EP0000037A1 - Method of producing salinomycin type antibiotics and new salinomycin type antibiotics - Google Patents

Method of producing salinomycin type antibiotics and new salinomycin type antibiotics Download PDF

Info

Publication number
EP0000037A1
EP0000037A1 EP78100061A EP78100061A EP0000037A1 EP 0000037 A1 EP0000037 A1 EP 0000037A1 EP 78100061 A EP78100061 A EP 78100061A EP 78100061 A EP78100061 A EP 78100061A EP 0000037 A1 EP0000037 A1 EP 0000037A1
Authority
EP
European Patent Office
Prior art keywords
salinomycin
salinomycins
producing
fatty acid
culture
Prior art date
Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.)
Granted
Application number
EP78100061A
Other languages
German (de)
French (fr)
Other versions
EP0000037B1 (en
Inventor
Yukio Miyazaki
Akira Shibata
Tateo Yahagi
Masayuki Hara
Kaoru Hara
Singo Yoneda
Hiroko Kasahara
Yuko Nakamura
Current Assignee (The listed assignees may be inaccurate. Google has not performed a legal analysis and makes no representation or warranty as to the accuracy of the list.)
Kaken Pharmaceutical Co Ltd
Original Assignee
Kaken Chemical Co Ltd
Priority date (The priority date is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the date listed.)
Filing date
Publication date
Application filed by Kaken Chemical Co Ltd filed Critical Kaken Chemical Co Ltd
Publication of EP0000037A1 publication Critical patent/EP0000037A1/en
Application granted granted Critical
Publication of EP0000037B1 publication Critical patent/EP0000037B1/en
Expired legal-status Critical Current

Links

Classifications

    • CCHEMISTRY; METALLURGY
    • C07ORGANIC CHEMISTRY
    • C07HSUGARS; DERIVATIVES THEREOF; NUCLEOSIDES; NUCLEOTIDES; NUCLEIC ACIDS
    • C07H19/00Compounds containing a hetero ring sharing one ring hetero atom with a saccharide radical; Nucleosides; Mononucleotides; Anhydro-derivatives thereof
    • C07H19/01Compounds containing a hetero ring sharing one ring hetero atom with a saccharide radical; Nucleosides; Mononucleotides; Anhydro-derivatives thereof sharing oxygen

