JP2693536B2 - Process for producing (7R) -cyclopenta [d] pyrimidine derivative - Google Patents
Process for producing (7R) -cyclopenta [d] pyrimidine derivativeInfo
- Publication number
- JP2693536B2 JP2693536B2 JP32851588A JP32851588A JP2693536B2 JP 2693536 B2 JP2693536 B2 JP 2693536B2 JP 32851588 A JP32851588 A JP 32851588A JP 32851588 A JP32851588 A JP 32851588A JP 2693536 B2 JP2693536 B2 JP 2693536B2
- Authority
- JP
- Japan
- Prior art keywords
- cyclopenta
- pyrimidine
- culture
- dihydro
- cyanoanilino
- 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.)
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Description
【発明の詳細な説明】 (産業上の利用分野) 本発明は抗うつ作用および脳障害改善作用を有する
(7R)−4−(4−シアノアニリノ)−6,7−ジヒドロ
−7−ヒドロキシ−5H−シクロペンタ〔d〕ピリミジン
の新規な製法に関する。DETAILED DESCRIPTION OF THE INVENTION (Field of Industrial Application) The present invention has (7R) -4- (4-cyanoanilino) -6,7-dihydro-7-hydroxy-5H having antidepressant action and brain disorder improving action. A novel process for the production of cyclopenta [d] pyrimidine.
(従来の技術) 4−(4−シアノアニリノ)−6,7−ジヒドロ−7−
ヒドロキシ−5H−シクロペンタ〔d〕ピリミジンは抗う
つ作用および脳障害改善作用を有する化合物として知ら
れている(特開昭62−70号および同63−183532号公開公
報)。(Prior art) 4- (4-cyanoanilino) -6,7-dihydro-7-
Hydroxy-5H-cyclopenta [d] pyrimidine is known as a compound having an antidepressant action and a cerebral disorder improving action (JP-A-62-70 and JP-A-63-183532).
(発明が解決しようとする課題) 4−(4−シアノアニリノ)−6,7−ジヒドロ−7−
ヒドロキシ−5H−シクロペンタ〔d〕ピリミジンは特開
昭62−70号公開公報記載の方法により得ることができ
る。そして、その光学活性体は常法に従って光学分割す
ることにより得られる。しかしながら、その光学分割の
手法は十分に確立されていない。(Problems to be solved by the invention) 4- (4-cyanoanilino) -6,7-dihydro-7-
Hydroxy-5H-cyclopenta [d] pyrimidine can be obtained by the method described in JP-A-62-70. Then, the optically active substance is obtained by optical resolution according to a conventional method. However, the method of optical division is not well established.
本発明者らは、微生物を用いて4−(4−シアノアニ
リノ)−6,7−ジヒドロ−5H−シクロペンタ〔d〕ピリ
ミジンを不斉水酸化して(7R)−4−(4−シアノアニ
リノ)−6,7−ジヒドロ−7−ヒドロキシ−5H−シクロ
ペンタ〔d〕ピリミジンが得られることを見出して本発
明を完成した。The present inventors have asymmetrically hydroxylated 4- (4-cyanoanilino) -6,7-dihydro-5H-cyclopenta [d] pyrimidine using a microorganism to obtain (7R) -4- (4-cyanoanilino)-. The present invention has been completed by finding that 6,7-dihydro-7-hydroxy-5H-cyclopenta [d] pyrimidine can be obtained.
(課題を解決するための手段) 本発明は4−(4−シアノアニリノ)−6,7−ジヒド
ロ−5H−シクロペンタ〔d〕ピリミジンをカニンガメラ
属に属する微生物を用いて水酸化して、式 を有する(7R)−4−(4−シアノアニリノ)−6,7−
ジヒドロ−7−ヒドロキシ−5H−シクロペンタ〔d〕ピ
リミジンを製造する方法である。(Means for Solving the Problems) The present invention comprises hydroxylating 4- (4-cyanoanilino) -6,7-dihydro-5H-cyclopenta [d] pyrimidine using a microorganism belonging to the genus Caningamegra, Having (7R) -4- (4-cyanoanilino) -6,7-
This is a method for producing dihydro-7-hydroxy-5H-cyclopenta [d] pyrimidine.
