JP2993767B2 - FO-1289A substance and method for producing the same - Google Patents

FO-1289A substance and method for producing the same

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Publication number
JP2993767B2
JP2993767B2 JP3162183A JP16218391A JP2993767B2 JP 2993767 B2 JP2993767 B2 JP 2993767B2 JP 3162183 A JP3162183 A JP 3162183A JP 16218391 A JP16218391 A JP 16218391A JP 2993767 B2 JP2993767 B2 JP 2993767B2
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JP
Japan
Prior art keywords
substance
culture
producing
aspergillus
belonging
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JP3162183A
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JPH04360895A (en
Inventor
智 大村
洋 供田
博之 西田
碌郎 増間
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Kitasato Institute
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Kitasato Institute
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  • Preparation Of Compounds By Using Micro-Organisms (AREA)
  • Micro-Organisms Or Cultivation Processes Thereof (AREA)
  • Medicines Containing Material From Animals Or Micro-Organisms (AREA)
  • Compounds Of Unknown Constitution (AREA)

Description

【発明の詳細な説明】DETAILED DESCRIPTION OF THE INVENTION

【0001】[0001]

【産業上の利用分野】本発明は、アシルコエンザイムA
コレステロールアシル転位酵素阻害を有する新規物質F
O−1289A物質およびその製造法に関する。The present invention relates to an acyl coenzyme A
Novel substance F having cholesterol acyltransferase inhibition
The present invention relates to an O-1289A substance and a method for producing the same.

【0002】[0002]

【従来の技術】従来、いくつかの高脂血症薬物が知られ
ていたが、未だに有効な物質は得られていない。2. Description of the Related Art Conventionally, several hyperlipidemic drugs have been known, but no effective substance has been obtained yet.

【0003】[0003]

【発明が解決しようとする課題】近年、食生活の向上に
伴い成人の高脂血症や動脈硬化などコレステロール蓄積
に起因する症状が現代病として問題視されている。コレ
ステロールはアシルコエンザイムAからアシル基転位に
よりコレステロールエステルとなり、細胞内および血中
リポ蛋白に蓄積される。このアシル基転位反応を触媒す
る酵素がアシルコエンザイムAコレステロールアシル転
位酵素であり、コレステロールの腸管からの吸収および
冠動脈における泡沫細胞の形成に深く係わっている。し
たがって、アシルコエンザイムAコレステロールアシル
転位酵素を阻害する物質は、かかる疾病に有効であるこ
とが推察される。In recent years, symptoms caused by cholesterol accumulation such as hyperlipidemia and arteriosclerosis in adults have been regarded as a modern disease with the improvement of dietary habits. Cholesterol is converted into a cholesterol ester by acyl group transfer from acyl coenzyme A, and is accumulated in lipoproteins in cells and blood. The enzyme that catalyzes the acyl transfer reaction is acyl coenzyme A cholesterol acyl transferase, which is closely involved in the absorption of cholesterol from the intestinal tract and the formation of foam cells in coronary arteries. Therefore, it is presumed that a substance that inhibits acyl coenzyme A cholesterol acyltransferase is effective for such diseases.

【0004】かかる実情において、アシルコエンザイム
Aコレステロールアシル転位酵素阻害活性を有する物質
を提供することは、高脂血症やそれに基く動脈硬化など
の成人病の治療上有用なことである。Under such circumstances, it is useful to provide a substance having acylcoenzyme A cholesterol acyltransferase inhibitory activity in the treatment of adult diseases such as hyperlipidemia and arteriosclerosis.

【0005】[0005]

【課題を解決するための手段】本発明者らは、微生物の
生産する代謝産物に付いて研究を続けた結果、新たな土
壌から分離したFO−1289菌株の培養物中にアシル
コエンザイムAコレステロールアシル転位酵素阻害活性
を有する物質が産生されることを見出した。次いで、該
培養物からアシルコエンザイムAコレステロールアシル
転位酵素阻害活性物質を分離、精製した結果、後記の理
化学的性質を有する物質は従来全く知られていないこと
から、本物質をFO−1289A物質と称することにし
た。本発明は、係る知見に基いて完成されたものであっ
て、分子式C3137NO10で表されるFO−1289A
物質を提供するものである。The present inventors have continued their research on metabolites produced by microorganisms and found that acyl coenzyme A cholesterol acyl was contained in a culture of FO-1289 strain isolated from fresh soil. It has been found that a substance having a translocation enzyme inhibitory activity is produced. Next, the substance having acylcoenzyme A cholesterol acyltransferase inhibitory activity was separated and purified from the culture, and as a result, no substance having the physicochemical properties described below has been known at all. Therefore, this substance is referred to as FO-1289A substance. It was to be. The present invention has been completed on the basis of the above findings, and is a FO-1289A represented by a molecular formula of C 31 H 37 NO 10.
To provide the substance.