Definitions

  • the present invention relates to an improvement in a method of producing polyether type antibiotics on an industrial sc le.
  • Salinomvcin 4-methvlsalino- mycin, SY-1, SY-2, SY-3, SY-4, SY-5, SY-6, SY-7 and SY-8 substance are called Salinomycin type antibiotics because they have similar chemical structures.
  • salinomycins means each compound, or any mixture of at least two compounds, selected from the group SY-7, SY-8 consisting of salinomycin, SY-1, SY-2, SY-3, SY-4, SY-5, SY-6/and the like.
  • the present inventors already found that salinomycin, SY-1 and SY-2 were produced in the culture of Streptomyces albus waxman and henrich No.80614 strain ( FERM-P. No.419 ), and succeeded in isolating the antibiotics from the culture ( British Patent No.1378414, Japanese Unexamined Patent Publication No. 86191/1976 and Japanese Patent Application No. 5762/1977).
  • the inventors continued the study and found that, when the above strain is cultured in a medium containing fatty acid or its precursor, it produces salinomycin, SY-1, and SY-2 ' in high yield, and also produces new compounds such as SY-3, SY-4, SY-5, SY-6, SY-7 and SY-8.
  • Another object of the present invention is to provide a method of producing Salinomycin type antibiotics such as salinomycin, 4-methylsalinomycin, SY-1, SY-2, SY-3, SY-4, SY-5, SY-6, SY-7 and SY-8 substances in high yield.
  • Salinomycin type antibiotics such as salinomycin, 4-methylsalinomycin, SY-1, SY-2, SY-3, SY-4, SY-5, SY-6, SY-7 and SY-8 substances in high yield.
  • salinomycin type antibiotics such as salinomycin, 4-methylsalinomycin, SY-1, SY-2, SY-3, SY-4, SY-5, SY-6, SY-7 and SY-8 substances are produced by culturing a salinomycin type antibiotic-producing microorganism in a medium containing a fatty acid or its precursor and ammonia or an ammonium salt or urea.
  • the fatty acids used in the present invention are saturated or unsaturated fatty acids, for example, acetic acid, propionic acid, caproic acid, capric acid, palmitic acid, stearic acid, methacrylic acid, undecylic acid, and particularly linolic acid, linolenic acid or oleic acid being preferable.
  • the precursor of fatty acid means a substance that is capable of giving said fatty acid .outside or inside the microorganism cell, such as mono- di- or triglycerides of fatty acid, esters of fatty acid or salts of fatty acid.
  • esters with The esters of fatty acid can be/C1-C18 alcohols of said fatty acid.
  • the salts of fatty acid can be ammonium salt and alkali metal salts and alkaline earth metal salts of said fatty acid.
  • the addition amount is generally about 1-25 % , particularly about 12-20% based on the medium.
  • Ammonia is used in gaseous form or in the form of an aqueous solution.
  • ammonium salt there are used ammonium salts of inorganic acids such as hydrochloric acid, sulfuric acid, nitric acid and phosphoric acid or organic acids such as acetic acid, propionic acid, higher fatty acid, oxalic acid, tartaric acid, hydrogentartaric acid, citric acid, lactic acid and malic acid.
  • the addition amount is generally about 0.1-1.0% particularly about 0.3-0.5% based on the medium.
  • addition is effective so long as production of potency of I the addition polyether type antibiotic continues, and / is conducted at any time either before or after beginning of cultivation.
  • cultivation conditions of the present invention can be selected in accordance with the methods described in said known literatures, excepting that fatty acid or its precursor is used as major carbon source and that ammonia or ammonium salt is used as essential component of the medium, it is possible to raise the production efficiency by varying the conditions depending on the kind of antibiotics.
  • microorganismsused in the present invention include generally polyether type antibiotics producing strains belonging to the genus of Streptomyces as well as the strains described in said literatures and their natural or artificial mutants.
  • Separation and purification of the products can be carried out in accordance with known methods. Since the objective substance is often contained mainly in the solid portion containing the cells when the production amount of the objective substance is abundant, it is desirable to vary the extraction step properly in order to heighten the recovery percentage of the objective substance from the solid portion. It is possible to use the objective compound in the state that it is contained in the solid portion depending on the use purposes, without separating the objective substance from the solid portion.
  • the production amount of polyether type antibiotics, particularly Salinomycin type antibiotics can be remarkably increased.
  • the yield of Salinomycin is generally 100-300 Y/ml in known method, whereas the yield is about 10,000-20,000 y/ml in the medium containing fatty acid or its precursor, and the yield is further increased to about 50,000-80,000 Y/ml when said medium contains further ammonia or ammonium salt.
  • salinomycins mainly occur in the mycelial mass,and it is preferrable to recover salinomycins from the mycelial mass.
  • other new compounds especially SY-3, SY-4, SY-5, SY-6 and the like are obtained from the culture.
  • the strains used in this invention include Streptomyces albus No.80614 and its mutants artificially or naturally produced, as well as the other Streptomyces strains capable of producing salinomycins. However, some of the salinomycins can occasionally not be detected in the culture, depending on the strain and fermentation conditions.
  • Fermentation conditions employed in this invention can be any one commonly used for culturing Actinomycetes, except that main carbon source should be a fatty acid or its precursor. Maximum production of salinomycins usually occurs after 150 to 260 hours The from the start of fermentation. /ratio of each of salinomycins produced sometimes varies depending on the incubation time. Naturally, the composition of medium and fermentation conditions should be decided for each strain and external conditions, so that most desirable results are obtained.
  • Salinomycins can be isolated from the culture medium by utilizing the physico-chemical properties of salinomycins. Because salinomycins are structurally related to each other, the known extraction methods for salinomycin and SY-1 can be applied to the isolation of salinomycins, however, as for salinomycin, because a large portion of salinomycin is contained in mycelial mass, the extraction process is preferrably modified so as to increase the recovery rate of salinomycin. For example, it is preferred to adjust the whole fermentation broth to PH 2.0-6.0 to precipitate salinomycin, and then to extract the mycelial mass together with the precipitate thus formed with an organic solvent.
  • the preferred solvents are acetone, ethyl acetate, butyl acetate, n-hexane, chloroform and the like.
  • the effluent is collected in 2-5 fractions according to the purpo-e. Separation and purification of salinomycins are effected by the procedures utilizing the difference between the properties of desired compound and imprities. Chromatograpy, solvent extraction and the like are repeated for each fraction to give salinomycin, SY-1, SY-2, SY-3, SY-4, SY-5, SY-6, SY-7, SY-8 anc the like, individually or as mixtures. The resulting products can be further purified by recrystallization or chromatography.
