CA2543629A1 - 2-phenyl-benzofuran derivatives, method for the production thereof and their use - Google Patents
2-phenyl-benzofuran derivatives, method for the production thereof and their use Download PDFInfo
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- C07—ORGANIC CHEMISTRY
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- C07D307/77—Heterocyclic compounds containing five-membered rings having one oxygen atom as the only ring hetero atom ortho- or peri-condensed with carbocyclic rings or ring systems
- C07D307/78—Benzo [b] furans; Hydrogenated benzo [b] furans
- C07D307/86—Benzo [b] furans; Hydrogenated benzo [b] furans with an oxygen atom directly attached in position 7
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- A61K31/335—Heterocyclic compounds having oxygen as the only ring hetero atom, e.g. fungichromin
- A61K31/34—Heterocyclic compounds having oxygen as the only ring hetero atom, e.g. fungichromin having five-membered rings with one oxygen as the only ring hetero atom, e.g. isosorbide
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- A61P31/00—Antiinfectives, i.e. antibiotics, antiseptics, chemotherapeutics
- A61P31/04—Antibacterial agents
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- C12R2001/00—Microorganisms ; Processes using microorganisms
- C12R2001/645—Fungi ; Processes using fungi
- C12R2001/66—Aspergillus
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Abstract
The invention relates to 2-phenyl-benzofuran compounds of formula (I), which are formed by the microorganism Aspergillus flavipes ST003878 (DSM 15290) during fermentation, to a method for the production thereof and to their use as medicaments for treating and/or preventing bacterial infectious diseases or mycoses.
Description
2-Phenylbenzofuran derivatives, a process for preparing them, and their use.
A, large number of antibiotics are employed therapeutically for treating infectious diseases caused by bacteria. However, the pathogens are becoming increasingly resistant to the drugs employed; there is even the threat of serious danger arising due to what are termed muitiresistant organisms, which have not merely become resistant to single antibiotic groups, such as ~3-lactam antibiotics, glycopeptides or macrolides, but in fact carry several resistances simultaneously. There even exist pathogens which have become resistant to all the antibiotics which are commercially available. It is no longer possible to treat infectious diseases which are caused by these organisms. For this reason, there is a great need for new compositions which can be used against resistant organisms. While many thousand antibiotics have been described in the literature, most of them are too toxic to be used as drugs.
The cell walls of Gram-positive and Gram-negative bacteria consist for the most part of peptidoglycan (murein), which, as what is termed the murein sacculus, encloses the cell completely and lends its mechanical stability as well as helping to determine its morphological form. Peptidoglycan is a macromolecule which is composed of an alternating sequence of the 1,4-~3-glycosidically linked amino sugars N-acetylglucosamine and N-acetylmuramic acid. Crosslinkings by way of short peptide bridges provide the sugar chains with a high degree of stability. The biosynthesis of peptidoglycan is catalyzed by a number of enzymes which are dissolved in cytoplasm or else membrane-bound. Many of these enzymes are specific to bacteria and represent ideal points of attack in the search for new antibiotics.
The bifunctional bacterial N-acetylglucosamine-1-phosphate uridyl-transferase (GImU) catalyzes the formation of UDP-N-acetylglucosamine from glucosamine-1-phosphate in a two-step reaction. UDP-N-acetyl-glucosamine is a fundamental building block in bacterial cell wall biosynthesis and inhibiting its formation is therefore a promising route for finding novel antibacterial therapeutic agents (Sulzenbacher et al., J. Biol.
Chem. 2001, 276 (15), 11844-11851 ).
There have already been reports of compounds from cultures of Aspergillus flavipes, such as flavipin (Raistrick et al., Biochem. J. 1956, 63, 395), which has been described as being an inhibitor of the respiratory chain, and the phytotoxin flavipucine (Findlay et al., J.C.S. Perkin I 1972, 2071) or the compound F-90558 (Kuraya et al., JP 20012862292 A2), which have been described as being antineoplastic agents. Pyrimidin-2-ylamine-substituted phenylbenzofurans are described, for example, in Burri et al., WO 02/10156.
It has now been found, surprisingly, that the strain Aspergillus flavipes ST003878 (DSM 15290) is able to form novel antibiotics which are effective inhibitors of GImU and are suitable for use as model structures for developing additional agents possessing antibacterial activity.
The invention relates to a compound of the formula (I) R O ~ ~0 ORS ~ ~ s Y ~OR
ORs (1) where R~ and R2 are, independently of each other, H, OH or -O-(C~-C6)-alkyl, and R~, R4, R5, R6 and R~ are, independently of each other, H, -(C~-Cg)-alkyl or-C(O)-(C~-Cg)-alkyl, or a physiologically tolerated salt of a compound of the formula (I).
(C~-Cg)-Alkyl denotes a straight-chain or branched hydrocarbon group having 6 carbon atoms, for example methyl (Me), ethyl, n-propyl, isopropyl, tert-butyl or n-hexyl, preferably methyl.
A, large number of antibiotics are employed therapeutically for treating infectious diseases caused by bacteria. However, the pathogens are becoming increasingly resistant to the drugs employed; there is even the threat of serious danger arising due to what are termed muitiresistant organisms, which have not merely become resistant to single antibiotic groups, such as ~3-lactam antibiotics, glycopeptides or macrolides, but in fact carry several resistances simultaneously. There even exist pathogens which have become resistant to all the antibiotics which are commercially available. It is no longer possible to treat infectious diseases which are caused by these organisms. For this reason, there is a great need for new compositions which can be used against resistant organisms. While many thousand antibiotics have been described in the literature, most of them are too toxic to be used as drugs.
The cell walls of Gram-positive and Gram-negative bacteria consist for the most part of peptidoglycan (murein), which, as what is termed the murein sacculus, encloses the cell completely and lends its mechanical stability as well as helping to determine its morphological form. Peptidoglycan is a macromolecule which is composed of an alternating sequence of the 1,4-~3-glycosidically linked amino sugars N-acetylglucosamine and N-acetylmuramic acid. Crosslinkings by way of short peptide bridges provide the sugar chains with a high degree of stability. The biosynthesis of peptidoglycan is catalyzed by a number of enzymes which are dissolved in cytoplasm or else membrane-bound. Many of these enzymes are specific to bacteria and represent ideal points of attack in the search for new antibiotics.
The bifunctional bacterial N-acetylglucosamine-1-phosphate uridyl-transferase (GImU) catalyzes the formation of UDP-N-acetylglucosamine from glucosamine-1-phosphate in a two-step reaction. UDP-N-acetyl-glucosamine is a fundamental building block in bacterial cell wall biosynthesis and inhibiting its formation is therefore a promising route for finding novel antibacterial therapeutic agents (Sulzenbacher et al., J. Biol.
Chem. 2001, 276 (15), 11844-11851 ).
There have already been reports of compounds from cultures of Aspergillus flavipes, such as flavipin (Raistrick et al., Biochem. J. 1956, 63, 395), which has been described as being an inhibitor of the respiratory chain, and the phytotoxin flavipucine (Findlay et al., J.C.S. Perkin I 1972, 2071) or the compound F-90558 (Kuraya et al., JP 20012862292 A2), which have been described as being antineoplastic agents. Pyrimidin-2-ylamine-substituted phenylbenzofurans are described, for example, in Burri et al., WO 02/10156.
It has now been found, surprisingly, that the strain Aspergillus flavipes ST003878 (DSM 15290) is able to form novel antibiotics which are effective inhibitors of GImU and are suitable for use as model structures for developing additional agents possessing antibacterial activity.
The invention relates to a compound of the formula (I) R O ~ ~0 ORS ~ ~ s Y ~OR
ORs (1) where R~ and R2 are, independently of each other, H, OH or -O-(C~-C6)-alkyl, and R~, R4, R5, R6 and R~ are, independently of each other, H, -(C~-Cg)-alkyl or-C(O)-(C~-Cg)-alkyl, or a physiologically tolerated salt of a compound of the formula (I).
(C~-Cg)-Alkyl denotes a straight-chain or branched hydrocarbon group having 6 carbon atoms, for example methyl (Me), ethyl, n-propyl, isopropyl, tert-butyl or n-hexyl, preferably methyl.
Preference is given to R~ and R2 in the compound of the formula (I) being H.
Preference is furthermore given to R3, R4, R5, R6 and R7 in the compound of the formula (I) being, independently of each other, H or methyl.
Particular preference is given to R~ and R2 in the compound of the formula (I) being H and to R3, R4, R5, R6 and R~ being, independently of each other, H or methyl.
