l0. The dose for application in inhalant form is customarily between 0.2 and 2 mg per day. The customary (maintenance) dose in systemic therapy is approximately 10 mg per day, it being possible in the case of severe asthma attacks and in particular in status asthmaticus for significantly higher doses. (e. g. 250-500 mg i.v.) also to be used.
Pharmacolo Experimental procedure for recording the local and systemic action of the compounds to be tested on granulation tissue formation after cotton pellet implan-tation in the rat (cotton pellet method):
Male Sprague-Dawley rats (in each case 8-16 21~9~27 A
- WO 94/22899 - 11 - PCT/$P94/01015 animals per dose; weight per animal: 180-230 g) are each given one cotton ball (manufacturer: Hartmann, Heidenheim; cotton balls Size 2, No. 4865/2) of 13.0 ~ 0.5 mg, subcutaneously implanted bilaterallv in the shoulder blade area under isofluorane anesthesia and under sterile conditions. Before the start of the experiment, alcoholic solutions (0.05 ml/pellet; 96%
strength alcohol) of the compounds to be tested are in each case instilled into the cotton balls intended for implantation in the left side of the body. At the time of implantation, the pellets are dry, i.e. the substances have been deposited on the cotton fibers. The pellets on the right side of the body are implanted untreated.
In the course of 7 days, granulomas are formed as a result of foreign body irritation. On the 8th day, these are carefully excised from the sacrificed animals, i.e. with protection of the connective tissue capsule, dried (15 h at 120°C) and weighed. By subtraction of the proportion by weight of the cotton balls, the amount of the newly formed granulation tissue is obtained.
The percentage reduction of the mean granuloma dry weight of a treated group compared with the control group (= 100%) is used as a measure of the antiprolifer-ative action of a compound.
The local action of a compound is recorded on the left granulomas, and the systemic action on the right.
For recording the systemic corticoid action, the fresh weights of thymus and adrenal were also determined.
Table Antiproliferative action of the compounds according to the invention after local administration in the chronic inflammation model (measured by the effect on granulation tissue formation after s.c. cotton pellet implantation (so-called cotton pellet test)) 21~~~27 - WO 94/22899 - 12 - PCT/$P94/01015 Compound Dose Inhibition of n 1 x granulation tissue (number of formation animals) (mg per % p animal) (signifi Local* cance) Ia 0.2 69 < 0.001 8 Ib 0.2 32 < 0.001 8 * Instilled into the left pellet
Claims (51)
1. A compound having Formula I
or 16.alpha.,17-(22R,S)-cyclohexylmethylenedioxy-11.beta.,21-dihydroxypregna-1,4-diene-3,20-dione.
or 16.alpha.,17-(22R,S)-cyclohexylmethylenedioxy-11.beta.,21-dihydroxypregna-1,4-diene-3,20-dione.
2. A compound having Formula Ia or 16.alpha.,17-(22R)-cyclohexylmethylenedioxy-11.beta.,21-dihydroxypregna-1,4-diene-3,20-dione.
3. A compound having Formula Ib or 16.alpha.,17-(22S)-cyclohexylmethylenedioxy-11.beta.,21-dihydroxypregna-1,4-diene-3,20-dione.
4. The compound defined in Claim 1, wherein the compound of Formula I
comprises an epimer mixture of the compound of formula Ia and the compound of formula Ib in any desired mixture ratio.
comprises an epimer mixture of the compound of formula Ia and the compound of formula Ib in any desired mixture ratio.
5. The use of the compound defined in any one of Claims 1-4 for the treatment of a skin disorder.
6. The use of the compound defined in any one of Claims 1-4 for the treatment of a respiratory tract disorder.
7. The use of the compound defined in any one of Claims 1-4 for the treatment of an inflammatory bowel disorder.
8. The use of the compound defined in any one of Claims 1-4 for the treatment of rhinitis/conjunctivitis.
9. The use of the compound defined in any one of Claims 1-4 for the treatment of dermatitis.
10. The use defined in Claim 9 for the treatment of one of allergic contact eczema, atopic eczema, seborrhoeic eczema, lichen simplex, psoriasis, sunburn, anogenital pruritus, alopecia areata, hypertrophic scars and discoid lupus erythematosus.
11. The use of the compound defined in any one of Claims 1-4 for the treatment of bronchial asthma.
12. The use of the compound defined in any one of Claims 1-4 for the prophylaxis of a skin disorder.
13. The use of the compound defined in any one of Claims 1-4 for the prophylaxis of a respiratory tract disorder.
14. The use of the compound defined in any one of Claims 1-4 for the prophylaxis of an inflammatory bowel disorder.
15. The use of the compound defined in any one of Claims 1-4 for the prophylaxis of rhinitis/conjunctivitis.
16. The use of the compound defined in any one of Claims 1-4 for the prophylaxis of dermatitis.
17. The use defined in Claim 16 for the prophylaxis of one of allergic contact eczema, atopic eczema, seborrhoeic eczema, lichen simplex, psoriasis, sunburn, anogenital pruritus, alopecia areata, hypertrophic scars and discoid lupus erythematosus.
18. The use of the compound defined in any one of Claims 1-4 for the prophylaxis of bronchial asthma.
19. A pharmaceutical composition comprising the compound defined in any one of Claims 1-4, together with a pharmaceutically acceptable excipient therefor.
20. A skin disorder treatment composition comprising the compound defined in any one of Claims 1-4, together with a pharmaceutically acceptable excipient therefor.