  • Table 1 The properties of salinomycins obtained by the process of this invention are shown in the following table 1.
  • salinomycin, SY-1, and SY-2 especially salinomycin are obtained in surprisingly higher yield than the known process.
  • New compounds, SY-3 through -8 are also obtained according to this invention. They are comparable to salinomycin in their activities against microorganisms and useful as medicines. Also, because of their structural similarity to salinomycin, their usefulness as veterinary medicines looks very likely.
  • Streptomyces albus waxman and henrich No.80614 strain (FERM-P. No.419) is inoculated to a medium containing glycerine 2.0%, peptone 0.5% and meat extract 0.5% and cultured at 33°C for 48 hours under shaking.
  • 1 litre of this culture liquid is inoculated to 100 litres of liquid medium ( 200 litre tank made of stainless steel ) containing glucose 2%, starch 1%, soy bean powder 2.5%, beer yeast 0.4%, meat extract 0.1%, sodium chloride 0.2% and antifoaming agent KM-68-2F ( product of Shinetsu Chemical Industry Co., Ltd., silicone type ) 0.1% and cultured at 33°C for 144 hours under stirring with the aeration volume of 100 1/m. There is obtained a culture liquid containing .100-300 y/ml of Salinomycin.
  • the 80614 strain which is the same strain as described in Example 1 is inoculated to a medium containing glycerine 2.0%, peptone 0.25%, meat extract 0.5% and edible salt 0.1%, and cultured at 33°C for 48 hours under shaking.
  • This culture liquid in an amount corresponding to 1% of the medium is inoculated to the medium containing glucose 4.0%, soy bean powder 1.0%, beer yeast 1.0% and calcium carbonate 0.2%, and cultured for 30 hours at 33°C under shaking, and this culture liquid is made the second-stage pre-culture liquid.
  • This second-stage pre-culture liquid is inoculated to 100 litres of liquid medium containing soy bean oil 10%, glucose 1.0%, soy bean powder 1.0%, calcium carbonate 0.5%, potassium secondary phosphate 0.01%, and cultured for 210 hours at 33°C with an aeration volume of 100 1/m under stirring. There is obtained a culture liquid containing 20,000 Y/ml of Salinomycin.
  • the 80614 strain which is the same strain as described in Example 1 is inoculated to a medium containing glycerine 2.0%, peptone 0.25%, meat extract 0.5% and edible salt 0.1%, and cultured at 33°C for 48 hours under shaking.
  • This culture liquid in an amount corresponding to 1% of the medium is inoculated to the medium containing glucose 4.0%, soy bean powder 1.0%, beer yeast 1.0% and calcium carbonate 0.2%, and cultured for 30 hours at 33°C under shaking, and this culture liquid is made the second-stage, pre-culture liquid.
  • This second-stage pre-culture liquid is inoculated to 100 litres of liquid medium containing soy.bean oil 10%, glucose 1.0%, soy bean powder 1.0%, calcium carbonate 0.5%, potassium secondary phosphate 0.01%, and cultured for 210 hours at 33°C with an aeration volume of 100 1/m under stirrinq. There is obtained a culture liquid containing 20,000 ⁇ /ml of salinomycin(salinomycin only).
  • the culture liquid obtained in (A) is adjusted to PH 4.5-5.0 with dilute hydrochloride, admixed with 4% by weight per volume of filter aid with stirring, and filtered.
  • the filtrate ( 80 litres ) is extracted with 50 litres of butyl acetate with stirring.
  • Mycelial mass is extracted with 30 litres of butyl acetate.
  • Both butyl acetate solutions are combined and washed with 20 litres of 5% aqueous sodium bicarbonate solution.
  • One litre of the washed butyl acetate solution is concentrated under vacuum to dryness to give 250g of crude powder of salinomycin containing trace amount of SY-1 and SY-2.
  • the almina column as mentioned above is further developed with a 100:15 mixture of ethyl acetate-methanol to elute SY-2, which is separated and purified by silica gel chromatography in the same manner as described above, and crystallized from acetone-water solution to give 3mg of pure crystalline SY-2.
  • the culture obtained in (A) is adjusted to pH 4.5-5.0, heated at 60°C for 10 minutes with stirring, admixed with 4% by weight per volume of filter aid with stirring and filtered.
  • the resulting mycelial mass contains salinomycins and SY group compounds in high yield.
  • Mycelial mass obtained in (B) is extracted twice with 50 litres of ethyl acetate. The extracts are combined and washed with 50 litres of 5% aqueous sodium bicarbonate solution. Ethyl acetate phase is concentrated under vacuum to dryness to yield 7kg of crude salinomycins complex containing SY group compounds.
  • the mother liquor separated from the precipitate in the process in (A) is concentrated to dryness to give 4.6kg of complex contain-- ing a small amount of salinomycin and SY group compounds.
  • the complex is dissolved in 50 litres of hexane-ethyl acetate solvent mixture (2:1) and applied to the column of 12kg of almina packed in the same solvent system, developed with 20 litres of a 100:2 mixture of ethyl acetate-methanol to elute SY-3, SY-7 and salinomycin.
  • Two hundred g of the mixture of salinomycin and SY-1 is separated by precipitation in the same manner as described in (D).
  • the filtrate containing SY-3 and SY-7 is concentrated to dryness to give 100g of crude powder.
  • the above almina column is eluted with 20 litres of a 5:1 mixture of ethyl acetate-methanol, and the effluent is concentrated under vacuum to give 200g of crude powder, which contains the complex of SY-2, SY-4, SY-5, SY-6 and SY-8.
  • These compounds are isolated individually by silica gel column chromatography. Two hundred g of the crude powder is dissolved in 500ml of a 100:2 mixture of chloroform-methanol, applied to the column of 2kg silica gel (Wakogel C-200) packed in the same solvent mixture, and developed with the same solvent mixture to give.each fraction containing SY-2, SY-4, SY-5, SY-6 and SY-8, respectively.
  • Example 1 The second-stage pre-culture liquid of Example 1 in an amount corresponding 10% of the medium is inoculated to the medium containing glucose 4%, soy bean powder 3%, defatted wheat germs 3.0%, calcium carbonate 0.2% and antifoaming agent KM-68-2F 0.1%, and cultured for 24 hours at 33°C to give the third-stage pre-culture liquid.
  • the complex is dissolved in 600ml of chloroform-methanol solution(100:2), and then treated by chromatography(20kg silica gel) in the same manner as described above to give 40g of SY-2, 600mg each of SY-4 and SY-5, 1900mg of SY-6 and 300ing of SY-8 as crude powders, purification of which according to the procedure of Example 2 (E) gives 30g of crystallin SY-2, 180mg of SY-4 powder, 120mg of SY-5 powder, 350mg of SY-6 powder and 90mg of SY-8 powder, all in pure form.
  • the third-stage pre-culture liquid in Example 3 in an amount corresponding to 10% of the medium is inoculated to the medium (50ml-) containing each fat-and-oil shown in the following Table 12%, soy bean powder 0.5%, defatted wheat germs 1.0%, sodium chloride 0.2%, potassium chloride 0.2%, calcium carbonate 0.5%, ammonium sulfate 0.3%, potassium secondary phosphate,0.02% and magnesium sulfate 0.01%, and cultured at 33°C for 216 hours under shaking.
  • the production amounts of salinomycin at the end of cultivation are shown in the following Table.