In addition, the invention relates to a compound of the formula (I) which is characterized by a compound of the formula (1l) H, ~O
,~ H O
OH
HO ~ ~O ~ ~
OH ~ OH, OH ~~~)~
a compound of the formula (III) H, , o H O
OH
HO ~ ~O
OH
home OH X111), a compound of the formula (IV) H_ ,o H O
' OH
Ho ~ 'o OMe ~ pH
OMe and a compound of the formula (~
H_ ,o H O
HO I ~ Q I I ~ OH
OMe OMe OMe The present invention furthermore relates to all obvious chemical equivalents of the compounds of the formula (I) according to the invention.
These equivalents are compounds which exhibit a minor chemical difference, and consequently have the same effect, or are converted, under mild conditions, into the compounds according to the invention. Said equivalents also include, for example, salts, reduction products, oxidation products, esters, ethers, acetals or amides of the compounds of the formula (I) as well as equivalents which the skilled person can prepare using standard methods, and, in addition, all optical antipodes and diastereomers, and all stereoisomeric forms.
Physiologically tolerated salts of compounds of the formula (I) are understood as being both their organic salts and their inorganic salts as are described in Remington's Pharmaceutical Sciences (17th Edition, page 1418 (1985)). Because of their physical and chemical stability, and their 5 solubility, sodium salts, potassium salts, calcium salts and ammonium salts are preferred, inter alia, for acid groups; salts of hydrochloric acid, sulfuric acid and phosphoric acid, or of carboxylic acids or sulfonic acids, such as acetic acid, citric acid, benzoic acid, malefic acid, fumaric acid, tartaric acid and p-toluenesulfonic acid, are preferred, inter alia, for basic groups.
The compounds of the formula (I) according to the invention are unrelated to conventional antibiotics such as the ~3-lactams (penicillins and cephalosporins), aminoglycosides (streptomycin), macrolides (erythromycin), quinolones (ciprofloxacin), sulfonamides and glycopeptides (vancomycin).
The invention furthermore relates to a process for preparing a compound of the formula (I), which comprises 1. fermenting the microorganism Aspergillus flavipes ST003878 (DSM
15290), or one of its variants andlor mutants, in a culture medium until one or more compounds of the formula (I) accrues in the culture medium, and 2. isolating a compound of the formula (I) from the culture medium, and 3. where appropriate derivatizing the compound of the formula (I) and/or converting it into a physiologically tolerated salt.
The invention preferably relates to a process for preparing a compound of the formula (I) wherein, in step 1, the compound of the formula ((l) is formed during the fermentation, in step 2, the compound of the formula (II) is isolated and, in step 3, it is derivatized, where appropriate, to give a compound of the formula (I} and/or converted into a physiologically tolerated salt.
The process comprises culturing Aspergillus flavipes ST003878 (DSM
15290) under aerobic conditions in a culture medium which contains a carbon source, a nitrogen source, inorganic salts and, where appropriate, trace elements. In this culture medium, Aspergillus flavipes ST003878 (DSM 15290) forms a mixture of compounds of the formula (I). The quantitative proportion of one or more of the compounds according to the invention can be varied in dependence on the composition of the culture medium. In addition, the composition of the medium can be used to drive the synthesis of individual compounds.
Suitable carbon sources for the fermentation are assimilible carbohydrates and sugar alcohols, such as glucose, lactose, sucrose, glycerol, starch or D-mannitol, and also carbohydrate-containing natural products, such as malt extract and yeast extract. Examples of nitrogen-containing nutrients are amino acids; peptides and proteins and also their breakdown products, for example casein, peptones or tryptones; meat extracts; yeast extracts;
gluten; ground seeds, for example from maize, wheat, oats, beans, soybean or the cotton plant; distillation residues from alcohol production;
meat meals; yeast extracts; ammonium salts; nitrates. Preference is given to the nitrogen source being one or more peptides which have been obtained synthetically or biosynthetically. Examples of inorganic salts are chlorides, carbonates, sulfates or phosphates of the alkali metals or alkaline earth metals, iron, zinc, cobalt and manganese. Examples of trace elements are cobalt and manganese.
The culture medium preferably contains glucose, starch, rolled oats and/or glycerol.
The compounds according to the invention are particularly preferably formed in a nutrient solution which contains from about 0.05 to to 5°!°, preferably from 2 to 3%, of potato starch and from about 0.05 to 3°!°, preferably from 0.05 to 1 %, of yeast extract. The values in percent are in each case based on the weight of the total nutrient solution.
The microorganism is cultured aerobically, i.e., for example, submerged while being shaken or stirred in shaking flasks or fermenters, or on solid medium, where appropriate while introducing air or oxygen. The microorganism can be cultured in a temperature range of from about 15 to 35°C, preferably at from about 20 to 30°C, in particular at 25°C. The pH
range should be between 3 and 10, preferably between 4.5 and 6.5. In general, the microorganism is cultured under these conditions over a period of from 2 to 30 days, preferably of from 72 to 360 hours. The organism is advantageously cultured in several steps, i.e. one or more preliminary cultures are initially prepared in a liquid nutrient medium, with these preliminary cultures then being inoculated into the actual production medium, i.e. the main culture, for example in a volume ratio of 1:10 to 1:100. The preliminary culture is obtained, for example, by inoculating the mycelium into a nutrient solution and allowing it to grow for from about 72 to 360 hours, preferably from 96 to 240 hours. The mycelium can be obtained, for example, by allowing the strain to grow for from about 1 to 20 days, preferably from 6 to 10 days, on a solid or liquid nutrient substrate, for example yeast malt agar, rolled oats agar or potato dextrose agar.
The course of the fermentation, and the formation of the compounds of the formula (I) according to the invention, can be monitored in accordance with the methods which are known to the skilled person, for example by means of detecting biological activity in bioassays or by means of chromatographic methods, such as thin layer chromatography (TLC) or high performance liquid chromatography (HPLC).
The fungus Aspergillus flavipes ST003878 (DSM 15290) is able, for example, to form compounds of the formula (I) by means of a surface culture or stationary culture on solid nutrient substrates. Solid nutrient substrates are prepared by, for example, adding agar or gelatin to aqueous nutrient media. However, it is also possible to obtain the compound of the formula (I) by means of fermenting the fungus Aspergillus flavipes ST003878 (DSM 15290) while submerged, i.e. in an aqueous suspension, with the compound (I) usually being located in the culture cell mass. It is therefore expedient to separate off the fermentation solution by means of filtration or centrifugation. The filtrate is extracted using an absorption resin as the solid phase. The mycelium and the surface culture are expediently extracted with an organic solvent which is miscible, or partially miscible, with water, for example a (C~-C4)-alcohol, preferably methanol or 2-propanol.
While the extractions can be carried out over a wide pH range, it is expedient to carry them out in a neutral or weakly acid medium, preferably between pH 3 and pH 7, where appropriate in the added presence of a reducing agent. The extracts can, for example, be concentrated and dried in vacuo.
Preference is furthermore given to R3, R4, R5, R6 and R7 in the compound of the formula (I) being, independently of each other, H or methyl.
Particular preference is given to R~ and R2 in the compound of the formula (I) being H and to R3, R4, R5, R6 and R~ being, independently of each other, H or methyl.
In addition, the invention relates to a compound of the formula (I) which is characterized by a compound of the formula (1l) H, ~O
,~ H O
OH
HO ~ ~O ~ ~
OH ~ OH, OH ~~~)~
a compound of the formula (III) H, , o H O
OH
HO ~ ~O
OH
home OH X111), a compound of the formula (IV) H_ ,o H O
' OH
Ho ~ 'o OMe ~ pH
OMe and a compound of the formula (~
H_ ,o H O
HO I ~ Q I I ~ OH
OMe OMe OMe The present invention furthermore relates to all obvious chemical equivalents of the compounds of the formula (I) according to the invention.
These equivalents are compounds which exhibit a minor chemical difference, and consequently have the same effect, or are converted, under mild conditions, into the compounds according to the invention. Said equivalents also include, for example, salts, reduction products, oxidation products, esters, ethers, acetals or amides of the compounds of the formula (I) as well as equivalents which the skilled person can prepare using standard methods, and, in addition, all optical antipodes and diastereomers, and all stereoisomeric forms.
