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JPS6312292A - Production of l-lysine - Google Patents

Production of l-lysine

Info

Publication number
JPS6312292A
JPS6312292A JP15677586A JP15677586A JPS6312292A JP S6312292 A JPS6312292 A JP S6312292A JP 15677586 A JP15677586 A JP 15677586A JP 15677586 A JP15677586 A JP 15677586A JP S6312292 A JPS6312292 A JP S6312292A
Authority
JP
Japan
Prior art keywords
lysine
producing
naphthoquinoline
strain
present
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
JP15677586A
Other languages
Japanese (ja)
Other versions
JPH0555114B2 (en
Inventor
Hideaki Yonekura
米倉 秀昭
Toshihiko Hirao
平尾 俊彦
Tomoki Azuma
東 朋樹
Toshihide Nakanishi
中西 俊秀
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.)
KH Neochem Co Ltd
Original Assignee
Kyowa Hakko Kogyo 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 Kyowa Hakko Kogyo Co Ltd filed Critical Kyowa Hakko Kogyo Co Ltd
Priority to JP15677586A priority Critical patent/JPS6312292A/en
Priority to MX711587A priority patent/MX168303B/en
Priority to FR8709309A priority patent/FR2601035B1/en
Priority to CN 87104553 priority patent/CN1022931C/en
Priority to HU300487A priority patent/HU200797B/en
Priority to AU75059/87A priority patent/AU597387B2/en
Publication of JPS6312292A publication Critical patent/JPS6312292A/en
Publication of JPH0555114B2 publication Critical patent/JPH0555114B2/ja
Granted legal-status Critical Current

Links

Classifications

    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12PFERMENTATION OR ENZYME-USING PROCESSES TO SYNTHESISE A DESIRED CHEMICAL COMPOUND OR COMPOSITION OR TO SEPARATE OPTICAL ISOMERS FROM A RACEMIC MIXTURE
    • C12P13/00Preparation of nitrogen-containing organic compounds
    • C12P13/04Alpha- or beta- amino acids
    • C12P13/08Lysine; Diaminopimelic acid; Threonine; Valine

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  • Organic Chemistry (AREA)
  • Chemical & Material Sciences (AREA)
  • Engineering & Computer Science (AREA)
  • Zoology (AREA)
  • Life Sciences & Earth Sciences (AREA)
  • Wood Science & Technology (AREA)
  • Chemical Kinetics & Catalysis (AREA)
  • Microbiology (AREA)
  • General Chemical & Material Sciences (AREA)
  • Biotechnology (AREA)
  • Health & Medical Sciences (AREA)
  • Biochemistry (AREA)
  • Bioinformatics & Cheminformatics (AREA)
  • General Engineering & Computer Science (AREA)
  • General Health & Medical Sciences (AREA)
  • Genetics & Genomics (AREA)
  • Preparation Of Compounds By Using Micro-Organisms (AREA)
  • Micro-Organisms Or Cultivation Processes Thereof (AREA)

Abstract

PURPOSE:To produce the titled compound useful as a food additive, etc., on an industrial scale at a low cost, by culturing a microbial strain belonging to glutamic acid-producing coryne-form strain resistant to beta-naphthoquinoline and capable of producing L-lysine in a medium and separating the product from the cultured liquid. CONSTITUTION:A microbial strain belonging to glutamic acid-producing coryne- form strain resistant to beta-naphthoquinoline and capable of producing L-lysine [e.g. Corynebacterium glutamicum H-4412 (FERM BP-1069), etc.] is cultured in a medium containing glucose, etc., as carbon source, urea, etc., as nitrogen source and potassium phosphate, etc., as inorganic component. The produced and accumulated L-lysine is separated from the cultured liquid.

Description

【発明の詳細な説明】 産業上の利用分野 本発明は発酵法によるL−リジンの製造法に関する。さ
らに詳しくは、本発明はコリネ型グルタミン酸生産菌に
属し、β−ナフトキノリンに抵抗性を有し、かつL−リ
ジン生産能を有する微生物を培地に培養して、該培養物
からL−リジンを採取することを特徴とする発酵法によ
るL−リジンの製造法に関する。DETAILED DESCRIPTION OF THE INVENTION Field of the Invention The present invention relates to a method for producing L-lysine by fermentation. More specifically, the present invention involves culturing in a medium a microorganism that belongs to coryneform glutamate-producing bacteria, is resistant to β-naphthoquinoline, and has the ability to produce L-lysine, and L-lysine is collected from the culture. The present invention relates to a method for producing L-lysine by a fermentation method, characterized in that:

その目的とするところは必須アミノ酸の1つであり、医
薬品あるいは飼料や食品への添加剤として需要の大きい
L−IJリジン工業的に安価に製造する方法を提供する
ことにある。The purpose is to provide a method for industrially producing L-IJ lysine, which is one of the essential amino acids and is in high demand as an additive to pharmaceuticals, feeds, and foods.