Landscapes

  • Chemical & Material Sciences (AREA)
  • Organic Chemistry (AREA)
  • Health & Medical Sciences (AREA)
  • Life Sciences & Earth Sciences (AREA)
  • Engineering & Computer Science (AREA)
  • Biochemistry (AREA)
  • Biotechnology (AREA)
  • General Health & Medical Sciences (AREA)
  • Genetics & Genomics (AREA)
  • Molecular Biology (AREA)
  • Preparation Of Compounds By Using Micro-Organisms (AREA)

Abstract

Polyether type antibiotics, such as salinomycin, 4-methyl- salinomycin and compounds designated by SY-1 up to SY-8, and their production by polyether-type antibiotic-producing micro-organisms belonging to, a.o., Streptomyces albus Waxman & Heinrich Nr.80614 (FERM-P Nr.419) in a medium containing a fatty acid or its precursor, and, optionally, ammonia or an ammonium salt or urea.

Description

    BACKGROUND OF THE INVENTION:
  • The present invention relates to an improvement in a method of producing polyether type antibiotics on an industrial sc le.
  • As polyether type antibiotic,there have been known Monensin (sournal of American Chemical Society, Vol.89, page 5757, 1 67), X-206 (Chemical Communications. 927, 1971), Salinomycin (Br tish Patent No. 1,378,414), SY-1 substance (Japanese O.P.I. 86191/76), S' 2 substance (Japanese Patent Application No. 5762/77), 4-methylsalinomycin (A 2808b substance) Japanese O.P.I. 9788/76, Losalocid (Journal of American Chemical Society, Vol.73, 5295, 1951) Dianemycin ( Journal of Antibiotics, Vol. 22, page 161, 1969 ), Nigericin ( Biochemical and Biophysical Research Communication, Vol.33, page 29, 1968 ), A-204 A ( Journal of American Chemical Society, Vol. 95, 3399, 1973 )
    and the like, and among these, Salinomvcin, 4-methvlsalino- mycin, SY-1, SY-2, SY-3, SY-4, SY-5, SY-6, SY-7 and SY-8 substance are called Salinomycin type antibiotics because they have similar chemical structures.
  • In this invention, the term "salinomycins" means each compound, or any mixture of at least two compounds, selected from the group SY-7, SY-8 consisting of salinomycin, SY-1, SY-2, SY-3, SY-4, SY-5, SY-6/and the like.
  • The present inventors already found that salinomycin, SY-1 and SY-2 were produced in the culture of Streptomyces albus waxman and henrich No.80614 strain ( FERM-P. No.419 ), and succeeded in isolating the antibiotics from the culture ( British Patent No.1378414, Japanese Unexamined Patent Publication No. 86191/1976 and Japanese Patent Application No. 5762/1977).
  • The inventors continued the study and found that, when the above strain is cultured in a medium containing fatty acid or its precursor, it produces salinomycin, SY-1, and SY-2'in high yield, and also produces new compounds such as SY-3, SY-4, SY-5, SY-6, SY-7 and SY-8.
  • As described in said literatures, these are produced by culturing an antibiotic producing microorganism belonging to the genus of Streptomyces. However, the yield of each antibiotic produced by such known method is not always satisfactory.
    • SUMMARY OF THE INVENTION:
  • It is an object of the present invention to provide a method of producing polyether type antibiotics in remarkably high yields with industrial advantages.
  • Another object of the present invention is to provide a method of producing Salinomycin type antibiotics such as salinomycin, 4-methylsalinomycin, SY-1, SY-2, SY-3, SY-4, SY-5, SY-6, SY-7 and SY-8 substances in high yield.
  • The foregoing and other objects of the present invention have been attained by culturing a polyether type antibiotic-producing microorganism in a medium containing a fatty acid or its precursor and ammonia or an ammonium salt or urea.
    • DETAILED DESCRIPTION OF THE PREFERRED EMBODIMENTS:
  • In the special feature of the present invention, salinomycin type antibiotics such as salinomycin, 4-methylsalinomycin, SY-1, SY-2, SY-3, SY-4, SY-5, SY-6, SY-7 and SY-8 substances are produced by culturing a salinomycin type antibiotic-producing microorganism in a medium containing a fatty acid or its precursor and ammonia or an ammonium salt or urea.
  • The fatty acids used in the present invention are saturated or unsaturated fatty acids, for example, acetic acid, propionic acid, caproic acid, capric acid, palmitic acid, stearic acid, methacrylic acid, undecylic acid, and particularly linolic acid, linolenic acid or oleic acid being preferable. The precursor of fatty acid means a substance that is capable of giving said fatty acid .outside or inside the microorganism cell, such as mono- di- or triglycerides of fatty acid, esters of fatty acid or salts of fatty acid. Further, there can be used soy bean oil, safflower oil, cotton seed oil, sesame oil, olive oil, rape oil, peanut oil, maize oil (corn oil), sunflower oil and like vegetable oils, cod oil and like fish oils and lard and like animal fat-and-oils, which contain said precursors. esters with The esters of fatty acid can be/C1-C18 alcohols of said fatty acid.
    The salts of fatty acid can be ammonium salt and alkali metal salts and alkaline earth metal salts of said fatty acid.
  • The addition amount is generally about 1-25%, particularly about 12-20% based on the medium.
  • Ammonia is used in gaseous form or in the form of an aqueous solution. As ammonium salt there are used ammonium salts of inorganic acids such as hydrochloric acid, sulfuric acid, nitric acid and phosphoric acid or organic acids such as acetic acid, propionic acid, higher fatty acid, oxalic acid, tartaric acid, hydrogentartaric acid, citric acid, lactic acid and malic acid. The addition amount is generally about 0.1-1.0% particularly about 0.3-0.5% based on the medium.
  • As for the time for addition of these additives, addition is effective so long as production of potency of I the addition polyether type antibiotic continues, and/is conducted at any time either before or after beginning of cultivation. Although the cultivation conditions of the present invention can be selected in accordance with the methods described in said known literatures, excepting that fatty acid or its precursor is used as major carbon source and that ammonia or ammonium salt is used as essential component of the medium, it is possible to raise the production efficiency by varying the conditions depending on the kind of antibiotics.
  • The microorganismsused in the present invention include generally polyether type antibiotics producing strains belonging to the genus of Streptomyces as well as the strains described in said literatures and their natural or artificial mutants.
  • Separation and purification of the products can be carried out in accordance with known methods. Since the objective substance is often contained mainly in the solid portion containing the cells when the production amount of the objective substance is abundant, it is desirable to vary the extraction step properly in order to heighten the recovery percentage of the objective substance from the solid portion. It is possible to use the objective compound in the state that it is contained in the solid portion depending on the use purposes, without separating the objective substance from the solid portion.
  • According to the present invention the production amount of polyether type antibiotics, particularly Salinomycin type antibiotics can be remarkably increased. For example, the yield of Salinomycin is generally 100-300 Y/ml in known method, whereas the yield is about 10,000-20,000 y/ml in the medium containing fatty acid or its precursor, and the yield is further increased to about 50,000-80,000 Y/ml when said medium contains further ammonia or ammonium salt.
  • The preferable feature of the present invention to produce salinomycin type antibiotics will be further illustrated.