Physiologically tolerated salts of compounds of the formula (I) are understood as being both their organic salts and their inorganic salts as are described in Remington's Pharmaceutical Sciences (17th Edition, page 1418 (1985)). Because of their physical and chemical stability, and their 5 solubility, sodium salts, potassium salts, calcium salts and ammonium salts are preferred, inter alia, for acid groups; salts of hydrochloric acid, sulfuric acid and phosphoric acid, or of carboxylic acids or sulfonic acids, such as acetic acid, citric acid, benzoic acid, malefic acid, fumaric acid, tartaric acid and p-toluenesulfonic acid, are preferred, inter alia, for basic groups.
The compounds of the formula (I) according to the invention are unrelated to conventional antibiotics such as the ~3-lactams (penicillins and cephalosporins), aminoglycosides (streptomycin), macrolides (erythromycin), quinolones (ciprofloxacin), sulfonamides and glycopeptides (vancomycin).
The invention furthermore relates to a process for preparing a compound of the formula (I), which comprises 1. fermenting the microorganism Aspergillus flavipes ST003878 (DSM
15290), or one of its variants andlor mutants, in a culture medium until one or more compounds of the formula (I) accrues in the culture medium, and 2. isolating a compound of the formula (I) from the culture medium, and 3. where appropriate derivatizing the compound of the formula (I) and/or converting it into a physiologically tolerated salt.
The invention preferably relates to a process for preparing a compound of the formula (I) wherein, in step 1, the compound of the formula ((l) is formed during the fermentation, in step 2, the compound of the formula (II) is isolated and, in step 3, it is derivatized, where appropriate, to give a compound of the formula (I} and/or converted into a physiologically tolerated salt.
The process comprises culturing Aspergillus flavipes ST003878 (DSM
15290) under aerobic conditions in a culture medium which contains a carbon source, a nitrogen source, inorganic salts and, where appropriate, trace elements. In this culture medium, Aspergillus flavipes ST003878 (DSM 15290) forms a mixture of compounds of the formula (I). The quantitative proportion of one or more of the compounds according to the invention can be varied in dependence on the composition of the culture medium. In addition, the composition of the medium can be used to drive the synthesis of individual compounds.
Suitable carbon sources for the fermentation are assimilible carbohydrates and sugar alcohols, such as glucose, lactose, sucrose, glycerol, starch or D-mannitol, and also carbohydrate-containing natural products, such as malt extract and yeast extract. Examples of nitrogen-containing nutrients are amino acids; peptides and proteins and also their breakdown products, for example casein, peptones or tryptones; meat extracts; yeast extracts;
gluten; ground seeds, for example from maize, wheat, oats, beans, soybean or the cotton plant; distillation residues from alcohol production;
meat meals; yeast extracts; ammonium salts; nitrates. Preference is given to the nitrogen source being one or more peptides which have been obtained synthetically or biosynthetically. Examples of inorganic salts are chlorides, carbonates, sulfates or phosphates of the alkali metals or alkaline earth metals, iron, zinc, cobalt and manganese. Examples of trace elements are cobalt and manganese.
The culture medium preferably contains glucose, starch, rolled oats and/or glycerol.
The compounds according to the invention are particularly preferably formed in a nutrient solution which contains from about 0.05 to to 5°!°, preferably from 2 to 3%, of potato starch and from about 0.05 to 3°!°, preferably from 0.05 to 1 %, of yeast extract. The values in percent are in each case based on the weight of the total nutrient solution.
The microorganism is cultured aerobically, i.e., for example, submerged while being shaken or stirred in shaking flasks or fermenters, or on solid medium, where appropriate while introducing air or oxygen. The microorganism can be cultured in a temperature range of from about 15 to 35°C, preferably at from about 20 to 30°C, in particular at 25°C. The pH
range should be between 3 and 10, preferably between 4.5 and 6.5. In general, the microorganism is cultured under these conditions over a period of from 2 to 30 days, preferably of from 72 to 360 hours. The organism is advantageously cultured in several steps, i.e. one or more preliminary cultures are initially prepared in a liquid nutrient medium, with these preliminary cultures then being inoculated into the actual production medium, i.e. the main culture, for example in a volume ratio of 1:10 to 1:100. The preliminary culture is obtained, for example, by inoculating the mycelium into a nutrient solution and allowing it to grow for from about 72 to 360 hours, preferably from 96 to 240 hours. The mycelium can be obtained, for example, by allowing the strain to grow for from about 1 to 20 days, preferably from 6 to 10 days, on a solid or liquid nutrient substrate, for example yeast malt agar, rolled oats agar or potato dextrose agar.
The course of the fermentation, and the formation of the compounds of the formula (I) according to the invention, can be monitored in accordance with the methods which are known to the skilled person, for example by means of detecting biological activity in bioassays or by means of chromatographic methods, such as thin layer chromatography (TLC) or high performance liquid chromatography (HPLC).
The fungus Aspergillus flavipes ST003878 (DSM 15290) is able, for example, to form compounds of the formula (I) by means of a surface culture or stationary culture on solid nutrient substrates. Solid nutrient substrates are prepared by, for example, adding agar or gelatin to aqueous nutrient media. However, it is also possible to obtain the compound of the formula (I) by means of fermenting the fungus Aspergillus flavipes ST003878 (DSM 15290) while submerged, i.e. in an aqueous suspension, with the compound (I) usually being located in the culture cell mass. It is therefore expedient to separate off the fermentation solution by means of filtration or centrifugation. The filtrate is extracted using an absorption resin as the solid phase. The mycelium and the surface culture are expediently extracted with an organic solvent which is miscible, or partially miscible, with water, for example a (C~-C4)-alcohol, preferably methanol or 2-propanol.
While the extractions can be carried out over a wide pH range, it is expedient to carry them out in a neutral or weakly acid medium, preferably between pH 3 and pH 7, where appropriate in the added presence of a reducing agent. The extracts can, for example, be concentrated and dried in vacuo.
One method of purifying the compounds according to the invention is that of solution distribution between a stationary and a mobile phase, in a manner known per se, for example by means of chromatography on adsorption resins, for example on Diaion~ HP-20 (Mitsubishi Casei Corp., Tokyo), on Amberlite~ XAD 7 (Rohm and Haas, USA) or Amberchrom~
CG, (Toso Haas, Philadelphia, USA). Numerous reverse, phase supports, for example RPg and RP~g, as are well known within the context of high pressure liquid chromatography (HPLC), are also suitable.
Another possibility for purifying the antibiotic according to the invention is that of using what are termed normal-phase chromatography supports, for example silica gel or AI203, or others, in a manner known per se.
An alternative isolation method is that of using molecular sieves, such as Fractogel~ TSK HW-40 (Merck, Germany) or Sephadex~ G-25 (Amersham Biosciences), in a manner known per se. In addition to this, it is also possible to use crystallization to isolate biflavipin from enriched material.
Organic solvents and their mixtures, either anhydrous or with water added, are, for example, suitable for this purpose. An additional method for isolating and purifying the antibiotics according to the invention consists in using anion exchangers, preferably in a pH range from 4 to 10, and cation exchangers, preferably in a pH range of from 2 to 5. The use of buffer solutions to which portions of organic solvents have been added is particularly suitable for this purpose.
An isolate of the microorganism strain Aspergillus tlavipes ST003878 was deposited, in accordance with the rules of the Budapest Treaty, in the Deutsche Sammlung von Mikroorganismen and Zellkulturen [German collection of microorganisms and cell cultures] GmbH (DSMZ), Mascheroder Weg 1 B, 38124 Brunswick, Germany, under the number DSM 15290.
The fungus Aspergiilus flavipes ST003878 (DSM 15290) has a white substrate mycelium. During sporulation, the color of the mycelium changes to yellow to brown. Cultures on Czapek agar medium which ace about 10 days of age form large amounts of yellow to brownish exudates. The conidia are colorless and round, having a diameter of 2-3 Nm The primary and secondary sterigmata are of similar length (5-6 Nm) and are brown in color.
Instead of the strain Rspergillus flavipes ST003878 (DSM 15290), it is also possible to use one of its mutants and/or variants which is able to produce one of the compounds of the formula (I) according to the invention.
A mutant is a microorganism in which one or more genes in the genome have been modified, with the gene or the genes which is/are responsible, in the case of the present invention, for the ability of the organism to produce one or more of the compounds of the formula (I) remaining functional and inheritable.
These mutants can be generated, in a manner known per se, using physical means, for example irradiation, as with ultraviolet rays or x-rays, or using chemical mutagens, such as ethyl methanesulfonate (EMS);
2-hydroxy-4-methoxybenzophenone (MOB) or N-methyl-N'-nitro-N-nitrosoguanidine (MNNG), or as described by Brock et al. in "Biology of Microorganisms, Prentice Hall, pages 238-247 (1984).