本発明に使用されるカニンガメラ属に属する微生物と
しては、例えば カニンガメラ・エチヌラータ(Cunninghamellaechinu
lata)IFO 4443 同 IFO 4446 同 IFO 4447 が好適である。Examples of the microorganism belonging to the genus Cunninghamella used in the present invention include Cunninghamella echinu
lata) IFO 4443 The same IFO 4446 The same IFO 4447 is suitable.
本発明において好適に用いられる微生物は、公的な菌
保存機関(IFO)より入手可能である。Microorganisms preferably used in the present invention can be obtained from a public bacterial preservation organization (IFO).
なお、カビの諸性質は一定したものでなく、自然的、
人口的に容易に変化することは周知のとおりであり、本
発明で使用しうる菌株はカニンガメラ属に属し、4−
(4−シアノアニリノ)−6,7−ジヒドロ−5H−シクロ
ペンタ〔d〕ピリミジンを(7R)−4−(4−シアノア
ニリノ)−6,7−ジヒドロ−7−ヒドロキシ−5H−シク
ロペンタ〔d〕ピリミジンに変換しうる菌株すべてを包
含するものである。It should be noted that the properties of mold are not constant, they are natural,
It is well known that the population can easily be changed, and the strains usable in the present invention belong to the genus Kaningamela, 4-
(4-Cyananilino) -6,7-dihydro-5H-cyclopenta [d] pyrimidine to (7R) -4- (4-cyanoanilino) -6,7-dihydro-7-hydroxy-5H-cyclopenta [d] pyrimidine It includes all strains that can be converted.
本発明の方法を実施するに際して、水酸化する方法と
しては、変換菌をその生育に適した培養条件下で培養
し、(1)原料化合物を培地中に添加して接触させる方
法(2)変換菌を培養・集菌し、得られた変換菌菌体を
原料化合物と接触させる方法、および(3)変換菌菌体
から調製した無細胞抽出液を原料化合物と接触させる方
法などが採用される。In carrying out the method of the present invention, as a method of hydroxylating, a method of culturing a converting bacterium under a culture condition suitable for its growth, and (1) adding a starting compound to a medium and bringing them into contact (2) conversion A method of culturing and collecting bacteria and contacting the obtained converted bacterial cells with the starting compound, and (3) a method of contacting the cell-free extract prepared from the converted bacterial cells with the starting compound are used. .
変換菌の培養は、通常微生物が利用出来る栄養物を含
有する培地中で培養することにより行なわれる。栄養源
としては、一般の微生物の培養に使用される公知のもの
を使用することが出来る。Culture of the transformed bacteria is usually performed by culturing in a medium containing nutrients that can be used by the microorganism. As a nutrient source, a known nutrient used for culturing a general microorganism can be used.
たとえば、炭素源としては、グルコース、シュークロ
ース、マルトース、乳糖、澱粉、グリセリン、水飴、糖
蜜、大豆油等が使用される。また窒素源としては、大豆
粉、小麦はい芽、肉粉、魚粉、肉エキス、ペプトン、コ
ーンスティープリカー、乾燥酵母、硝酸アンモニウムな
どのアンモニウム塩等が使用される。その他、必要に応
じて、食塩、塩化カリウム、炭酸カルシウム、燐酸塩等
の無機塩のほか、菌の発育を助け、前記の水酸化能を有
する酵素の生産を促進する添加物等を適宜組み合わせて
使用することが出来る。For example, as a carbon source, glucose, sucrose, maltose, lactose, starch, glycerin, starch syrup, molasses, soybean oil and the like are used. Examples of the nitrogen source include soybean flour, wheat germ, meat flour, fishmeal, meat extract, peptone, corn steep liquor, dried yeast, and ammonium salts such as ammonium nitrate. In addition, if necessary, in addition to inorganic salts such as salt, potassium chloride, calcium carbonate, and phosphate, as well as additives and the like that assist the growth of bacteria and promote the production of the enzyme having the hydroxylation ability, etc. Can be used.
培養は好気的条件下で行なわれ、培養温度は20−28
℃、好適には24−27℃である。The culture is carried out under aerobic conditions, and the culture temperature is 20-28.
℃, preferably 24-27 ℃.