  • According to the method of this invention, salinomycins mainly occur in the mycelial mass,and it is preferrable to recover salinomycins from the mycelial mass. In addition to salinoriiycin, SY-1, and SY-2, other new compounds, especially SY-3, SY-4, SY-5, SY-6 and the like are obtained from the culture.
  • The strains used in this invention include Streptomyces albus No.80614 and its mutants artificially or naturally produced, as well as the other Streptomyces strains capable of producing salinomycins. However, some of the salinomycins can occasionally not be detected in the culture, depending on the strain and fermentation conditions.
  • Fermentation conditions employed in this invention can be any one commonly used for culturing Actinomycetes, except that main carbon source should be a fatty acid or its precursor. Maximum production of salinomycins usually occurs after 150 to 260 hours The from the start of fermentation. /ratio of each of salinomycins produced sometimes varies depending on the incubation time. Naturally, the composition of medium and fermentation conditions should be decided for each strain and external conditions, so that most desirable results are obtained.
  • Salinomycins can be isolated from the culture medium by utilizing the physico-chemical properties of salinomycins. Because salinomycins are structurally related to each other, the known extraction methods for salinomycin and SY-1 can be applied to the isolation of salinomycins, however, as for salinomycin, because a large portion of salinomycin is contained in mycelial mass, the extraction process is preferrably modified so as to increase the recovery rate of salinomycin. For example, it is preferred to adjust the whole fermentation broth to PH 2.0-6.0 to precipitate salinomycin, and then to extract the mycelial mass together with the precipitate thus formed with an organic solvent. Among the preferred solvents are acetone, ethyl acetate, butyl acetate, n-hexane, chloroform and the like. After applying the solution to the absorptive materials suitable for the absorption of salinomycins, the salinomycins are eluted by a suitable solvent system.
  • The effluent is collected in 2-5 fractions according to the purpo-e. Separation and purification of salinomycins are effected by the procedures utilizing the difference between the properties of desired compound and imprities. Chromatograpy, solvent extraction and the like are repeated for each fraction to give salinomycin, SY-1, SY-2, SY-3, SY-4, SY-5, SY-6, SY-7, SY-8 anc the like, individually or as mixtures. The resulting products can be further purified by recrystallization or chromatography. The properties of salinomycins obtained by the process of this invention are shown in the following table 1.
    Figure imgb0001
    Figure imgb0002
  • According to the preferred feature of this invention, salinomycin, SY-1, and SY-2, especially salinomycin are obtained in surprisingly higher yield than the known process. New compounds, SY-3 through -8 are also obtained according to this invention. They are comparable to salinomycin in their activities against microorganisms and useful as medicines. Also, because of their structural similarity to salinomycin, their usefulness as veterinary medicines looks very likely.
    • REFERENCE EXAMPLE 1:
  • Streptomyces albus waxman and henrich No.80614 strain (FERM-P. No.419) is inoculated to a medium containing glycerine 2.0%, peptone 0.5% and meat extract 0.5% and cultured at 33°C for 48 hours under shaking. 1 litre of this culture liquid is inoculated to 100 litres of liquid medium ( 200 litre tank made of stainless steel ) containing glucose 2%, starch 1%, soy bean powder 2.5%, beer yeast 0.4%, meat extract 0.1%, sodium chloride 0.2% and antifoaming agent KM-68-2F ( product of Shinetsu Chemical Industry Co., Ltd., silicone type ) 0.1% and cultured at 33°C for 144 hours under stirring with the aeration volume of 100 1/m. There is obtained a culture liquid containing .100-300 y/ml of Salinomycin.
    • REFERENCE EXAMPLE 2:
  • The 80614 strain which is the same strain as described in Example 1 is inoculated to a medium containing glycerine 2.0%, peptone 0.25%, meat extract 0.5% and edible salt 0.1%, and cultured at 33°C for 48 hours under shaking. This culture liquid in an amount corresponding to 1% of the medium is inoculated to the medium containing glucose 4.0%, soy bean powder 1.0%, beer yeast 1.0% and calcium carbonate 0.2%, and cultured for 30 hours at 33°C under shaking, and this culture liquid is made the second-stage pre-culture liquid. One litre of this second-stage pre-culture liquid is inoculated to 100 litres of liquid medium containing soy bean oil 10%, glucose 1.0%, soy bean powder 1.0%, calcium carbonate 0.5%, potassium secondary phosphate 0.01%, and cultured for 210 hours at 33°C with an aeration volume of 100 1/m under stirring. There is obtained a culture liquid containing 20,000 Y/ml of Salinomycin.
    • EXAMPLE 1: (A) Production of salinomycin:
  • The 80614 strain which is the same strain as described in Example 1 is inoculated to a medium containing glycerine 2.0%, peptone 0.25%, meat extract 0.5% and edible salt 0.1%, and cultured at 33°C for 48 hours under shaking. This culture liquid in an amount corresponding to 1% of the medium is inoculated to the medium containing glucose 4.0%, soy bean powder 1.0%, beer yeast 1.0% and calcium carbonate 0.2%, and cultured for 30 hours at 33°C under shaking, and this culture liquid is made the second-stage, pre-culture liquid. One litre of this second-stage pre-culture liquid is inoculated to 100 litres of liquid medium containing soy.bean oil 10%, glucose 1.0%, soy bean powder 1.0%, calcium carbonate 0.5%, potassium secondary phosphate 0.01%, and cultured for 210 hours at 33°C with an aeration volume of 100 1/m under stirrinq. There is obtained a culture liquid containing 20,000 γ/ml of salinomycin(salinomycin only).
    • (B) Separation and purification of salinomycin, SY-1 and SY-2.
  • The culture liquid obtained in (A) is adjusted to PH 4.5-5.0 with dilute hydrochloride, admixed with 4% by weight per volume of filter aid with stirring, and filtered. The filtrate ( 80 litres ) is extracted with 50 litres of butyl acetate with stirring. Mycelial mass is extracted with 30 litres of butyl acetate. Both butyl acetate solutions are combined and washed with 20 litres of 5% aqueous sodium bicarbonate solution. One litre of the washed butyl acetate solution is concentrated under vacuum to dryness to give 250g of crude powder of salinomycin containing trace amount of SY-1 and SY-2.
  • Fifty grams of the crude salinomycin powder is dissolved in a ethyl acetate and applied to/column ( 50g of active almina, commercial product of Wako Junyaku Co. ). After washing the column with one litre of ethyl acetate, salinomycin and SY-1 are eluted with a 100:5 mixture of ethyl acetate-methanol solution. The fractions containing salinomycin and SY-1 are combined and concentrated. The concentrate is diluted in 50ml of chloroform-methanol solution ( 100:2 ) and applied to the column of 300g silica gel ( Wakogel-200, Wako Junyaku Co. ) packed in the same solvent mixture. Elution is carried out with the same solvent mixture to give pure salinomycin fraction and pure SY-1 fraction. Each fraction is concentrated and crystallized from acetone-water solution to give 5g of salinomycin and 30mg of SY-1 in pure crystals, respectively.
  • The almina column as mentioned above is further developed with a 100:15 mixture of ethyl acetate-methanol to elute SY-2, which is separated and purified by silica gel chromatography in the same manner as described above, and crystallized from acetone-water solution to give 3mg of pure crystalline SY-2.
    • EXAMPLE 2: (A) Salinomycin is cultured in the same manner as described in Example 1. (B) Recovery of salinomycins