A variant is a phenotype of the microorganism. Microorganisms have the ability to adapt to their environment and therefore exhibit pronounced physiological flexibility. In the case of phenotypic adaptation, alf the cells of the microorganism are involved, with the nature of the change not being genetically conditioned and being reversible under altered circumstances (H. Stolp, Microbial ecology: organism, habitats, activities. Cambridge University Press, Cambridge, GB, page 180, 1988).
Screening for mutants and/or variants which synthesize one or more of the compounds according to the invention is effected in accordance with the following scheme:
- lyophilization of the fermentation medium;
- extraction of the lyophilizate with an organic solvent - extraction of a compound from the culture filtrate using solid phases - analysis by means of HPLC or TLC or by means of testing the biological activity.
The above-described fermentation conditions apply both for Aspergillus flavipes ST003878 (DSM 15290) and for mutants andlor variants thereof.
Derivatizations are carried out as follows: hydroxyl groups of the compound 5 of the formula (I) (R3 to R7 are, independently of each other, H) can be esterified using an activated acid, preferably an acid chloride CI-C(O)-(C~-Cg)-alkyl (R3 to R7 are, independently of each other, -C(O)-(C~-Cg)-alkyl).
In addition, hydroxyl groups can be etherified by, for example, reaction with a (C~-Cg)-alkyl halide in acid medium or by reaction with a trimethylsilyl-10 diazo-(C~-Cg)-alkyl compound, preferably with trimethylsilyldiazomethane.
A phenylic aldehyde function (R~ and/or R2 is H) is, for example, oxidized to an acid function using manganese oxide or using Jones reagent (sulfuric chromium(VI) oxide). The acid function which is formed in this connection can be esterified by means of 4-dimethylaminopyridine (4-DMAP) under Steglich conditions or with a (C~-Cg)-alcohol in acid medium. Said derivatizations are examples of methods which are known per se and are described, inter alia, in J. March, Advanced Organic Chemistry, John Wiley & Sons, 4th Edition, 1992. In order to carry out the reactions selectively, it may be advantageous to introduce protecting groups, in a manner known per se, prior to the reaction. The protecting groups are eliminated after the reaction and the reaction product is then purified.
The compounds according to the invention are powerful inhibitors of bacterial N-acetylglucosamine-1-phosphate uridyltransferase (GImU); they are therefore suitable for the treatment and/or prophylaxis of diseases which are caused by bacterial infections or mycoses.
The inhibition of the GImU can be determined in a biochemical test using the following method:
The assay was carried out in a 384-plate format. The reaction volume was p1 per test. The reaction mixture contained 10 NI of test substance and 15 NI of substrate solution consisting of acetyICoA and D-glucosamine-1-phosphate. The enzyme reaction was started by adding 15 NI of GImU
35 enzyme solution. After 60 minutes of incubation at 30°C, the reaction was stopped by adding 10 NI of developer reagent (DTNB dissolved in guanidine). The plates were then centrifuged (1 min, 1000 rpm) and stored for a further 45 minutes at room temperature before the absorption was read at 405 nm in a photometer. In order to be able to calculate the inhibitory activity of the test compounds, positive controls (signal with GImU) and negative controls (signal without GImU) were included on each plate. In order to exclude falsely positive samples, which could be caused by nonspecific substance effects (e.g. color), blank plates, which contained the substances but no GImU, were included in parallel with the test plates.
After correction for the blanks, the inhibitory activities of the substances were calculated in accordance with the following formula:
Inhibition (%) = 100 x [1-(OD405 nm substance/OD405 nm positive control)]
An inhibition constant, ICSp, of 1 NM was determined for the inhibitory effect of the compound of formula (II) on the enzyme N-acetylglucosamine-1-phosphate uridyltransferase (GImU).
The invention therefore furthermore relates to the use of a compound of the formula (I), preferably of a compound of the formula (1l), or of a physiologically tolerated salt thereof, for producing a pharmaceutical in human or animal medicine, in particular for producing a pharmaceutical for the treatment and/or prophylaxis of bacterial infectious diseases and/or mycoses.
In addition, the present invention relates to a pharmaceutical having a content of at least one compound of the formula (I) according to the invention, preferably having a content of the compound of the formula (II).
Said pharmaceutical is produced by mixing at least one compound of the formula (I) with one or more pharmacologically suitable auxiliary substances or carrier substances and bringing the mixture into a form suitable for administration.
While the pharmaceuticals according to the invention can be administered orally or parenteraliy, it is also in principle possible to use them rectally.
Examples of suitable solid or liquid galenic preparation forms are granules, powders, tablets, sugar-coated tablets, (micro)capsules, suppositories, syrups, emulsions, suspensions, aerosols, drops or injectable solutions in ampoule form, and also preparations giving a protracted release of active compound, in the production of which use is customarily made of pharmacologically suitable carrier substances or auxiliary substances, such as disintegrants, binders, coating agents, swelling agents, gliders, lubricants, flavorings, sweeteners or solubilizers, for example magnesium carbonate, titanium dioxide, lactose, mannitol and other sugars, talc, lactalbumin, gelatin, starch, vitamins, cellulose and its derivatives, animal or vegetable oils, polyethylene glycols and solvents, such as water, alcohols, glycerol and polyhydric alcohols.
Where appropriate, the dosage units for oral administration can be microencapsulated in order to delay the release, or extend it over a longer period, as, for example, by means of coating or embedding the active compound, in particle form, in suitable polymers, waxes or the like.
0.1-1000, preferably 0.2-100 mg/kg of body weight islare administered as an expedient dose. These quantities are expediently administered in dosage units which at least contain the effective daily quantity of the compounds according to the invention, e.g. 30-3000, preferably 50-1000 mg.
The daily dose to be administered depends on the body weight, age, sex and condition of the mammal. However, higher and lower daily doses may sometimes also be appropriate. The daily dose can be administered both by means of a once-only administration in the form of a single dosage unit, or in several smaller dosage units, and by means of the multiple administration of subdivided doses at predetermined intervals.
The following examples are intended to clarify the invention without limiting the scope of the invention in any way.
Percentage values relate to the weight. Mixing ratios in the case of liquids relate to volume unless otherwise indicated.
Example 1: Preparing a glycerol culture of Aspergillus flavipes ST003878 (DSM 15290) 30 ml of nutrient solution (malt extract, 2.0°I°, yeast extract, 0.2%, glucose, 1.0%, (NH4)2HP04, 0.05%, pH 6.0) were inoculated, in a sterile 100 ml Erlenmeyer flask, with the strain Aspergillus flavipes ST003878 (DSM
CG, (Toso Haas, Philadelphia, USA). Numerous reverse, phase supports, for example RPg and RP~g, as are well known within the context of high pressure liquid chromatography (HPLC), are also suitable.
Another possibility for purifying the antibiotic according to the invention is that of using what are termed normal-phase chromatography supports, for example silica gel or AI203, or others, in a manner known per se.
An alternative isolation method is that of using molecular sieves, such as Fractogel~ TSK HW-40 (Merck, Germany) or Sephadex~ G-25 (Amersham Biosciences), in a manner known per se. In addition to this, it is also possible to use crystallization to isolate biflavipin from enriched material.
Organic solvents and their mixtures, either anhydrous or with water added, are, for example, suitable for this purpose. An additional method for isolating and purifying the antibiotics according to the invention consists in using anion exchangers, preferably in a pH range from 4 to 10, and cation exchangers, preferably in a pH range of from 2 to 5. The use of buffer solutions to which portions of organic solvents have been added is particularly suitable for this purpose.
An isolate of the microorganism strain Aspergillus tlavipes ST003878 was deposited, in accordance with the rules of the Budapest Treaty, in the Deutsche Sammlung von Mikroorganismen and Zellkulturen [German collection of microorganisms and cell cultures] GmbH (DSMZ), Mascheroder Weg 1 B, 38124 Brunswick, Germany, under the number DSM 15290.
The fungus Aspergiilus flavipes ST003878 (DSM 15290) has a white substrate mycelium. During sporulation, the color of the mycelium changes to yellow to brown. Cultures on Czapek agar medium which ace about 10 days of age form large amounts of yellow to brownish exudates. The conidia are colorless and round, having a diameter of 2-3 Nm The primary and secondary sterigmata are of similar length (5-6 Nm) and are brown in color.
Instead of the strain Rspergillus flavipes ST003878 (DSM 15290), it is also possible to use one of its mutants and/or variants which is able to produce one of the compounds of the formula (I) according to the invention.