次に、(1)法は、原料化合物を添加して培養するこ
とにより行なわれる。添加の時期は、使用する変換菌の
至適培養条件、特に培養装置、培地組成、培養温度等に
より異なるが、変換菌の水酸化能が高まり始める時期が
よく、通常は変換菌の培養開始後1−5日経過した時点
が好ましい。原料化合物の添加量は、培地に対して0.01
−1.0%、好ましくは0.01−0.1%である。Next, the method (1) is carried out by adding the starting compound and culturing. The timing of the addition varies depending on the optimal culture conditions of the transformed bacteria used, especially the culture device, medium composition, culture temperature, etc. It is preferred that 1-5 days have elapsed. The amount of the raw material compound added is 0.01 to the medium.
-1.0%, preferably 0.01-0.1%.
原料化合物添加後の培養は、好気的条件下、上記の培
養温度で行なわれる。培養期間は、原料化合物の添加後
1−10日程度である。The cultivation after the addition of the starting compound is carried out at the above-mentioned culturing temperature under aerobic conditions. The culture period is about 1-10 days after the addition of the raw material compound.
(2)法は、上記(1)の方法により変換菌を少量の
原料化合物の存在下で培養し、変換菌の水酸化能が最大
となるまで培養することにより行なわれる。The method (2) is carried out by culturing the transformed bacterium in the presence of a small amount of the starting compound according to the above method (1) and culturing the transformed bacterium until the hydroxylation ability of the transformed bacterium is maximized.
すなわち、水酸化能は培地の種類、温度等によって異
なるが、通常は培養開始後2−3日で最大となるので、
この時点で培養を終了する。集菌は培養物を遠心分離、
濾過等の方法に付すことによって行なわれる。集菌され
た変換菌菌体は、通常、生理食塩水、緩衝液等で洗浄し
て使用するのが好ましい。このようにして得られた変換
菌菌体を原料化合物と接触させるには、通常は水性媒体
中、例えばpH5−9の燐酸緩衝液中で行なわれる。接触
による反応は、通常20−40℃、好適には25−35℃で行な
われる。原料化合物の濃度は、通常培地に対して0.01−
0.1%である。反応時間は、原料化合物の濃度、反応温
度等によるが、通常は1−5日位である。That is, the hydroxylation ability varies depending on the type of medium, temperature, etc., but usually becomes maximum 2-3 days after the start of culture.
At this point, the culture is terminated. Harvesting involves centrifuging the culture,
It is carried out by applying a method such as filtration. It is preferable that the collected transformed cells are usually washed with a physiological saline solution, a buffer solution or the like before use. The thus obtained transformed bacterial cells are brought into contact with the starting compound, usually in an aqueous medium, for example, in a phosphate buffer of pH 5-9. The reaction by contact is usually carried out at 20-40 ° C, preferably at 25-35 ° C. The concentration of the starting compound is usually 0.01-
0.1%. The reaction time depends on the concentration of the raw material compound, the reaction temperature, etc., but is usually about 1-5 days.
(3)法での無細胞抽出液は、上記の方法で得られた
変換菌菌体に物理的又は化学的手法を適用し、たとえ
ば、磨砕、超音波処理等によって菌体破砕物として、ま
たは有機溶媒、界面活性剤、酵素処理等によって菌体溶
解液として得られる。The cell-free extract obtained by the method (3) is obtained by applying a physical or chemical technique to the transformed bacterial cells obtained by the above method, for example, by grinding, sonication, etc. Alternatively, it can be obtained as a cell lysate by treatment with an organic solvent, a surfactant, an enzyme, or the like.
このようにして得られた無細胞抽出液を原料化合物と
接触させるには、上記の変換菌菌体と接触させる方法と
同様して行なわれる。The contact of the cell-free extract thus obtained with the starting compound is carried out in the same manner as the above-mentioned method of contacting the cells of the converting bacterium.