【0006】更に、本発明は、アスペルギルス属に属
し、FO−1289A物質を生産する能力を有する微生
物を培地に培養して培養物にFO−1289A物質を蓄
積せしめ、該培養物からFO−1289A物質を採取す
ることを特徴とするFO−1289A物質の製造法を提
供するものである。Further, the present invention relates to a method of culturing a microorganism belonging to the genus Aspergillus and having the ability to produce a FO-1289A substance in a culture medium to accumulate the FO-1289A substance in a culture, and then producing the FO-1289A substance from the culture. And a method for producing a FO-1289A substance.

【0007】FO−1289A物質を生産する能力を有
する微生物(以下、FO−1289A物質生産菌と称す
る)は、アスペルギルス属に属するが、例えば本発明者
らが分離したアスペルギルス属に属するFO−1289
菌株は、本発明の最も有効に使用される菌株の一例であ
って、本菌株の菌学的性状を示すと次の通りである。[0007] Microorganisms capable of producing the FO-1289A substance (hereinafter referred to as FO-1289A substance-producing bacteria) belong to the genus Aspergillus, and for example, FO-1289 belonging to the genus Aspergillus isolated by the present inventors.
The strain is an example of the most effectively used strain of the present invention, and the microbiological properties of the strain are as follows.

【0008】本発明のFO−1289A物質を生産する
ために使用される菌株としては、例えば本発明者らによ
つて土壌から分離されたアスペルギルス エスピー.
Aspergillus sp.)FO−1289株
が挙げられる。The strain used for producing the FO-1289A substance of the present invention includes, for example, Aspergillus sp. Isolated from the soil by the present inventors.
( Aspergillus sp.) FO-1289 strain.

【0009】I.本菌株は、マルトエキストラクト寒天
培地、ツアペツク・イーストエキストラクト寒天培地、
20%シユークロース・ツアペツク・イーストエキスト
ラクト寒天培地で良好に生育し、分生子の着生も良好で
ある。ツアペツク・イーストエキストラクト寒天培地に
生育したコロニーを顕微鏡で観察すると、菌糸は透明で
隔壁を有しており、分生子柄は主に基底菌糸より直生
し、その表面は滑面である。I. This strain is a malt extract agar medium, Tupetsk yeast extract agar medium,
It grows well on a 20% sucrose-tupetsk-yeast extract agar medium and has good conidium formation. When the colonies grown on the Tupetsk yeast extract agar medium are observed with a microscope, the hyphae are transparent and have partition walls, the conidiophores mainly grow straight from the basal hyphae, and the surface is smooth.

【0010】分生子柄の先端は、ふくらみ、フラスコ形
の頂のう(直径10−25μm)を形成する。メトレは
形成されず、フイアライドは頂のう上に直生する。分生
子は直径2〜3μmで、その形は球形、亜球形である。The tips of the conidiophores bulge, forming a flask-shaped apex (10-25 μm in diameter). No metres are formed, and the fluoride grows directly on the top. Conidia are 2-3 μm in diameter and are spherical and subspherical.

【0011】II.培養上の諸性状 (1)表1に本菌株の培養所見を示す。本所見は各種培
地上で25℃、7日間培養した場合の肉眼的に観察した
結果である。II. Characteristics of culture (1) Table 1 shows the culture findings of this strain. This finding is the result of macroscopic observation when cultured on various media at 25 ° C. for 7 days.

【0012】[0012]

【表1】 [Table 1]

【0013】(2)ツアペツク・イーストエキストラク
ト寒天培地における37℃、7日間培養した場合の生育
状態は、非常に旺盛(80mm以上)である。一方、5
℃、7日間培養した場合、生育しなかった。前記のすべ
ての培地には、菌の生育に伴う分泌液および菌核の形成
は観察されなかった。(2) The growth state when cultured at 37 ° C. for 7 days on a Tupetsk yeast extract agar medium is very vigorous (80 mm or more). 5
When the cells were cultured at 7 ° C. for 7 days, they did not grow. No formation of secretions and sclerotium was observed in all of the above-mentioned media as the bacteria grew.