A mutant is a microorganism in which one or more genes in the genome have been modified, with the gene or the genes which is/are responsible, in the case of the present invention, for the ability of the organism to produce one or more of the compounds of the formula (I) remaining functional and inheritable.
These mutants can be generated, in a manner known per se, using physical means, for example irradiation, as with ultraviolet rays or x-rays, or using chemical mutagens, such as ethyl methanesulfonate (EMS);
2-hydroxy-4-methoxybenzophenone (MOB) or N-methyl-N'-nitro-N-nitrosoguanidine (MNNG), or as described by Brock et al. in "Biology of Microorganisms, Prentice Hall, pages 238-247 (1984).
A variant is a phenotype of the microorganism. Microorganisms have the ability to adapt to their environment and therefore exhibit pronounced physiological flexibility. In the case of phenotypic adaptation, alf the cells of the microorganism are involved, with the nature of the change not being genetically conditioned and being reversible under altered circumstances (H. Stolp, Microbial ecology: organism, habitats, activities. Cambridge University Press, Cambridge, GB, page 180, 1988).
Screening for mutants and/or variants which synthesize one or more of the compounds according to the invention is effected in accordance with the following scheme:
- lyophilization of the fermentation medium;
- extraction of the lyophilizate with an organic solvent - extraction of a compound from the culture filtrate using solid phases - analysis by means of HPLC or TLC or by means of testing the biological activity.
The above-described fermentation conditions apply both for Aspergillus flavipes ST003878 (DSM 15290) and for mutants andlor variants thereof.
Derivatizations are carried out as follows: hydroxyl groups of the compound 5 of the formula (I) (R3 to R7 are, independently of each other, H) can be esterified using an activated acid, preferably an acid chloride CI-C(O)-(C~-Cg)-alkyl (R3 to R7 are, independently of each other, -C(O)-(C~-Cg)-alkyl).
In addition, hydroxyl groups can be etherified by, for example, reaction with a (C~-Cg)-alkyl halide in acid medium or by reaction with a trimethylsilyl-10 diazo-(C~-Cg)-alkyl compound, preferably with trimethylsilyldiazomethane.
A phenylic aldehyde function (R~ and/or R2 is H) is, for example, oxidized to an acid function using manganese oxide or using Jones reagent (sulfuric chromium(VI) oxide). The acid function which is formed in this connection can be esterified by means of 4-dimethylaminopyridine (4-DMAP) under Steglich conditions or with a (C~-Cg)-alcohol in acid medium. Said derivatizations are examples of methods which are known per se and are described, inter alia, in J. March, Advanced Organic Chemistry, John Wiley & Sons, 4th Edition, 1992. In order to carry out the reactions selectively, it may be advantageous to introduce protecting groups, in a manner known per se, prior to the reaction. The protecting groups are eliminated after the reaction and the reaction product is then purified.
The compounds according to the invention are powerful inhibitors of bacterial N-acetylglucosamine-1-phosphate uridyltransferase (GImU); they are therefore suitable for the treatment and/or prophylaxis of diseases which are caused by bacterial infections or mycoses.
The inhibition of the GImU can be determined in a biochemical test using the following method:
The assay was carried out in a 384-plate format. The reaction volume was p1 per test. The reaction mixture contained 10 NI of test substance and 15 NI of substrate solution consisting of acetyICoA and D-glucosamine-1-phosphate. The enzyme reaction was started by adding 15 NI of GImU
35 enzyme solution. After 60 minutes of incubation at 30°C, the reaction was stopped by adding 10 NI of developer reagent (DTNB dissolved in guanidine). The plates were then centrifuged (1 min, 1000 rpm) and stored for a further 45 minutes at room temperature before the absorption was read at 405 nm in a photometer. In order to be able to calculate the inhibitory activity of the test compounds, positive controls (signal with GImU) and negative controls (signal without GImU) were included on each plate. In order to exclude falsely positive samples, which could be caused by nonspecific substance effects (e.g. color), blank plates, which contained the substances but no GImU, were included in parallel with the test plates.
After correction for the blanks, the inhibitory activities of the substances were calculated in accordance with the following formula:
Inhibition (%) = 100 x [1-(OD405 nm substance/OD405 nm positive control)]
An inhibition constant, ICSp, of 1 NM was determined for the inhibitory effect of the compound of formula (II) on the enzyme N-acetylglucosamine-1-phosphate uridyltransferase (GImU).
The invention therefore furthermore relates to the use of a compound of the formula (I), preferably of a compound of the formula (1l), or of a physiologically tolerated salt thereof, for producing a pharmaceutical in human or animal medicine, in particular for producing a pharmaceutical for the treatment and/or prophylaxis of bacterial infectious diseases and/or mycoses.
In addition, the present invention relates to a pharmaceutical having a content of at least one compound of the formula (I) according to the invention, preferably having a content of the compound of the formula (II).
Said pharmaceutical is produced by mixing at least one compound of the formula (I) with one or more pharmacologically suitable auxiliary substances or carrier substances and bringing the mixture into a form suitable for administration.
While the pharmaceuticals according to the invention can be administered orally or parenteraliy, it is also in principle possible to use them rectally.
Examples of suitable solid or liquid galenic preparation forms are granules, powders, tablets, sugar-coated tablets, (micro)capsules, suppositories, syrups, emulsions, suspensions, aerosols, drops or injectable solutions in ampoule form, and also preparations giving a protracted release of active compound, in the production of which use is customarily made of pharmacologically suitable carrier substances or auxiliary substances, such as disintegrants, binders, coating agents, swelling agents, gliders, lubricants, flavorings, sweeteners or solubilizers, for example magnesium carbonate, titanium dioxide, lactose, mannitol and other sugars, talc, lactalbumin, gelatin, starch, vitamins, cellulose and its derivatives, animal or vegetable oils, polyethylene glycols and solvents, such as water, alcohols, glycerol and polyhydric alcohols.
Where appropriate, the dosage units for oral administration can be microencapsulated in order to delay the release, or extend it over a longer period, as, for example, by means of coating or embedding the active compound, in particle form, in suitable polymers, waxes or the like.
0.1-1000, preferably 0.2-100 mg/kg of body weight islare administered as an expedient dose. These quantities are expediently administered in dosage units which at least contain the effective daily quantity of the compounds according to the invention, e.g. 30-3000, preferably 50-1000 mg.
The daily dose to be administered depends on the body weight, age, sex and condition of the mammal. However, higher and lower daily doses may sometimes also be appropriate. The daily dose can be administered both by means of a once-only administration in the form of a single dosage unit, or in several smaller dosage units, and by means of the multiple administration of subdivided doses at predetermined intervals.
The following examples are intended to clarify the invention without limiting the scope of the invention in any way.
Percentage values relate to the weight. Mixing ratios in the case of liquids relate to volume unless otherwise indicated.
Example 1: Preparing a glycerol culture of Aspergillus flavipes ST003878 (DSM 15290) 30 ml of nutrient solution (malt extract, 2.0°I°, yeast extract, 0.2%, glucose, 1.0%, (NH4)2HP04, 0.05%, pH 6.0) were inoculated, in a sterile 100 ml Erlenmeyer flask, with the strain Aspergillus flavipes ST003878 (DSM
15290) and incubated for 6 days, at 25°C and 140 rpm, on a rotating shaker. 1.5 ml of this culture were subsequently diluted with 2.5 ml of 80%
glycerol and stored at -135°C.
Example 2: Preparing a preliminary culture of Aspergillus flavipes ST003878 (DSM 15290) in an Erlenmeyer flask.
100 ml of nutrient solution (malt extract, 2.0%, yeast extract, 0.2°l0, glucose, 1.0%, (NH4)2HP04, 0.05%, pH 6.0) are inoculated, in a sterile 300 ml Erlenmeyer flask, with the strain Aspergillus flavipes ST003878 (DSM
15290) and incubated for 4 days, at 25°C and 140 rpm, on a rotating shaker. 2 ml of this preliminary culture are then inoculated for the purpose of preparing the main cultures.
Example 3: Fermenting Aspergillus flavipes ST003878 (DSM 15290) in an Erlenmeyer flask In each case 100 ml of nutrient solution (potato dextrose broth, 2.4%, yeast extract, 0.2%, pH 5.2) are inoculated, in a sterile 300 ml Erlenmeyer flask, with the strain Aspergillus flavipes ST003878 (DSM 15290) and incubated for 11 days, at 25°C and 140 rpm, on a rotating shaker. 300 ml of this preliminary culture are then inoculated for the purpose of preparing the main cultures.