従来の技術 従来、発酵法によるL−リジンの製造法に関してはコリ
ネバクテリウム属、ブレビバクテリウム属、アースロバ
フタ−属、バチルス属の細菌やその他の微生物のホモセ
リン(またはメチオニンとスレオニン)要求性変異株(
特公昭36−6499号、 USP2,979.439
)やその他要求性変異株〔特公昭48−28677号、
同51−21078号、同51−34477号(LIS
P3,825.472)。Conventional technology Conventionally, regarding the production of L-lysine by fermentation, homoserine (or methionine and threonine) auxotrophic mutant strains of bacteria of the genera Corynebacterium, Brevibacterium, Arthrobacterium, Bacillus and other microorganisms have been used. (
Special Publication No. 36-6499, USP 2,979.439
) and other auxotrophic mutants [Special Publication No. 48-28677,
No. 51-21078, No. 51-34477 (LIS
P3,825.472).

同55−1040号、特開昭56−8692号。No. 55-1040, JP-A No. 56-8692.

同55−9784号〕を用いる方法、また各種薬剤抵抗
性変異株〔特公昭48−28078号(USP3.70
7.441 ) 、同53−1833号。No. 55-9784], and various drug-resistant mutant strains [Special Publication No. 48-28078 (USP 3.70)].
7.441), No. 53-1833.

同53−43591号、同59−4993号、特開昭5
3−9394号、同55−9785号(USP3,68
7.810 ) :1などを用いる方法、あるいはこれ
らの組合せの性質を有する微生物を用いる方法などが知
られている。No. 53-43591, No. 59-4993, JP-A-5
No. 3-9394, No. 55-9785 (USP 3,68
7.810):1, and methods using microorganisms having a combination of these properties are known.

発明が解決しようとする問題点 必須アミノ酸の1つであり、医薬品あるいは飼料や食品
への添加剤として需要の大きいL−’Jリジン、工業的
に安価に製造する方法の開発は常に望まれている。Problems to be Solved by the Invention L-'J lysine is one of the essential amino acids and is in great demand as an additive for pharmaceuticals, feed, and food, and it has always been desired to develop a method to produce it industrially at low cost. There is.

問題点を解決するための手段 本発明者は、L−リジンの生産性の改良された菌株を得
るため種々研究を重ねた結果、コリネ型グルタミン酸生
産菌に属するL−IJリジン産菌株にさらにβ−ナフト
キノリン抵抗性を付与すると、L−リジン生産性が飛躍
的に向上することを見出し、本発明を完成するに至った
。発酵法によるL−リジンの製造に際し、キノリン類に
対する耐性を付与することによってリジン生産能が向上
することが知られている(特公昭59−4993号)が
、これらの薬剤による生育阻害はL−ロイシンで解除さ
れることが示されている。従って、これらのキノリン類
は、L−ロイシンアナログとして作用していることが推
定される。しかし、β−ナフトキノリンによる生育阻害
は、L−ロイシンで回復されないことから、β−ナフト
キノリンは特公昭59−4993号におけるキノリン類
とは別の範鴫に属する物質であると考えられる。このよ
うな性質をもったβ−ナフトキノリンに抵抗性を有する
菌株を用いればl、−+Jリジン生産性が飛躍的に改善
されることは本発明者によってはじめて見出された知見
である。Means for Solving the Problems As a result of various studies to obtain a strain with improved productivity of L-lysine, the present inventor has further added β to the L-IJ lysine-producing strain belonging to coryneform glutamic acid-producing bacteria. - It was discovered that L-lysine productivity was dramatically improved by imparting naphthoquinoline resistance, and the present invention was completed. When producing L-lysine by fermentation, it is known that lysine production ability is improved by imparting resistance to quinolines (Japanese Patent Publication No. 4993/1983); however, growth inhibition by these drugs is It has been shown to be released by leucine. Therefore, it is presumed that these quinolines act as L-leucine analogs. However, since the growth inhibition caused by β-naphthoquinoline is not recovered by L-leucine, β-naphthoquinoline is considered to be a substance belonging to a different category from the quinolines described in Japanese Patent Publication No. 59-4993. It was discovered for the first time by the present inventors that l,-+J lysine productivity can be dramatically improved by using a bacterial strain that is resistant to β-naphthoquinoline and has such properties.