21. A respiratory tract treatment composition comprising the compound defined in any one of Claims 1-4, together with a pharmaceutically acceptable excipient therefor.
22. An inflammatory bowel disorder treatment composition comprising the compound defined in any one of Claims 1-4, together with a pharmaceutically acceptable excipient therefor.
23. A rhinitis/conjunctivitis treatment composition comprising the compound defined in any one of Claims 1-4, together with a pharmaceutically acceptable excipient therefor.
24. A dermatitis treatment composition comprising the compound defined in any one of Claims 1-4, together with a pharmaceutically acceptable excipient therefor.
25. The composition defined in Claim 24, wherein the dermatitis is one of allergic contact eczema, atopic eczema, seborrhoeic eczema, lichen simplex, psoriasis, sunburn, anogenital pruritus, alopecia areata, hypertrophic scars and discoid lupus erythematosus.
26. A bronchial asthma treatment composition comprising the compound defined in any one of Claims 1-4, together with a pharmaceutically acceptable excipient therefor.
27. A skin disorder prophylactic composition comprising the compound defined in any one of Claims 1-4, together with a pharmaceutically acceptable excipient therefor.
28. A respiratory tract prophylactic composition comprising the compound defined in any one of Claims 1-4, together with a pharmaceutically acceptable excipient therefor.
29. An inflammatory bowel disorder prophylactic composition comprising the compound defined in any one of Claims 1-4, together with a pharmaceutically acceptable excipient therefor.
30. A rhinitis/conjunctivitis prophylactic composition comprising the compound defined in any one of Claims 1-4, together with a pharmaceutically acceptable excipient therefor.
31. A dermatitis prophylactic composition comprising the compound defined in any one of Claims 1-4, together with a pharmaceutically acceptable excipient therefor.
32. The composition defined in Claim 31, wherein the dermatitis is one of allergic contact eczema, atopic eczema, seborrhoeic eczema, lichen simplex, psoriasis, sunburn, anogenital pruritus, alopecia areata, hypertrophic scars and discoid lupus erythematosus.
33. A bronchial asthma prophylactic composition comprising the compound defined in any one of Claims 1-4, together with a pharmaceutically acceptable excipient therefor.
34. The composition defined in any one of Claims 20-33 in the form of a topical formulation.
35. The composition defined in Claim 34, wherein the topical formulation contains the compound defined in any one of Claims 1-4 in a concentration of from 0.1 % to 1 %.
36. The composition defined in any one of Claims 20-33 in the form of an inhalant formulation.
37. The composition defined in any one of Claims 20-33 in the form of formulation selected from a powder, an emulsion, a suspension, a spray, an oil, an ointment, a fatty ointment, a cream, a paste, a gel and a solution.
38. The composition defined in any one of Claims 20-33 in the form of a micronized powder.
39. A process for the preparation of a compound of the Formula I
which comprises a reaction between 16-hydroxyprednisolone and cyclohexanecarboxaldehyde.
which comprises a reaction between 16-hydroxyprednisolone and cyclohexanecarboxaldehyde.
40. The process defined in Claim 39, wherein the reaction is conducted in the presence of a solvent.
41. The process defined in Claim 40, wherein the solvent is selected from the group comprising ether, ester, halogenated hydrocarbon, nitrated hydrocarbon and mixtures thereof.
42. The process defined in Claim 41, wherein the ether comprises at least one of dioxane and diisopropyl ether.
43. The process defined in Claim 41, wherein the ester comprises ethyl acetate.
44. The process defined in Claim 41, wherein the halogenated hydrocarbon comprises at least on of methylene chloride and chloroform.
45. The process defined in Claim 41, wherein the nitrated hydrocarbon comprises nitromethane.
46. The process defined in Claim 39, wherein the reaction is conducted in the absence of a solvent.
47. The process defined in any one of Claims 39-46, wherein the reaction is conducted in the presence of an acid.
48. The process defined in Claim 39-46, wherein the reaction is conducted in the presence of a catalytic amount of an acid.
49. The process defined in any one of Claims 47-48, wherein the acid comprises a mineral acid.
50. The process defined in any one of Claims 47-48, wherein the acid is selected from the group comprising perchloric acid, hydrochloric acid, tetrafluoroboric acid, sulfonic acid and mixtures thereof.
51. The process defined in any one of Claims 39-50, wherein the reaction is conducted at a temperature in the range of 0° to 60°C.
Applications Claiming Priority (3)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| CH1023/93-1 | 1993-04-02 | ||
| CH102393 | 1993-04-02 | ||
| PCT/EP1994/001015 WO1994022899A1 (en) | 1993-04-02 | 1994-03-31 | New prednisolone derivates |
Publications (2)
| Publication Number | Publication Date |
|---|---|
| CA2159627A1 CA2159627A1 (en) | 1994-10-13 |
| CA2159627C true CA2159627C (en) | 2006-05-23 |
Family
ID=36481340
Family Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| CA002159627A Expired - Lifetime CA2159627C (en) | 1993-04-02 | 1994-03-31 | Novel prednisolone derivatives |
Country Status (1)
| Country | Link |
|---|---|
| CA (1) | CA2159627C (en) |
-
1994
- 1994-03-31 CA CA002159627A patent/CA2159627C/en not_active Expired - Lifetime
Also Published As
| Publication number | Publication date |
|---|---|
| CA2159627A1 (en) | 1994-10-13 |
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