Example 4: Fermenting Aspergillus flavipes ST003878 (DSM 15290) in a fermenter A 10 I fermenter is operated under the following conditions:
Nutrient medium: 24 g of potato dextrose broth/I
2 g of yeast extractJl pH 5.2 (prior to sterilization) Incubation period: 166 hours Incubation temperature: 28°C
Stirrer speed: 180 rpm Aeration: 16 L min ~
glycerol and stored at -135°C.
Example 2: Preparing a preliminary culture of Aspergillus flavipes ST003878 (DSM 15290) in an Erlenmeyer flask.
100 ml of nutrient solution (malt extract, 2.0%, yeast extract, 0.2°l0, glucose, 1.0%, (NH4)2HP04, 0.05%, pH 6.0) are inoculated, in a sterile 300 ml Erlenmeyer flask, with the strain Aspergillus flavipes ST003878 (DSM
15290) and incubated for 4 days, at 25°C and 140 rpm, on a rotating shaker. 2 ml of this preliminary culture are then inoculated for the purpose of preparing the main cultures.
Example 3: Fermenting Aspergillus flavipes ST003878 (DSM 15290) in an Erlenmeyer flask In each case 100 ml of nutrient solution (potato dextrose broth, 2.4%, yeast extract, 0.2%, pH 5.2) are inoculated, in a sterile 300 ml Erlenmeyer flask, with the strain Aspergillus flavipes ST003878 (DSM 15290) and incubated for 11 days, at 25°C and 140 rpm, on a rotating shaker. 300 ml of this preliminary culture are then inoculated for the purpose of preparing the main cultures.
Example 4: Fermenting Aspergillus flavipes ST003878 (DSM 15290) in a fermenter A 10 I fermenter is operated under the following conditions:
Nutrient medium: 24 g of potato dextrose broth/I
2 g of yeast extractJl pH 5.2 (prior to sterilization) Incubation period: 166 hours Incubation temperature: 28°C
Stirrer speed: 180 rpm Aeration: 16 L min ~
Foam formation was suppressed by repeatedly adding an ethanolic solution of polyol. The production maximum was reached after approx. 160 hours.
Example 5: Isolating the compound of the formula (II) 25 liters of culture solution, obtained as described in example 4, contained 90 mg of the compound of the formula (II). The culture broth was filtered and the mycelium (1.65 kg) was extracted with 10 liters of 2-propanol. The clear alcoholic phase was concentrated down in vacuo to 2 I and, after 1 g of ascorbic acid had been added as antioxidant, loaded onto a column of 785 ml in volume which was filled with the adsorption resin MCI Gel CHP20P. Column dimensions: width x height: 10 cm x 25 cm. The column was eluted with a solvent gradient of from 5% acetonitrile in water to 100%
acetonitrile and a column throughput of 15 liters per hour. Fractions which each contained 2.5 liters were collected. Fractions 7 to 9, which contained the compound of the formula (II), were checked by HPLC analyses, pooled and concentrated in vacuo. The pH of the solution, which had to a large extent been freed from the isopropanol, was also adjusted to 4.2 and once again loaded onto an MCI Gel~ CHP20P column (490 ml, column dimensions: 5 cm x 25 cm). The elution was effected using a gradient of from 0.01 % ammonium formate (pH 4.2) to 100°l° acetonitrile.
With the column throughput being 40 ml per minute, fractions containing 200 ml were taken. Fractions 12 and 13 contained the enriched compound of the formula (II). They were combined, concentrated in vacuo and, for the purpose of further chromatographic purification, separated on a Luna 10N
C18 phenomenex~ column (column dimensions: 21 mm x 250 mm).
0.025% trifluoroacetic acid and from 0% to 100% acetonitrile were used as the eluent, with the flow-through rate being 25 ml/minute. The fraction size was 50 ml. Fraction 14 contained the greatly enriched compound of the formula (II); it was slightly concentrated in vacuo and left to stand at +4°C.
The lemon-yellow compound of the formula (II) crystallized out and was filtered off, dried and bottled under argon (20 mg).
Example 6: High pressure liquid chromatography (HPLC) of the compound of the formula (II) Column: YMC-PRO 18~, 120°A, 250-4.4, with precolumn, Mobile phase: A: 5% acetonitrife in 0.02°l° trifluoroacetic acid, 2 minutes, B: 100% acetonitrile, Gradient: from A to B in 18 minutes.
5 Flow rate: 1 ml per minute, Detection by UV absorption at 210 nm.
The compound of the formula (II) was found to have a retention time of 13.9 minutes.
Example 7: Characterizing the compound of the formula (II) A molar mass (M - H} of 357.0673 was found by means of electron spray ionization mass spectrometry (ESI-MS} in the negative mode while a molecular weight (M + H} of 359.0811 was found in the positive mode, corresponding to the empirical formula C~gH~40g and a molecular weight of 358.31.
The physicochemical and spectroscopic properties of the compound (II) can be summarized as follows:
Appearance: lemon-yellow crystalline substance which is soluble in medium-polar and polar organic solvents. Stable in neutral and mildly acid medium but unstable in strongly acidic and alkaline solutions and under the influence of oxygen.
Empirical formula: C~gH~40g Molecular weight: 358.31 UV maxima: 220, 245, 307 and 365 nm in water/acetonitrile (1:1) at pH 2.
Table 1: Chemical shifts of the compound (II) in DMSO at 300 K.
H C
2 - 151.57 3 7.47 108.94 3a - 122.83 4 - 117.21 5 - 127.54 5-Me 2.58 11.03 6 - 140.91 6-OH broad -7 - 136.42 7-OH broad -7a - 142.35 8 10.42 190.2 broad) 9 - 124.84 10 - 112.61 11 - 150.17 11-OH 12.1 (broad)-12 - 132.68 12-OH broad -13 - 151.52 13-OH broad -14 - 118.72 14-Me 2.01 12.66 15 9.48 194.74 Example 8: Methylating the compound of the formula (II) 12 mg of the compound of the formula (II), obtained as described in example 5, were dissolved in 3 ml of methanol after which 1 ml of (trimethylsilyl)diazomethane [2 M solution in hexane, Aldrich] was added.
The reaction mixture was left to stand at room temperature and the course of the reaction was monitored by HPLC. After the compound of the formula (II) employed had been completely reacted, the reaction was terminated by adding water and concentrating in vacuo. The resulting methylation products were purified chromatographically on a Luna 5N RP18 phenomenex~ column using a gradient containing 0.02% trifluoroacetic acid and acetonitrile. After the pure fractions had been freeze-dried, the following were obtained by means of HPLC (conditions as in example 5):
2 mg of compound of the formula (III), monomethyl ether, retention time, 15.4 minutes, 2.7 mg of compound of the formula (I~, dimethyl ether, retention time, 16.9 minutes, 1.9 mg of compound of the formula (~, trimethyl ether, retention time, 19.4 minutes.
Example 9: Characterizing the compound of the formula (Ill) In ESI-MS, the compound of the formula (III) gave a molecular peak of 373.0 in the positive mode (M + H) and of 371.0 in the negative mode (M -H), corresponding to a MW = 372 and an empirical formula of C~gH~gOg.
8 i 5/ 4 3a 3 15 1 I ~ 10 OH
HO 6 ~7a O 14 ~ \ 11 OH
112' OH
Table 2: Chemical shifts of the compound (III) in DMSO at 300 K.
H C
2 - 150.95 3 7.51 109.16 3a - 122.65 4 - 117.28 - 127.75 5-Me 2.58 11.06 6 - 141.03 6-OH broad -7 - 136.47 7-OH broad -7a - 142.45 8 10.42 190.24 9 - 129.11 - 112.98 11 - 154.87 11-OH 12.22 -12 - 134.76 12-OMe 3.83 60.28 13 - 155.68 13-OH broad -14 - 119.05 14-Me 2.01 12.66 9.49 194.73 Example 10: Characterizing the compound of the formula (I~
In ESI-MS, the compound of the formula (I~ gave a molecular peak of 387.1 in the positive mode (M + H) and of 385.0 in the negative mode, corresponding to a MW = 386 and an empirical formula of C2pH~gOg.
Table 3: Chemical shifts of the compound (I~ in DMSO at 300 K.