以下、本発明の詳細な説明する。The present invention will be explained in detail below.

本発明は、コリネ型グルタミン酸生産菌に属し、β−ナ
フトキノリンに抵抗性を有し、かつL−リジン生産能を
有する微生物を培地に培養し、培養物中にL IJリジ
ン生成蓄積させ、該培養物からL−リジンを採取するこ
とを特徴とするL−リジンの製造法を提供する。The present invention involves culturing a microorganism belonging to coryneform glutamate-producing bacteria, having resistance to β-naphthoquinoline, and having L-lysine producing ability in a medium, producing and accumulating L-IJ lysine in the culture, and To provide a method for producing L-lysine, which is characterized by collecting L-lysine from a substance.

本明細書において、コリネ型グルタミン酸生産菌とは、
コリネバクテリウム属、ブレビバクテリウム属、ミクロ
バクテリウム属またはアースロバフタ−属に属する一群
のグルタミン酸生産菌をいう〔「発酵と工業」第40巻
、 102.1982年参照〕。As used herein, coryneform glutamate-producing bacteria are
A group of glutamic acid-producing bacteria belonging to the genus Corynebacterium, Brevibacterium, Microbacterium, or Arthrobacterium [see "Fermentation and Industry" Vol. 40, 102, 1982].

本発明で用いる微生物は、コリネ型グルタミン酸生産菌
に属し、β−ナフトキノリンに抵抗性を有するL−リジ
ン生産菌株であればいかなる菌株をも用いることができ
る。すなわち、本発明ではコリネ型グルタミン酸生産菌
に属し、L−リジン生産能を有する菌株にβ−ナフトキ
ノリン抵抗性を付与させた菌株を用いてもよいし、コリ
ネ型グルタミン酸生産菌に属し、β−ナフトキノリン抵
抗性を有する菌株にL−Uジン生産能を付与させた菌株
を用いてもよい。The microorganism used in the present invention belongs to coryneform glutamic acid-producing bacteria, and any L-lysine-producing strain that is resistant to β-naphthoquinoline can be used. That is, in the present invention, a strain that belongs to the coryneform glutamate-producing bacteria and has the ability to produce L-lysine may be imparted with β-naphthoquinoline resistance, or a strain that belongs to the coryneform glutamate-producing bacteria and has the ability to produce β-naphthoquinoline may be used. A strain obtained by imparting the ability to produce L-U gin to a resistant strain may also be used.

コリネ型グルタミン酸生産菌に属するL−リジン生産能
を有する菌株としては、各種の栄養(例えばホモセリン
、メチオニン、スレオニン、ヒスチジン、ブ(1リン、
アラニン、ロインン、イソL1イシン、バリン、セリン
、グルタミン酸、パントテン酸、ニコチン酸アミド、酢
酸、アデニン、ヒポキサンチン、イノシトールおよびこ
れらの組合せ)要求性、各種のアミノ酸アナログ(例え
ばリジン、スレオニン、メチオニン、ロイシン、インロ
イシン、バリン、アスパラギン酸、トリプトファンある
いはヒスチジンのアナログおよびこれらの組合せ)抵抗
性、その他薬剤(例えば各種抗生物質、サルファ剤、各
種有機酸、キノン化合物。Bacterial strains that belong to coryneform glutamate-producing bacteria and have the ability to produce L-lysine contain various nutrients (e.g., homoserine, methionine, threonine, histidine,
alanine, loinine, isoL1 isine, valine, serine, glutamic acid, pantothenic acid, nicotinamide, acetic acid, adenine, hypoxanthine, inositol and combinations thereof), various amino acid analogs (e.g. lysine, threonine, methionine, leucine) , inleucine, valine, aspartic acid, tryptophan or histidine analogs, and combinations thereof), and other drugs (e.g., various antibiotics, sulfa drugs, various organic acids, quinone compounds).