【0014】III.生理学的性状 (1)生育温度範囲:15℃〜47℃、至適生育温度範
囲27℃〜40℃ (2)生育pH範囲:3〜11、至適生育pH範囲5〜
8 (3)好気性、嫌気性の区別:好気性III. Physiological properties (1) Growth temperature range: 15 ° C to 47 ° C, optimal growth temperature range 27 ° C to 40 ° C (2) Growth pH range: 3 to 11, optimal growth pH range 5 to 5
8 (3) Aerobic and anaerobic distinction: aerobic

【0015】上記FO−1289株の形態的特徴、培養
上の諸性状、生理学的性状に基づき、既知菌種との比較
を試みた結果、本菌株をアスペルギルス(Asperg
illus)属に属する一菌株と同定し、アスペルギル
ス エスピー.FO−1289と命名した。本菌株は、
アスペルギルス エスピー.FO−1289(Aspe
rgillus sp.FO−1289)として工業技
術院微生物工業技術研究所に寄託されている。(FER
M P−12194号)。[0015] Based on the morphological characteristics, culture characteristics, and physiological characteristics of the FO-1289 strain, an attempt was made to compare it with known bacterial strains. As a result, this strain was identified as Aspergillus ( Asperg).
illus ), identified as one strain belonging to the genus Aspergillus sp. FO-1289. This strain is
Aspergillus sp. FO-1289 ( Aspe
rgillus sp. FO-1289). (FER
MP-12194).

【0016】以上、FO−1289A生産菌について説
明したが、菌の一般的性状として菌学上の性状はきわめ
て変異し易く、一定したものではなく、自然的にあるい
は通常行われる紫外線照射または変異誘導体、例えばN
−メチル−N−ニトロ−N−ニトロソグアニジン、エチ
ルメタンスルホネートなどを用いる人工的変異手段によ
り変異することは周知の事実であり、このような人工的
変異株は勿論、自然変異株も含め、アスペルギルス属に
属し、FO−1289A物質を生産する能力を有する菌
株は、すべて本発明に使用することができる。また、細
胞融合、遺伝子操作などの細胞工学的に変異させた菌株
も物質FO−1289A物質生産菌として包含される。The FO-1289A producing bacteria have been described above. However, as a general property of the bacteria, the mycological properties are extremely liable to vary, are not constant, and are naturally or normally performed by ultraviolet irradiation or mutated derivatives. , For example N
-Methyl-N-nitro-N-nitrosoguanidine, ethyl methanesulfonate, etc., it is a well-known fact that mutation occurs by artificial mutation means. Any strain belonging to the genus and capable of producing the FO-1289A substance can be used in the present invention. In addition, strains mutated by cell engineering such as cell fusion and genetic manipulation are also included as substance FO-1289A substance-producing bacteria.

【0017】本発明においては、先ずアスペルギルス属
に属するFO−1289A物質生産菌が培地に培養され
る。本菌の培養においては、通常真菌の培養法が一般に
用いられる。培地としては、微生物が同化し得る炭素
源、資化し得る窒素源、さらには必要に応じて無機酸塩
などを含有させた栄養培地が使用される。同化し得る炭
素源としては、ブドウ糖、ショ糖、糖密、デキストリ
ン、セルロースなどが単独または組み合わせて用いられ
れる。In the present invention, a FO-1289A substance-producing bacterium belonging to the genus Aspergillus is first cultured in a medium. In culturing the fungus, a fungal culture method is generally used. As the medium, a nutrient medium containing a carbon source that can be assimilated by microorganisms, a nitrogen source that can be assimilated, and, if necessary, an inorganic acid salt or the like is used. As the assimilable carbon source, glucose, sucrose, molasses, dextrin, cellulose and the like are used alone or in combination.