  • The culture obtained in (A) is adjusted to pH 4.5-5.0, heated at 60°C for 10 minutes with stirring, admixed with 4% by weight per volume of filter aid with stirring and filtered. The resulting mycelial mass contains salinomycins and SY group compounds in high yield.
    • (C) Separation of salinomycins complex
  • Mycelial mass obtained in (B) is extracted twice with 50 litres of ethyl acetate. The extracts are combined and washed with 50 litres of 5% aqueous sodium bicarbonate solution. Ethyl acetate phase is concentrated under vacuum to dryness to yield 7kg of crude salinomycins complex containing SY group compounds.
    • (D) Separation and purification of salinomycin
  • Seven kg of crude powder obtained in (C) is dissolved in 100 litres of hexane, concentrated under vacuum to 20 litres and left at 5°C to give 2.7kg of crude crystallin salinomycin. After repeating this procedure, recrystallization of salinomycin from hexane gives 2.4kg of pure salinomycin sodium salt.
    • (E) Separation and purification of SY group compounds
  • The mother liquor separated from the precipitate in the process in (A) is concentrated to dryness to give 4.6kg of complex contain-- ing a small amount of salinomycin and SY group compounds. The complex is dissolved in 50 litres of hexane-ethyl acetate solvent mixture (2:1) and applied to the column of 12kg of almina packed in the same solvent system, developed with 20 litres of a 100:2 mixture of ethyl acetate-methanol to elute SY-3, SY-7 and salinomycin. Two hundred g of the mixture of salinomycin and SY-1 is separated by precipitation in the same manner as described in (D). The filtrate containing SY-3 and SY-7 is concentrated to dryness to give 100g of crude powder.
  • One hundred g of the crude powder thus obtained is dissolved in 300ml of a 100:2 mixture of chloroform-methanol and applied to the column of 6kg of silica gel (Wakogel C-200, Wako Junyaku Co.), and developed with the same solvent mixture. Each of SY-3 and SY-7 fractions is concentrated and applied to silica gel thin layer chromatogram (Wakogel B-10 with thickness of 0.25 mm, solvent system; a 20:1 mixture of chloroform-methanol). SY-3'and SY-7 are collected by scraping off the areas with Rf values 0.45 and 0.80, respectivelly. The silica gel holding each compound is eluted with a 20:1 mixture of chloroform-methanol and the solvent mixture is removed by evaporation to give l8mg of SY-3 and 35mg of SY-7 both in pure powders.
  • The above almina column is eluted with 20 litres of a 5:1 mixture of ethyl acetate-methanol, and the effluent is concentrated under vacuum to give 200g of crude powder, which contains the complex of SY-2, SY-4, SY-5, SY-6 and SY-8. These compounds are isolated individually by silica gel column chromatography. Two hundred g of the crude powder is dissolved in 500ml of a 100:2 mixture of chloroform-methanol, applied to the column of 2kg silica gel (Wakogel C-200) packed in the same solvent mixture, and developed with the same solvent mixture to give.each fraction containing SY-2, SY-4, SY-5, SY-6 and SY-8, respectively. Each fraction is concentrated to dryness to give 20g of SY-2, 300mg of SY-4, 250mg of SY-5, 800mg of SY-6 and 100mg of SY-8 as crude powders, respectively. Crude SY-2 powders are crystallized from acetone water to give 15g of pure crystalline SY-2.
  • Other crude powders are purified by thin layer chromatography of silica gel in the same manner as employed in the separation and purification of SY-3 and SY-7 to give 26mg of SY-4, 20mg of SY-5, 80mg of SY-6 and 30mg of SY-8 each in pure powders.
    • EXAMPLE 3:
  • (A) The second-stage pre-culture liquid of Example 1 in an amount corresponding 10% of the medium is inoculated to the medium containing glucose 4%, soy bean powder 3%, defatted wheat germs 3.0%, calcium carbonate 0.2% and antifoaming agent KM-68-2F 0.1%, and cultured for 24 hours at 33°C to give the third-stage pre-culture liquid.
  • Ten litres of the third-stage pre-culture liquid is inoculated to the medium containing soy bean oil 16%, soy bean powder 0.5%, defatted wheat germs 1.0%, sodium chloride 0.2%, potassium chloride 0.2%, ammonium sulfate 0.3%, calcium secondary phosphate 0.02%, magnesium sulfate 0.01% and antifoaming agent KM-68-2F 0.1%, and cultured for 290 hours at 33°C with an aeration volume of 100 1/m under stirring. The production amount of salinomycin at the end of cultivation is 60,000 Y/ml (salinomycin only). - In this case the similar production amount is attained even when soy bean oil is added in a small amount at the beginning and then the addition amount is increased. No difference in production amount is observed between cases in which silicone type and polyether type antifoaming agents are used.
  • (B) 'rreat the fermentation broth obtained in (A) according to the procedure of Example 2 (B) to give mycelial mass containig salinomycins in high yield.
  • (C) Treat the mycelial mass obtained in (B) according to the procedure of Example 2 (C) to give l6kg of the complex of SY-1, 2, 3, 4, 5, 6, 7 and 8.
  • (D) Dissolve l6kg of crude powder obtained in (C) in 100 litres of hexane and concentrate under vacuum to 40 litres. Then treat the solution according to the same procedure described in Example 2 (D) to give 7.lkg of crude crystallin salinomycin and then 6.3kg of pure salinomycin sodium salt.
  • (E) The mother liquor separated from crystals in the process in (D) is concentrated to dryness to give 9.7kg of the complex containing SY-1 through -8. The complex is dissolved in 100 litres of a 2:1 mixture of hexane-ethyl acetate, applied to the column of 20kg of aluminain the same manner as described in Example 2 (E) and developed with 30 litres of a 100:2 mixture of ethyl acetate-methanol to elute SY-1, SY-3 and SY-7. The effluent is treated in the same manner as described in Example 2 (E) to give 400g of salinomycin-SY-1 mixture and 130g of crude powder containing SY-3 and SY-7.
  • One hundred and thirty g of said crude powder is dissolved in 400ml of chloroform-methanol solution (100:2), treated by silica gel column chromatography (8kg of silica gel is used) to give SY-3- and SY-7-fractions. Each fraction is chromatographed over silica gel thin layer according to Example 2 (E), and after removing the solvent by evaporation, 30mg of SY-3 and 50mg of SY-7 are obtained as pure powders.
  • The above aluminacolumn is eluted with 40 litres of a 5:1 mixture of ethyl acetate-methanol and the effluent is concentrated to dryness to give 250g of crude powder containing the complex of SY-2, SY-4, SY-5, SY-6 and SY-7. The complex is dissolved in 600ml of chloroform-methanol solution(100:2), and then treated by chromatography(20kg silica gel) in the same manner as described above to give 40g of SY-2, 600mg each of SY-4 and SY-5, 1900mg of SY-6 and 300ing of SY-8 as crude powders, purification of which according to the procedure of Example 2 (E) gives 30g of crystallin SY-2, 180mg of SY-4 powder, 120mg of SY-5 powder, 350mg of SY-6 powder and 90mg of SY-8 powder, all in pure form.
    • EXAMPLE 4:
  • The third-stage pre-culture liquid in Example 3 in an amount corresponding to 10% of the medium is inoculated to the medium (50ml-) containing each fat-and-oil shown in the following Table 12%, soy bean powder 0.5%, defatted wheat germs 1.0%, sodium chloride 0.2%, potassium chloride 0.2%, calcium carbonate 0.5%, ammonium sulfate 0.3%, potassium secondary phosphate,0.02% and magnesium sulfate 0.01%, and cultured at 33°C for 216 hours under shaking. The production amounts of salinomycin at the end of cultivation are shown in the following Table.
    Figure imgb0003
  • From the resulting culture, salinomycins are separated individually and purified according to the procedures of Examples 1 - 3.