変換反応終了後、目的化合物は生成物から既知の方法
で採取、分離、精製することができる。たとえば、得ら
れた生成物を濾過し、得られた濾液を酢酸エチルのよう
な、水と混和しにくい有機溶媒で抽出し、抽出液から溶
媒を留去したのち、得られた粗目的化合物をシリカゲ
ル、アルミナ等を用いたカラムクロマトグラフィーに付
し、適切な溶離剤で溶出することによって分離、精製す
ることができる。After the completion of the conversion reaction, the target compound can be collected, separated and purified from the product by a known method. For example, the obtained product is filtered, and the obtained filtrate is extracted with an organic solvent that is hardly miscible with water, such as ethyl acetate, and after the solvent is distilled off from the extract, the obtained crude target compound is obtained. Separation and purification can be achieved by column chromatography using silica gel, alumina or the like and eluting with a suitable eluent.
本発明の光学活性体はラセミ体と同様に抗うつ作用お
よび脳障害改善作用を示す。The optically active substance of the present invention exhibits an antidepressant action and a cerebral disorder improving action similarly to the racemic form.
また、その投与形態および投与量は特開昭62−70号お
よび同63−183522号公開公報の記載に準じて使用され
る。The dosage form and dosage are used according to the disclosures of JP-A Nos. 62-70 and 63-183522.
(実施例) 次に実施例をあげて本発明を更に具体的に説明する
が、本発明はこれらに限定されるものではない。(Examples) Next, the present invention will be described more specifically with reference to Examples, but the present invention is not limited thereto.
実施例1 下記の組成のA培地20mlを含有する100ml容三角フラ
スコに表に示す微生物をそれぞれ植菌した。これを26
℃,200r.p.m.で2日間回転振とう培養した。培養開始2
日後に4−(4−シアノアニリノ)−6,7−ジヒドロ−5
H−シクロペンタ〔d〕ピリミジンの5%ジメチルスル
ホキシド溶液を0.1ml添加し、更に7日間、26℃、200r.
p.m.で培養した。培養終了後、培養液に80%メタノール
を4倍量加えて希釈した。次いで、希釈液を高速液体ク
ロマトグラフィー(カラム;ヤマムラ化学研究所製、YM
C−Pack A−312 ODS:溶出液;アセトニトリル−0.5%酢
酸アンモニウム(50:50):流速;1.0ml/分:検出波長;3
15nm)に付して原料化合物から4−(4−シアノアニリ
ノ)−6,7−ジヒドロ−7−ヒドロキシ−5H−シクロペ
ンタ〔d〕ピリミジン(ラセミ体)への変換率を求め
た。更に、(7R)−4−(4−シアノアニリノ)−6,7
−ジヒドロ−7−ヒドロキシ−5H−シクロペンタ〔d〕
ピリミジン((R)体)の光学純度は高速液体クロマト
グラフィー(カラム;ダイセル化学工業(株)製、CHIR
ALPAK WE:溶出液;アセトニトリル−0.25mM硫酸銅(90:
10):流速;0.5ml/分:検出波長;315nm)に付して、保
持時間が(S)体が20分、(R)体が26分で分離するこ
とにより、求めた。結果を表に示す。Example 1 Each of the microorganisms shown in the table was inoculated into a 100 ml Erlenmeyer flask containing 20 ml of the A medium having the following composition. 26 this
Culture was carried out at 200 ° C. and 200 rpm for 2 days with rotary shaking. Start of culture 2
Days later 4- (4-cyanoanilino) -6,7-dihydro-5
0.1 ml of 5% dimethylsulfoxide solution of H-cyclopenta [d] pyrimidine was added, and further 7 days, 26 ° C, 200r.
Cultured at pm. After completion of the culture, the culture solution was diluted by adding 4 times the volume of 80% methanol. Then, the diluted solution was subjected to high performance liquid chromatography (column; Yamamura Chemical Laboratory, YM
C-Pack A-312 ODS: eluent; acetonitrile-0.5% ammonium acetate (50:50): flow rate; 1.0 ml / min: detection wavelength; 3
The conversion rate from the starting compound to 4- (4-cyanoanilino) -6,7-dihydro-7-hydroxy-5H-cyclopenta [d] pyrimidine (racemic form) was determined. Furthermore, (7R) -4- (4-cyanoanilino) -6,7
-Dihydro-7-hydroxy-5H-cyclopenta [d]
The optical purity of pyrimidine ((R) form) was measured by high performance liquid chromatography (column; Daicel Chemical Industries, Ltd., CHIR
ALPAK WE: Eluent; acetonitrile-0.25 mM copper sulfate (90:
10): Flow rate; 0.5 ml / min: Detection wavelength; 315 nm), and the retention time was determined by separating the (S) form in 20 minutes and the (R) form in 26 minutes. The results are shown in the table.