【0018】資化し得る窒素源としては、ペプトン、肉
エキス、酵母エキス、乾燥酵母、大豆粉、コーン・ステ
イープ・リカー、綿実粕、カゼイン、大豆蛋白加水分解
物、アミノ酸、尿素などの有機窒素源、硝酸塩、アンモ
ニウム塩などの無機窒素化合物が単独または組み合わせ
て用いられる。その他、必要に応じてナトリウム塩、カ
リウム塩、カルシウム塩、マグネシウム塩、リン酸塩な
どの無機塩、重金属塩類が添加される。さらに、培地に
は、必要に応じて、本菌の生育やFO−1289A物質
の生産を促進する微量栄養素、発育促進物質、前駆物質
などを適当に添加してもよい。Examples of nitrogen sources that can be assimilated include organic nitrogen such as peptone, meat extract, yeast extract, dried yeast, soy flour, corn steep liquor, cottonseed meal, casein, soybean protein hydrolyzate, amino acids, and urea. Sources, inorganic nitrogen compounds such as nitrates and ammonium salts are used alone or in combination. In addition, if necessary, inorganic salts such as sodium salt, potassium salt, calcium salt, magnesium salt and phosphate, and heavy metal salts are added. Furthermore, if necessary, micronutrients, growth promoting substances, precursors, and the like that promote the growth of the present bacterium and the production of the FO-1289A substance may be appropriately added to the medium.

【0019】培養は通常振とうまたは通気攪拌培養など
の好気的条件下で行うのがよい。工業的には深部通気攪
拌培養が好ましい。培養のpHは中性付近で培養を行う
のが好ましい。培養温度は20〜37℃で行い得るが、
通常は24〜30℃に保つのがよい。培養時間は、液体
の場合、通常2〜3日間培養を行うと、本FO−128
9A物質が蓄積されるので、培養中の蓄積量が最大に達
した時に、培養を終了すればよい。The culture is usually carried out under aerobic conditions such as shaking or aeration and stirring culture. Industrially, deep aeration stirring culture is preferred. The culture is preferably performed at a pH around neutrality. The cultivation temperature can be 20-37 ° C,
Usually, it is good to keep at 24 to 30 ° C. In the case of liquid, the FO-128 is usually cultured for 2 to 3 days.
Since the substance 9A is accumulated, the culture may be terminated when the accumulated amount during the culture reaches the maximum.

【0020】これらの培地組成、培地の液性、培養温
度、培養速度、通気量などの培養条件は使用する菌株の
種類や外部の条件などに応じて好ましい結果が得られる
ように適宜調節、選択されることはいうまでもない。液
体培養において、発泡があるときは、シリコン油、植物
油、界面活性剤などの消泡剤を適宜使用できる。The culture conditions such as the medium composition, the liquid properties of the medium, the culture temperature, the culture rate and the aeration rate are appropriately adjusted and selected so as to obtain preferable results according to the kind of the strain used and the external conditions. Needless to say. If there is foaming in the liquid culture, an antifoaming agent such as silicone oil, vegetable oil, or a surfactant can be used as appropriate.

【0021】このようにして得られた培養物に蓄積され
るFO−1289A物質は、菌体内および培養濾液中に
含有されるので、培養物を遠心分離して培養濾液と菌体
とに分離し、各々から本FO−1289A物質を採取す
るのが有利である。Since the FO-1289A substance accumulated in the culture thus obtained is contained in the cells and in the culture filtrate, the culture is centrifuged to separate the culture filtrate and the cells. , It is advantageous to collect the present FO-1289A material from each.

【0022】培養濾液からFO−1289A物質を採取
するには、先ず培養濾液を酢酸エチル、酢酸ブチル、ベ
ンゼンなどの非親水性有機溶媒で抽出し、抽出液を減圧
濃縮して粗製のFO−1289A物質が得られる。この
粗製物質はさらに脂溶性物質の精製に通常用いられる公
知の方法、例えばシリカゲル、アルミナなどの担体を用
いるカラムクロマトグラフイーにより各々FO−128
9A物質を分離精製することができる。To collect the FO-1289A substance from the culture filtrate, the culture filtrate is first extracted with a non-hydrophilic organic solvent such as ethyl acetate, butyl acetate, benzene, etc., and the extract is concentrated under reduced pressure to obtain crude FO-1289A. The substance is obtained. The crude substance is further purified by a known method usually used for purification of a fat-soluble substance, for example, FO-128 by column chromatography using a carrier such as silica gel or alumina.
9A substance can be separated and purified.