Claims (8)

1. A method of producing polyether type antibiotics by culturing a polyether type antibiotic-producing microorganism, characterized in that the microorganism is cultured in a medium containing fatty acid salt or its precursor and optionally ammonia or an ammonium/or urea.
2. A method according to claim 1, characterized in that a vegetable oil or an animal oil is used as precursor of fatty acid.
3. A method according to one of claims 1 or 2, characterized in that the polyether type antibiotic is a salinomycin type antibiotic.
4. A method of producing salinomycins by culturing a salinomycins-producing Streptomyces microorganism and recovering the salinomycin from the culture, characterized in that the microorganism is cultured in a medium containing fatty acid or its precursor and optionally ammonia or an ammonium salt or urea.
5. A method according to claim 4, characterized in that salinomycin is recovered together with the mycelial mass from the culture.
6. A method according to one of claims 4 or 5, characterized in that SY-1, SY-2, SY-3, SY-4, SY-5, SY-6, SY-7 and/or SY-8 is recovered from the culture.
7. Salinomycin type antiobiotic, produced by culturing a salinomycins producing Streptomyces microorganism in a medium containing fatty acid or its precursor and optionally ammonia or an ammonium salt or urea and recovering these salinomycins from the culture.
8. Salinomycin antiobtics SY-1, SY-2, SY-3, SY-5, SY-6, SY-7, SY-8, characterized by the properties stated in table 1.
EP19780100061 1977-06-01 1978-06-01 Method of producing salinomycin type antibiotics and new salinomycin type antibiotics Expired EP0000037B1 (en)

Applications Claiming Priority (2)

Application Number Priority Date Filing Date Title
JP6321577A JPS53148595A (en) 1977-06-01 1977-06-01 Preparation of salinomycines
JP63215/77 1977-06-01

Publications (2)

Publication Number Publication Date
EP0000037A1 true EP0000037A1 (en) 1978-12-20
EP0000037B1 EP0000037B1 (en) 1982-04-28

Family

ID=13222746

Family Applications (1)

Application Number Title Priority Date Filing Date
EP19780100061 Expired EP0000037B1 (en) 1977-06-01 1978-06-01 Method of producing salinomycin type antibiotics and new salinomycin type antibiotics

Country Status (3)

Country Link
EP (1) EP0000037B1 (en)
JP (1) JPS53148595A (en)
DE (1) DE2861764D1 (en)

Cited By (3)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US4450237A (en) * 1982-05-03 1984-05-22 Pfizer Inc. Streptomyces albus subspecies indicus
WO2001083801A2 (en) * 2000-05-04 2001-11-08 Biotika A.S. A method for isolating salinomycin from fermentation broth
US7053115B2 (en) 2003-04-07 2006-05-30 Hetero Drugs Limited Crystalline form of dorzolamide hydrochloride

Families Citing this family (1)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
CN1035333C (en) * 1992-04-28 1997-07-02 清远新北江制药有限公司 Method for prodn. of salino mycin and its sodium salt

Citations (3)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
NL6902863A (en) * 1968-02-23 1969-08-26
NL7503905A (en) * 1974-04-02 1975-10-06 Hoffmann La Roche ANTIBIOTICS.
NL7508629A (en) * 1974-07-23 1976-01-27 Hoechst Ag PROCESS FOR PREPARING MOENOMYCIN.