A培地組成 グルコース 10g イーストエキス 3g マルツエキス 3g ポリペプトン 5g イオン交換水 1000ml pH無調整 実施例2 実施例1で用いたと同じA培地500mlを含有する2
容三角フラスコにカニンガメラ・エチヌラータIFO 4446
を植菌し、26℃で3日間210r.p.m.で回転振とう培養し
て種培養液を得た。次いで、A培地に消泡剤(CB 442)
0.01%を加えた培地300を含む600タンクに種培養液
1%を加えて、26℃で通気量0.5v.v.m.、100〜110r.p.
m.で培養した。培養開始2日後に4−(4−シアノアニ
リノ)−6,7−ジヒドロ−5H−シクロペンタ〔d〕ピリ
ミジンの5%ジメチルスルホキシド溶液を3添加し、
更に5日間、26℃、100〜110r.p.m.で培養した。培養終
了後、培養液をフィルタープレスに付し、得られたろ液
330を酢酸エチル150で3回抽出し、抽出液を500ml
まで濃縮した。析出した結晶をろ去し、得られたろ液に
酢酸エチルを加え、次いで水洗した。得られた混液から
酢酸エチルを減圧下で留去し、析出する結晶をn−ヘキ
サン−トルエンで洗浄し、更に得られた結晶をシリカゲ
ルを用いたカラムクロマトグラフィー〔溶出液;酢酸エ
チル−メタノール(40:1)〕に付して精製すると(7R)
−4−(4−シアノアニリノ)−6,7−ジヒドロ−7−
ヒドロキシ−5H−シクロペンタ〔d〕ピリミジンの純品
2.91gが得られた。A medium composition Glucose 10g Yeast extract 3g Malt extract 3g Polypeptone 5g Ion-exchanged water 1000ml pH unadjusted Example 2 2 containing 500 ml of the same A medium as used in Example 1
Kaningamera Echinurata IFO 4446 in a conical Erlenmeyer flask
Was cultivated and cultured at 210 rpm for 3 days at 210 rpm to obtain a seed culture solution. Next, defoamer (CB 442) on medium A
1% of the seed culture solution was added to a 600 tank containing 300 medium containing 0.01%, and the aeration rate was 0.5 vvm at 26 ° C and 100 to 110 r.p.
Cultured at m. Two days after the start of the culture, 5% dimethyl sulfoxide solution of 4- (4-cyanoanilino) -6,7-dihydro-5H-cyclopenta [d] pyrimidine was added 3 times,
The cells were further cultured for 5 days at 26 ° C. and 100 to 110 rpm. After completion of the culture, the culture solution was applied to a filter press, and the obtained filtrate
330 is extracted 3 times with 150% ethyl acetate and 500 ml of extract
Concentrated. The precipitated crystals were removed by filtration, and ethyl acetate was added to the obtained filtrate, followed by washing with water. Ethyl acetate was distilled off from the obtained mixture under reduced pressure, the precipitated crystals were washed with n-hexane-toluene, and the obtained crystals were subjected to column chromatography using silica gel [eluent: ethyl acetate-methanol ( 40: 1)] and purified (7R)
-4- (4-cyanoanilino) -6,7-dihydro-7-
Pure product of hydroxy-5H-cyclopenta [d] pyrimidine
2.91 g were obtained.
1) 性状:白色結晶 2) 融点:213〜216℃ 3) 分子量:252.3 6) 質量分析スペクトル:(m/z) 252(M+),251(M+−H),223(251−C2H4),102 7) 1NMRスペクトル:δppm 重ジメチルスルホキシド中、内部基準にテトラメチル
シランを使用して測定した核磁気共鳴スペクトル(270M
Hz)は以下の通りである。1) Properties: White crystals 2) Melting point: 213-216 ° C 3) Molecular weight: 252.3 6) mass spectrum: (m / z) 252 ( M +), 251 (M + -H), 223 (251-C 2 H 4), 102 7) 1 NMR Spectrum: [delta] ppm heavy dimethylsulfoxide, internal standard Nuclear magnetic resonance spectrum (270M
Hz) is as follows.