【0023】菌体からFO−1289A物質を採取する
には、菌体を含水アセトン、含水メタノールなどの含水
親水性有機溶媒で抽出し、得られた抽出液を減圧濃縮
し、その濃縮物を酢酸エチル、酢酸ブチル、ベンゼンな
どの非親水性有機溶媒で抽出し、得られた抽出液は、前
記の培養濾液から得た抽出液と合わせて分離精製する
か、あるいは前記同じ方法によりFO−1289A物質
を分離精製することができる。To collect the FO-1289A substance from the cells, the cells are extracted with a water-containing hydrophilic organic solvent such as water-containing acetone and water-containing methanol, and the obtained extract is concentrated under reduced pressure. The extract is extracted with a non-hydrophilic organic solvent such as ethyl, butyl acetate, benzene, etc., and the obtained extract is separated and purified in combination with the extract obtained from the culture filtrate, or the FO-1289A substance is obtained by the same method as described above. Can be separated and purified.

【0024】次に、本発明のF−1289A物質の理化
学的性状について述べる。 (1)分子式;C3137NO10(高分解能スペクトルで
m/z583が観察された) (2)分子量;583(マススペクトルよりm/z58
3(M+ )が観察された) (3)比旋光度;〔α〕22 D =+73.2(C=1、ク
ロロホルム) (4)紫外線吸収スペクトル(メタノール中);図1の
通り (5)赤外線吸収スペクトル(四塩化炭素中);図2の
通りNext, the physicochemical properties of the substance F-1289A of the present invention will be described. (1) molecular formula; C 31 H 37 NO 10 (m / z 583 was observed in the high-resolution spectrum) (2) molecular weight; 583 (m / z 58 from the mass spectrum)
((3) (M + ) was observed) (3) Specific rotation; [α] 22 D = +73.2 (C = 1, chloroform) (4) Ultraviolet absorption spectrum (in methanol); ) Infrared absorption spectrum (in carbon tetrachloride);

【0025】(6)溶媒に対する溶解性;メタノール、
エタノール、アセトニトリル、酢酸エチル、ベンゼンに
可溶、水に不溶 (7)塩基性、酸性、中性の区別;中性 (8)物質の色、形状;黄色粉末 (9)プロトン核磁気共鳴スペクトル(重クロロホルム
中);図3の通り。(6) Solubility in a solvent: methanol,
Soluble in ethanol, acetonitrile, ethyl acetate, benzene, insoluble in water (7) Distinguishing between basic, acidic and neutral; neutral (8) Color and shape of substance; yellow powder (9) Proton nuclear magnetic resonance spectrum ( In deuterated chloroform); as in FIG.

【0026】次に、本発明のFO−1289A物質の生
物学的性状について述べる。 (1)ラツト由来アシルコエンザイムAコレステロール
アシル転位酵素に対する阻害作用 アシルコエンザイムAコレステロールアシル転位酵素活
性に対する影響はラツト肝ミクロソーム画分より調整し
た粗酵素を用い300μM〔1−14C〕Oleoyl−
CoA;3mg/mlコレステロールを各々20μl (0.
02μCi);6.67μl 添加し、37℃で30分間
反応させ、総脂質をクロロホルム:メタノール(2:
1)混合液で抽出後、TLC(キーゼルゲルGF254
展開溶媒として石油エーテル:ジエチルエーテル:酢
酸、90:10:1)で各脂質を分離後、コレステロー
ルエステル画分をかきとり、液体シンチレーシヨンカウ
ンターでアシルコエンザイムAコレステロールアシル転
位酵素活性を測定した。本酵素活性を50%阻害する濃
度を算定した結果はFO−1289A物質で0.03μ
g/mlであつた。Next, the biological properties of the FO-1289A substance of the present invention will be described. (1) rats from acyl-coenzyme A influence on the inhibitory action acyl-coenzyme A cholesterol acyltransferase activity against cholesterol acyltransferase is used crude enzyme prepared from rat liver microsome fraction 300μM [1-14 C] Oleoyl-
CoA; 20 μl each of 3 mg / ml cholesterol (0.
02 μCi); 6.67 μl was added thereto, and reacted at 37 ° C. for 30 minutes.
1) After extraction with the mixture, TLC (Kieselgel GF 254 ,
After separating each lipid with petroleum ether: diethyl ether: acetic acid (90: 10: 1) as a developing solvent, the cholesterol ester fraction was scraped off, and acyl coenzyme A cholesterol acyltransferase activity was measured with a liquid scintillation counter. The result of calculating the concentration that inhibits the enzyme activity by 50% is 0.03 μm for the FO-1289A substance.
g / ml.