Patent Citations (3)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
NL6902863A (en) * 1968-02-23 1969-08-26
NL7503905A (en) * 1974-04-02 1975-10-06 Hoffmann La Roche ANTIBIOTICS.
NL7508629A (en) * 1974-07-23 1976-01-27 Hoechst Ag PROCESS FOR PREPARING MOENOMYCIN.

Cited By (4)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US4450237A (en) * 1982-05-03 1984-05-22 Pfizer Inc. Streptomyces albus subspecies indicus
WO2001083801A2 (en) * 2000-05-04 2001-11-08 Biotika A.S. A method for isolating salinomycin from fermentation broth
WO2001083801A3 (en) * 2000-05-04 2002-06-13 Biotika As A method for isolating salinomycin from fermentation broth
US7053115B2 (en) 2003-04-07 2006-05-30 Hetero Drugs Limited Crystalline form of dorzolamide hydrochloride

Also Published As

Publication number Publication date
JPS53148595A (en) 1978-12-25
DE2861764D1 (en) 1982-06-09
EP0000037B1 (en) 1982-04-28

Similar Documents

Publication Publication Date Title
Endoa et al. Isolation of 11-nortetrodotoxin-6 (R)-ol and other tetrodotoxin derivatives from the puffer Fugu niphobles
US4212942A (en) Method of producing salinomycin antibiotics
EP0000037A1 (en) Method of producing salinomycin type antibiotics and new salinomycin type antibiotics
EP0029309A1 (en) Substances having antibiotic activity, processes for their preparation, pharmaceutical compositions containing them, their use in medicaments and microorganisms
US2595159A (en) Preparation of vitamin b12 concentrates from streptomyces griseus cultures
US3832358A (en) Deshydroxymethyl derivatives of monensin
US4213966A (en) Method for isolating polyether antibiotics
US4399274A (en) Isolation of non-ionic lipophilic materials on macroreticular polymeric absorbents
DE2839668C2 (en)
JP2828343B2 (en) Precipitation method of natural avermectin
DE69009923T2 (en) Antifungal antibiotic and its manufacture and use.
US5045457A (en) Novel compounds
Della Greca et al. Biotransformation of progesterone by the green alga Chlorella emersonii C211-8H
EP0652205A2 (en) Moenomycin degradation products containing hydroxylated or oxidized lateral lipid chain and moenomycin analogs, process for preparing and their use
US3423398A (en) Sangivamycin and derivatives thereof
US3948726A (en) Production of cephalosporin C
US5047338A (en) Polyester Antibiotic preparation
DE3407979C2 (en)
US4657859A (en) Process for the treatment of fermentation broth containing vitamin B12 and other corrinoids and for the preparation of vitamin B12 concentrates
CH640269A5 (en) Method for producing the antibiotic c-15003 p. 4
JPH03141290A (en) Antitumor antibiotic bmy-41339
US2916483A (en) Methymycin
US4753959A (en) Antibiotic lactone compound
US3950516A (en) Process for preparing cirramycin A1
GB1159290A (en) Fermentation process for 9-(beta-D-Arabinofuranosyl) Adenine

Legal Events

Date Code Title Description
PUAI Public reference made under article 153(3) epc to a published international application that has entered the european phase

Free format text: ORIGINAL CODE: 0009012

AK Designated contracting states

Kind code of ref document: A1

Designated state(s): DE FR GB

Designated state(s): DE FR GB

17P Request for examination filed
GRAA (expected) grant

Free format text: ORIGINAL CODE: 0009210

AK Designated contracting states

Kind code of ref document: B1

Designated state(s): DE FR GB

Designated state(s): DE FR GB

REF Corresponds to:

Ref document number: 2861764

Country of ref document: DE

Date of ref document: 19820609

REG Reference to a national code

Ref country code: FR

Ref legal event code: CD

REG Reference to a national code

Ref country code: GB

Ref legal event code: 727

REG Reference to a national code

Ref country code: GB

Ref legal event code: 727A

REG Reference to a national code

Ref country code: GB

Ref legal event code: 727B

REG Reference to a national code

Ref country code: GB

Ref legal event code: SP

PGFP Annual fee paid to national office [announced via postgrant information from national office to epo]

Ref country code: GB

Payment date: 19970523

Year of fee payment: 20

PGFP Annual fee paid to national office [announced via postgrant information from national office to epo]

Ref country code: FR

Payment date: 19970610

Year of fee payment: 20

PGFP Annual fee paid to national office [announced via postgrant information from national office to epo]

Ref country code: DE

Payment date: 19970725

Year of fee payment: 20

PG25 Lapsed in a contracting state [announced via postgrant information from national office to epo]

Ref country code: GB

Free format text: LAPSE BECAUSE OF EXPIRATION OF PROTECTION

Effective date: 19980531

REG Reference to a national code

Ref country code: GB

Ref legal event code: PE20

Effective date: 19980531

PLBE No opposition filed within time limit

Free format text: ORIGINAL CODE: 0009261

STAA Information on the status of an ep patent application or granted ep patent

Free format text: STATUS: NO OPPOSITION FILED WITHIN TIME LIMIT