1.8(1H,m),2.4(1H,m),2.7(1H,m)2.9(1H,m),
4.9(1H,d),5.5(1H,d),7.7(1H,d),8.0(2H,d),8.
6(1H,s),9.2(1H,s) 8) 比旋光度:▲〔α〕25 D▼−31.6゜(C=0.25,エ
タノール) 9) 光学純度:100%e.e.〔高速液体クロマトグラフィ
ー(カラム;ダイセル化学工業(株)製、CHIRALPAK W
E;溶出液;アセトニトリル−0.25mM硫酸銅(90:10):
流速;0.5ml/分;溶出波長;315nm:保持時間;26分〕1.8 (1H, m), 2.4 (1H, m), 2.7 (1H, m) 2.9 (1H, m),
4.9 (1H, d), 5.5 (1H, d), 7.7 (1H, d), 8.0 (2H, d), 8.
6 (1H, s), 9.2 (1H, s) 8) Specific rotation: ▲ [α] 25 D ▼ -31.6 ° (C = 0.25, ethanol) 9) Optical purity: 100% ee [High performance liquid chromatography ( Column: Daicel Chemical Industries, Ltd., CHIRALPAK W
E; Eluate; acetonitrile-0.25 mM copper sulfate (90:10):
Flow rate; 0.5 ml / min; elution wavelength; 315 nm: retention time; 26 minutes]
───────────────────────────────────────────────────── フロントページの続き (72)発明者 加賀崎 武之 福島県いわき市泉町下川字大剱389―4 三共株式会社内 (72)発明者 古林 隆司 山口県宇部市大字小串1978番地の5 宇 部興産株式会社宇部研究所内 ─────────────────────────────────────────────────── ─── Continuation of the front page (72) Takeyuki Kagasaki, 389-4 Ogura, Shimokawa, Izumi-cho, Iwaki-shi, Fukushima Sankyo Co., Ltd. (72) Ryuji Kobayashi, Ube, Yamaguchi Prefecture Usan Laboratory, Kosan Co., Ltd.
Claims (1)
ドロ−5H−シクロペンタ〔d〕ピリミジンをカニンガメ
ラ属に属する微生物を用いて水酸化して、式 を有する(7R)−4−(4−シアノアニリノ)−6,7−
ジヒドロ−7−ヒドロキシ−5H−シクロペンタ〔d〕ピ
リミジンに変換せしめ、変換反応物を含む系より前記式
を有する化合物を採取することからなる前記式を有する
化合物の製造法。1. A method of hydroxylating 4- (4-cyanoanilino) -6,7-dihydro-5H-cyclopenta [d] pyrimidine using a microorganism belonging to the genus Kaningamela, Having (7R) -4- (4-cyanoanilino) -6,7-
A process for producing a compound having the above formula, which comprises converting to dihydro-7-hydroxy-5H-cyclopenta [d] pyrimidine and collecting the compound having the above formula from the system containing the conversion reaction product.
Priority Applications (1)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| JP32851588A JP2693536B2 (en) | 1988-12-26 | 1988-12-26 | Process for producing (7R) -cyclopenta [d] pyrimidine derivative |
Applications Claiming Priority (1)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| JP32851588A JP2693536B2 (en) | 1988-12-26 | 1988-12-26 | Process for producing (7R) -cyclopenta [d] pyrimidine derivative |
Publications (2)
| Publication Number | Publication Date |
|---|---|
| JPH02174687A JPH02174687A (en) | 1990-07-06 |
| JP2693536B2 true JP2693536B2 (en) | 1997-12-24 |
Family
ID=18211139
Family Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| JP32851588A Expired - Fee Related JP2693536B2 (en) | 1988-12-26 | 1988-12-26 | Process for producing (7R) -cyclopenta [d] pyrimidine derivative |
Country Status (1)
| Country | Link |
|---|---|
| JP (1) | JP2693536B2 (en) |
-
1988
- 1988-12-26 JP JP32851588A patent/JP2693536B2/en not_active Expired - Fee Related
Also Published As
| Publication number | Publication date |
|---|---|
| JPH02174687A (en) | 1990-07-06 |
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