【0027】[0027]

【発明の効果】以上のように、本発明のFO−1289
A物質は、アシルコエンザイムAコレステロールアシル
転位酵素に対して著しい阻害活性を示すことから、ヒト
のコレステロール蓄積に起因する疾病の予防および治療
に有用である。As described above, the FO-1289 of the present invention has been described.
Substance A exhibits a remarkable inhibitory activity on acyl coenzyme A cholesterol acyltransferase and is therefore useful for prevention and treatment of diseases caused by cholesterol accumulation in humans.

【0028】次に、実施例を挙げて本発明を具体的に説
明する。Next, the present invention will be described specifically with reference to examples.

【実施例】500ml容三角フラスコにグルコース0.1
%、スターチ2.4%、ペプトン0.3%、肉エキス
0.3%、イーストエキストラクト0.5%、炭酸カル
シウム0.4%を含む培地(pH7.0に調整)100
mlを仕込み、綿栓後、蒸気滅菌し、寒天培地上に生育さ
せたアスペルギルス エスピー.FO−1289(FE
RM P−12194)を白金耳にて無菌的に接種し、
27℃で48時間振とう培養して種培養液を得た。[Example] 0.1 g of glucose was placed in a 500 ml Erlenmeyer flask.
100%, starch 2.4%, peptone 0.3%, meat extract 0.3%, yeast extract 0.5%, calcium carbonate 0.4% (adjusted to pH 7.0) 100
ml of Aspergillus sp., which had been cotton-plugged, steam-sterilized, and grown on an agar medium. FO-1289 (FE
RM P-12194) aseptically with a platinum loop.
A seed culture was obtained by shaking culture at 27 ° C. for 48 hours.

【0029】一方、50l ジヤーフアーメンター1基に
グルコース1.0%、トリプトン0.5%、酵母エキス
0.3%、マルトエキス0.3%、寒天0.1%(pH
6.0に調整)に仕込み、蒸気滅菌冷却後、種培養した
種培養液200mlを無菌的に移植し、攪拌速度250r
pm、通気量10l /分の培養条件下で27℃で72時
間、通気攪拌した。On the other hand, one 50 l jar armamenter contains 1.0% glucose, 0.5% tryptone, 0.3% yeast extract, 0.3% malt extract, 0.1% agar (pH
6.0), steam-sterilized and cooled, and then aseptically transplanted with 200 ml of a seed culture solution subjected to seed culture, and stirred at 250 rpm.
The mixture was stirred under aeration at 27 ° C. for 72 hours under culture conditions of 10 pm / min.

【0030】培養後、培養液30l を酢酸エチル18l
で抽出し、抽出液を減圧濃縮して粗製物を得た。この粗
製物をシリカゲル(250g、メルク社製、Art.9
385)のカラムにチヤージし、クロロホルム−メタノ
ール(99:1)で溶出するカラムクロマトグラフイー
を行った。各フラクシヨンは100mlづつ分画し、活性
成分を含むフラクシヨンを集め、減圧乾固して粗活性物
質1.5gを得た。After the cultivation, 30 l of the culture was added to 18 l of ethyl acetate.
And the extract was concentrated under reduced pressure to obtain a crude product. This crude product was silica gel (250 g, Merck, Art. 9).
385), and column chromatography was performed, eluting with chloroform-methanol (99: 1). Each fraction was fractionated in 100 ml portions, and the fractions containing the active ingredient were collected and dried under reduced pressure to obtain 1.5 g of a crude active substance.

【0031】これを5回に分けて高速液体クロマトグラ
フイーにより分離精製した。装置はトリロータV(日本
分光社製)を用い、カラムはYMC−Pack A−3
43(ODS系樹脂、山村化学研究所製)を用い、溶媒
系は、55%のアセトニトリル水を用い、検出はUV2
80nm、流速は8ml/分で行った。その結果、FO−
1289A物質50mgを単離した。This was separated and purified by high-performance liquid chromatography in five times. The device used was Trirotor V (manufactured by JASCO Corporation), and the column was YMC-Pack A-3.
43 (ODS resin, manufactured by Yamamura Chemical Laboratory), the solvent system was 55% acetonitrile water, and the detection was UV2.
At 80 nm, the flow rate was 8 ml / min. As a result, FO-
50 mg of 1289A substance was isolated.