H C
2 - 151.51 3 7.51 108.72 3a - 122.93 4 - 119.83 5 - 127.10 5-Me 2.58 10.86 6 - 143.62 6-OH 9.21 -7 - 137.18 7-OMe 4.15 60.44 7a - 143.74 8 10.48 190.88 9 - 122.97 10 - 115.84 11 - 150.54 11-OH 11.70 -12 - 139.24 12-OH 9.68 -13 - 151.69 13-OMe 3.87 59.90 14 - 123.98 14-Me 2.08 12.80 15 ~ 9.72 ~ 195.45 Example 11: Characterizing the compound of the formula (~
5 In ESI-MS, the compound of the formula (~ gave a molecular peak of 401.1 in the positive mode (M + H) and of 399.0 in the negative mode (M -H), corresponding to MW = 400 and an empirical formula of C2~H2pOg.
Table 4: Chemical shifts of the compound (~ in DMSO at 300 K.
H "C
2 - 150.90 3 7.56 108.95 3a - 122.73 4 - 119.91 - 127.28 5-Me 2.58 10.85 6 - 143.74 6-OH 9.25 -7 - 137.18 7-OMe 4.14 60.45 7a - 143.82 8 10.48 190.88 9 - 127.83 - 116.20 11 - 155.63 11-OH 11.82 -12 - 140.70 12-OMe 3.88 60.53 13 - 156.89 13-OMe 3.98 60.74 14 - 123.77 14-Me 2.06 12.85 ~ 9.73 ~ 195.00
Example 5: Isolating the compound of the formula (II) 25 liters of culture solution, obtained as described in example 4, contained 90 mg of the compound of the formula (II). The culture broth was filtered and the mycelium (1.65 kg) was extracted with 10 liters of 2-propanol. The clear alcoholic phase was concentrated down in vacuo to 2 I and, after 1 g of ascorbic acid had been added as antioxidant, loaded onto a column of 785 ml in volume which was filled with the adsorption resin MCI Gel CHP20P. Column dimensions: width x height: 10 cm x 25 cm. The column was eluted with a solvent gradient of from 5% acetonitrile in water to 100%
acetonitrile and a column throughput of 15 liters per hour. Fractions which each contained 2.5 liters were collected. Fractions 7 to 9, which contained the compound of the formula (II), were checked by HPLC analyses, pooled and concentrated in vacuo. The pH of the solution, which had to a large extent been freed from the isopropanol, was also adjusted to 4.2 and once again loaded onto an MCI Gel~ CHP20P column (490 ml, column dimensions: 5 cm x 25 cm). The elution was effected using a gradient of from 0.01 % ammonium formate (pH 4.2) to 100°l° acetonitrile.
With the column throughput being 40 ml per minute, fractions containing 200 ml were taken. Fractions 12 and 13 contained the enriched compound of the formula (II). They were combined, concentrated in vacuo and, for the purpose of further chromatographic purification, separated on a Luna 10N
C18 phenomenex~ column (column dimensions: 21 mm x 250 mm).
0.025% trifluoroacetic acid and from 0% to 100% acetonitrile were used as the eluent, with the flow-through rate being 25 ml/minute. The fraction size was 50 ml. Fraction 14 contained the greatly enriched compound of the formula (II); it was slightly concentrated in vacuo and left to stand at +4°C.
The lemon-yellow compound of the formula (II) crystallized out and was filtered off, dried and bottled under argon (20 mg).
Example 6: High pressure liquid chromatography (HPLC) of the compound of the formula (II) Column: YMC-PRO 18~, 120°A, 250-4.4, with precolumn, Mobile phase: A: 5% acetonitrife in 0.02°l° trifluoroacetic acid, 2 minutes, B: 100% acetonitrile, Gradient: from A to B in 18 minutes.
5 Flow rate: 1 ml per minute, Detection by UV absorption at 210 nm.
The compound of the formula (II) was found to have a retention time of 13.9 minutes.
Example 7: Characterizing the compound of the formula (II) A molar mass (M - H} of 357.0673 was found by means of electron spray ionization mass spectrometry (ESI-MS} in the negative mode while a molecular weight (M + H} of 359.0811 was found in the positive mode, corresponding to the empirical formula C~gH~40g and a molecular weight of 358.31.
The physicochemical and spectroscopic properties of the compound (II) can be summarized as follows:
Appearance: lemon-yellow crystalline substance which is soluble in medium-polar and polar organic solvents. Stable in neutral and mildly acid medium but unstable in strongly acidic and alkaline solutions and under the influence of oxygen.
Empirical formula: C~gH~40g Molecular weight: 358.31 UV maxima: 220, 245, 307 and 365 nm in water/acetonitrile (1:1) at pH 2.
Table 1: Chemical shifts of the compound (II) in DMSO at 300 K.
H C
2 - 151.57 3 7.47 108.94 3a - 122.83 4 - 117.21 5 - 127.54 5-Me 2.58 11.03 6 - 140.91 6-OH broad -7 - 136.42 7-OH broad -7a - 142.35 8 10.42 190.2 broad) 9 - 124.84 10 - 112.61 11 - 150.17 11-OH 12.1 (broad)-12 - 132.68 12-OH broad -13 - 151.52 13-OH broad -14 - 118.72 14-Me 2.01 12.66 15 9.48 194.74 Example 8: Methylating the compound of the formula (II) 12 mg of the compound of the formula (II), obtained as described in example 5, were dissolved in 3 ml of methanol after which 1 ml of (trimethylsilyl)diazomethane [2 M solution in hexane, Aldrich] was added.
The reaction mixture was left to stand at room temperature and the course of the reaction was monitored by HPLC. After the compound of the formula (II) employed had been completely reacted, the reaction was terminated by adding water and concentrating in vacuo. The resulting methylation products were purified chromatographically on a Luna 5N RP18 phenomenex~ column using a gradient containing 0.02% trifluoroacetic acid and acetonitrile. After the pure fractions had been freeze-dried, the following were obtained by means of HPLC (conditions as in example 5):
2 mg of compound of the formula (III), monomethyl ether, retention time, 15.4 minutes, 2.7 mg of compound of the formula (I~, dimethyl ether, retention time, 16.9 minutes, 1.9 mg of compound of the formula (~, trimethyl ether, retention time, 19.4 minutes.
Example 9: Characterizing the compound of the formula (Ill) In ESI-MS, the compound of the formula (III) gave a molecular peak of 373.0 in the positive mode (M + H) and of 371.0 in the negative mode (M -H), corresponding to a MW = 372 and an empirical formula of C~gH~gOg.
8 i 5/ 4 3a 3 15 1 I ~ 10 OH
HO 6 ~7a O 14 ~ \ 11 OH
112' OH
Table 2: Chemical shifts of the compound (III) in DMSO at 300 K.
H C
2 - 150.95 3 7.51 109.16 3a - 122.65 4 - 117.28 - 127.75 5-Me 2.58 11.06 6 - 141.03 6-OH broad -7 - 136.47 7-OH broad -7a - 142.45 8 10.42 190.24 9 - 129.11 - 112.98 11 - 154.87 11-OH 12.22 -12 - 134.76 12-OMe 3.83 60.28 13 - 155.68 13-OH broad -14 - 119.05 14-Me 2.01 12.66 9.49 194.73 Example 10: Characterizing the compound of the formula (I~
In ESI-MS, the compound of the formula (I~ gave a molecular peak of 387.1 in the positive mode (M + H) and of 385.0 in the negative mode, corresponding to a MW = 386 and an empirical formula of C2pH~gOg.
Table 3: Chemical shifts of the compound (I~ in DMSO at 300 K.
H C
2 - 151.51 3 7.51 108.72 3a - 122.93 4 - 119.83 5 - 127.10 5-Me 2.58 10.86 6 - 143.62 6-OH 9.21 -7 - 137.18 7-OMe 4.15 60.44 7a - 143.74 8 10.48 190.88 9 - 122.97 10 - 115.84 11 - 150.54 11-OH 11.70 -12 - 139.24 12-OH 9.68 -13 - 151.69 13-OMe 3.87 59.90 14 - 123.98 14-Me 2.08 12.80 15 ~ 9.72 ~ 195.45 Example 11: Characterizing the compound of the formula (~
5 In ESI-MS, the compound of the formula (~ gave a molecular peak of 401.1 in the positive mode (M + H) and of 399.0 in the negative mode (M -H), corresponding to MW = 400 and an empirical formula of C2~H2pOg.
Table 4: Chemical shifts of the compound (~ in DMSO at 300 K.