【図面の簡単な説明】[Brief description of the drawings]

【図1】FO−1289A物質の紫外線吸収スペクトル
である。(メタノール溶液として測定)FIG. 1 is an ultraviolet absorption spectrum of a FO-1289A substance. (Measured as methanol solution)

【図2】FO−1289A物質の赤外線吸収スペクトル
である。(四塩化炭素溶液として測定)FIG. 2 is an infrared absorption spectrum of a FO-1289A substance. (Measured as carbon tetrachloride solution)

【図3】FO−1289A物質のプロトン核磁気共鳴ス
ペクトルである。(重クロロホルム溶液として測定)FIG. 3 is a proton nuclear magnetic resonance spectrum of the FO-1289A substance. (Measured as deuterated chloroform solution)

───────────────────────────────────────────────────── フロントページの続き (51)Int.Cl.6 識別記号 FI C12R 1:66) (58)調査した分野(Int.Cl.6,DB名) C07G 17/00 C12N 1/14 C12P 1/02 BIOSIS(DIALOG) WPI(DIALOG)──────────────────────────────────────────────────続 き Continuation of the front page (51) Int.Cl. 6 identification code FI C12R 1:66) (58) Investigated field (Int.Cl. 6 , DB name) C07G 17/00 C12N 1/14 C12P 1 / 02 BIOSIS (DIALOG) WPI (DIALOG)

Claims (5)

(57)【特許請求の範囲】(57) [Claims] 【請求項1】 次の理化学的性質を有するFO−128
9A物質。 (1)分子式;C3137NO10(高分解能スペクトルで
m/z583が観察された) (2)分子量;583(マススペクトルよりm/z58
3(M+ )が観察された) (3)比旋光度;〔α〕22 D =+73.2(C=1、ク
ロロホルム) (4)紫外線吸収スペクトル(メタノール中);図1の
通り (5)赤外線吸収スペクトル(四塩化炭素中);図2の
通り (6)溶媒に対する溶解性;メタノール、エタノール、
アセトニトリル、酢酸エチル、ベンゼンに可溶、水に不
溶 (7)塩基性、酸性、中性の区別;中性 (8)物質の色、形状;黄色粉末1. FO-128 having the following physicochemical properties:
9A substance. (1) molecular formula; C 31 H 37 NO 10 (m / z 583 was observed in the high-resolution spectrum) (2) molecular weight; 583 (m / z 58 from the mass spectrum)
((3) (M + ) was observed) (3) Specific rotation; [α] 22 D = +73.2 (C = 1, chloroform) (4) Ultraviolet absorption spectrum (in methanol); ) Infrared absorption spectrum (in carbon tetrachloride); as shown in FIG. 2 (6) Solubility in solvent; methanol, ethanol,
Soluble in acetonitrile, ethyl acetate, benzene, insoluble in water (7) Basic, acidic, neutral distinction; neutral (8) Color and shape of substance; yellow powder 【請求項2】 アスペルギルス属に属し、FO−128
9A物質を生産する能力を有する微生物を培地に培養し
て培養中にFO−1289A物質を蓄積せしめ、該培養
物からFO−1289A物質を採取することを特徴とす
るFO−1289A物質の製造法。2. FO-128 belonging to the genus Aspergillus
A method for producing a FO-1289A substance, comprising culturing a microorganism capable of producing a 9A substance in a medium, accumulating the FO-1289A substance in the culture, and collecting the FO-1289A substance from the culture. 【請求項3】 アスペルギルス属に属し、FO−128
9A物質を生産する能力を有する微生物がアスペルギル
ス エスピー.FO−1289(Aspergillu
sp.FO−1289 FERM P−1219
4)である請求項2記載の製造法。3. FO-128 belonging to the genus Aspergillus
A microorganism capable of producing the 9A substance is Aspergillus sp. FO-1289 ( Aspergillu)
s sp. FO-1289 FERM P-1219
3. The method according to claim 2, wherein the method is 4). 【請求項4】 アスペルギルス属に属し、FO−128
9A物質を生産する能力を有する微生物。4. FO-128 belonging to the genus Aspergillus
A microorganism capable of producing 9A substances. 【請求項5】 微生物がアスペルギルス エスピー.F
O−1289である請求項4記載の微生物。5. The method according to claim 5, wherein the microorganism is Aspergillus sp. F
The microorganism according to claim 4, which is O-1289.
JP3162183A 1991-06-06 1991-06-06 FO-1289A substance and method for producing the same Expired - Lifetime JP2993767B2 (en)

Priority Applications (1)

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JP2993767B2 true JP2993767B2 (en) 1999-12-27

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