H "C
2 - 150.90 3 7.56 108.95 3a - 122.73 4 - 119.91 - 127.28 5-Me 2.58 10.85 6 - 143.74 6-OH 9.25 -7 - 137.18 7-OMe 4.14 60.45 7a - 143.82 8 10.48 190.88 9 - 127.83 - 116.20 11 - 155.63 11-OH 11.82 -12 - 140.70 12-OMe 3.88 60.53 13 - 156.89 13-OMe 3.98 60.74 14 - 123.77 14-Me 2.06 12.85 ~ 9.73 ~ 195.00
Claims (14)
1. A compound of the formula (I) wherein R1 and R2 are, independently of each other, H, OH or -O-(C1-C6)-alkyl, and R3, R4, R5, R6 and R7 are, independently of each other, H, -(C1-C6)-alkyl or -C(O)-(C1-C6)-alkyl, or a physiologically tolerated salt of a compound of the formula (I).
2. A compound of the formula (I) as claimed in claim 1, wherein R1 and R2 are H.
3. A compound of the formula (I) as claimed in claim 1 or 2, wherein R3, R4, R5, R6 and R7 are, independently of each other, H or methyl.
4. A compound of the formula (I) as claimed in one of claims 1 to 3, which is characterized by a compound of the formula (II)
5. A compound of the formula (I) as claimed in one of claims 1 to 3, which is characterized by a compound of the formula (III)
6. A compound of the formula (I) as claimed in one of claims 1 to 3, which is characterized by a compound of the formula (IV) (IV).
7. A compound of the formula (I) as claimed in one of claims 1 to 3, which is characterized by a compound of the formula (V) (V).
8. A process for preparing a compound of the formula (I) as claimed in one of claims 1 to 7, which comprises 1. fermenting the microorganism Aspergillus flavipes ST003878 (DSM 15290), or one of its variants and/or mutants, in a culture medium until one or more compounds of the formula (I) accrues in the culture medium, and 2. isolating a compound of the formula (I) from the culture medium, and 3. where appropriate derivatizing the compound of the formula (I) and/or converting it into a physiologically tolerated salt.
9. The process as claimed in claim 8, wherein, during the fermentation, the compound of the formula (II) is formed in step 1, the compound of the formula (II) is isolated in step 2 and, in step 3, it is derivatized, where appropriate, to give a compound of the formula (I) and/or converted into a physiologically tolerated salt.
10. The use of a compound of the formula (I) as claimed in one of claims 1 to 7, or of a physiologically tolerated salt thereof, for producing a pharmaceutical in human or animal medicine.
11. The use of a compound of the formula (I) as claimed in claim 10 for producing a pharmaceutical for the treatment and/or prophylaxis of bacterial infectious diseases and/or mycoses.
12. A pharmaceutical having a content of at least one compound of the formula (I) according to the invention as claimed in one of claims 1 to 7, or of a physiologically tolerated salt thereof.
13. A process for producing a pharmaceutical as claimed in claim 12, which comprises mixing at least one compound of the formula (I) with one or more pharmacologically suitable auxiliary substances or carrier substances.
14. The microorganism Aspergiltus flavipes ST003878 (DSM 15290).
Applications Claiming Priority (3)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| DE10351315.9 | 2003-10-31 | ||
| DE10351315A DE10351315A1 (en) | 2003-10-31 | 2003-10-31 | 2-phenyl-benzofuran derivatives, process for their preparation and their use |
| PCT/EP2004/011695 WO2005047275A1 (en) | 2003-10-31 | 2004-10-16 | 2-phenyl-benzofuran derivatives, method for the production thereof and their use |
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| Publication Number | Publication Date |
|---|---|
| CA2543629A1 true CA2543629A1 (en) | 2005-05-26 |
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| Application Number | Title | Priority Date | Filing Date |
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| CA002543629A Abandoned CA2543629A1 (en) | 2003-10-31 | 2004-10-16 | 2-phenyl-benzofuran derivatives, method for the production thereof and their use |
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| Country | Link |
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| EP (1) | EP1689731B1 (en) |
| JP (1) | JP4758905B2 (en) |
| KR (1) | KR20060110873A (en) |
| CN (1) | CN1875012A (en) |
| AR (1) | AR046212A1 (en) |
| AT (1) | ATE356120T1 (en) |
| AU (1) | AU2004288737A1 (en) |
| BR (1) | BRPI0415978A (en) |
| CA (1) | CA2543629A1 (en) |
| DE (2) | DE10351315A1 (en) |
| IL (1) | IL174975A0 (en) |
| MX (1) | MXPA06004082A (en) |
| UY (1) | UY28592A1 (en) |
| WO (1) | WO2005047275A1 (en) |
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| US20100249165A1 (en) * | 2007-06-08 | 2010-09-30 | University Of Copenhagen | Pdz domain modulators |
| CN101914080B (en) * | 2010-08-05 | 2012-10-03 | 上海交通大学 | Benzofuran-3-ketone substitute phenyl compound as well as preparation method and application |
| CN103242273B (en) | 2012-02-09 | 2015-06-03 | 中国科学院上海药物研究所 | 2-arylbenzofuran-7-methanamide compound, preparation method and application thereof |
| WO2014037349A1 (en) * | 2012-09-05 | 2014-03-13 | Bayer Cropscience Ag | Use of substituted 2,3-dihydro-1-benzofuran-4-carboxylic acids or salts thereof as active substances against abiotic plant stress |
| EP3360549A1 (en) | 2017-02-14 | 2018-08-15 | Rheinische Friedrich-Wilhelms-Universität Bonn | Small molecule therapeutics for treating metachromatic leukodystrophy |
| CN115943957B (en) * | 2022-07-18 | 2024-01-26 | 北京景霁智惠科技有限公司 | Application of TBFC in preparation of medicines for preventing and treating bacterial diseases |
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| JPS6143182A (en) * | 1984-08-03 | 1986-03-01 | Ss Pharmaceut Co Ltd | Novel antibiotic ss19508d and preparation thereof |
| JP2955395B2 (en) * | 1990-12-14 | 1999-10-04 | メルシャン株式会社 | Antifungal substance Mer-WF5027 and method for producing the same |
| WO2002010156A1 (en) * | 2000-07-29 | 2002-02-07 | Arpida Ag | Benzofuran derivatives and their use as antibacterial agents |
| GB2386891A (en) * | 2002-03-28 | 2003-10-01 | Pantherix Ltd | Antibacterial benzofuran-2H-3-ones |
| AU2003241562B9 (en) * | 2002-05-17 | 2008-05-15 | The Government Of The United States Of America As Represented By The Secretary Of The Department Of Health And Human Services, Centers For Disease Control And Prevention | Molecular identification of Aspergillus species |
-
2003
- 2003-10-31 DE DE10351315A patent/DE10351315A1/en not_active Withdrawn
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2004
- 2004-10-16 JP JP2006537126A patent/JP4758905B2/en not_active Expired - Fee Related
- 2004-10-16 MX MXPA06004082A patent/MXPA06004082A/en not_active Application Discontinuation
- 2004-10-16 AT AT04790531T patent/ATE356120T1/en not_active IP Right Cessation
- 2004-10-16 EP EP04790531A patent/EP1689731B1/en not_active Expired - Lifetime
- 2004-10-16 KR KR1020067008283A patent/KR20060110873A/en not_active Application Discontinuation
- 2004-10-16 BR BRPI0415978-0A patent/BRPI0415978A/en not_active Application Discontinuation
- 2004-10-16 DE DE502004003187T patent/DE502004003187D1/en not_active Expired - Lifetime
- 2004-10-16 WO PCT/EP2004/011695 patent/WO2005047275A1/en active IP Right Grant
- 2004-10-16 CA CA002543629A patent/CA2543629A1/en not_active Abandoned
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- 2004-10-16 CN CNA2004800326034A patent/CN1875012A/en active Pending
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| Publication number | Publication date |
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| DE502004003187D1 (en) | 2007-04-19 |
| JP4758905B2 (en) | 2011-08-31 |
| AR046212A1 (en) | 2005-11-30 |
| EP1689731A1 (en) | 2006-08-16 |
| AU2004288737A1 (en) | 2005-05-26 |
| WO2005047275A1 (en) | 2005-05-26 |
| UY28592A1 (en) | 2005-05-31 |
| DE10351315A1 (en) | 2005-06-16 |
| JP2007512238A (en) | 2007-05-17 |
| CN1875012A (en) | 2006-12-06 |
| ATE356120T1 (en) | 2007-03-15 |
| EP1689731B1 (en) | 2007-03-07 |
| IL174975A0 (en) | 2006-08-20 |
| MXPA06004082A (en) | 2006-06-27 |
| BRPI0415978A (en) | 2007-01-23 |
| KR20060110873A (en) | 2006-10-25 |
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