キノリン化合物およびこれらの組合せ)抵抗性の1つあ
るいはこれらの組合せの性質を有するL−リジン生産菌
株が挙げられる。quinoline compounds and combinations thereof) resistant to one or a combination thereof.

したがって、上記のようなし IJリジン産菌株に、さ
らにβ−ナフトキノリン抵抗性を付与することによって
本発明に使用する菌株を得ることもできるし、コリネ型
グルタミン酸生産菌に属し、β−ナフトキノリン抵抗性
を有する菌株に上記のような各種栄養要求性、各種アミ
ノ酸アナログ抵抗性、またはその他薬剤の抵抗性を付与
することによって得られるL−リジン生産菌株を本発明
で使用することもできる。また、本発明に用いる菌株は
上記のような性質の他にL−Uジン生産に寄与するいか
なる性質を備えていてもさしつかえない。Therefore, the strain used in the present invention can be obtained by further imparting β-naphthoquinoline resistance to the above-mentioned IJ lysine-producing strain, or it is possible to obtain the strain used in the present invention by further imparting β-naphthoquinoline resistance to the above-mentioned IJ lysine-producing strain. L-lysine-producing strains obtained by imparting various auxotrophic requirements, various amino acid analog resistances, or other drug resistances as described above to the L-lysine-producing strains can also be used in the present invention. In addition to the above-mentioned properties, the strain used in the present invention may have any properties that contribute to L-U gin production.

本発明の変異株を誘導する際に用いられる親株としては
、コリネ型グルタミン酸生産菌として知られている下記
微生物があげられる。例えば、コリネバクテリウム・グ
ルタミクムATCC13032゜コリネバクテリウム・
グルタミクムH−3149(FERM  BP−158
)、コリネバクテリウム・アセトアシドフィラムATC
C13870゜ブレビバクテリウム・ラクトフェルメン
タムATCC13869、ブレビバクテリウム・フラバ
ムATCC14067などがある。Parent strains used to induce the mutant strain of the present invention include the following microorganisms known as coryneform glutamate-producing bacteria. For example, Corynebacterium glutamicum ATCC13032゜Corynebacterium glutamicum
Glutamicum H-3149 (FERM BP-158
), Corynebacterium acetoacidophyllum ATC
C13870° Brevibacterium lactofermentum ATCC13869, Brevibacterium flavum ATCC14067, etc.

本発明における変異株の誘導は、紫外線照射やN−メチ
ル−N′−二トローN−二トロングアニジンなどによる
化学処理など、通常用いられる変異処理方法により行う
ことができる。Induction of mutant strains in the present invention can be carried out by commonly used mutation treatment methods such as ultraviolet irradiation and chemical treatment with N-methyl-N'-nitro-N-nitroguanidine.

変異処理した菌株から本発明の変異株を分離するには、
親株が生育阻害を示す濃度のβ−ナフトキノリン(40
u/m1以上)を含む最少培地寒天平板上に生育する変
異株を取得すればよい。To isolate the mutant strain of the present invention from the mutation-treated strain,
β-naphthoquinoline at a concentration that inhibits the growth of the parent strain (40
What is necessary is to obtain a mutant strain that grows on a minimal medium agar plate containing (u/ml or more).

本発明に使用する微生物のうち、β−ナフトキノリン抵
抗性菌株の具体的−例として、コリネバクテリウム・グ
ルタミクムH−4412の取得例を以下に示す。Among the microorganisms used in the present invention, an example of obtaining Corynebacterium glutamicum H-4412 is shown below as a specific example of a β-naphthoquinoline-resistant strain.

コリネバクテリウム・グルタミクムH−3149(FE
RM  BP−158)(チアリジン抵抗性。Corynebacterium glutamicum H-3149 (FE
RM BP-158) (thiarisin resistance.

リファンピシン抵抗性、ストレプトマイシン抵抗性、6
−アヂウラシル抵抗性)を親株として用いる。この親株
を0. I N ) !Jスス−レイン酸緩衝液(pH
6,0)中に10”細胞/mlの濃度に懸濁し、ここに
N−メチル−N′−二トローN−ニトロソグアニジンを
最終濃度062■/mlになるように添加し、室温で3
0分間静置する。親株が生育阻害を示す濃度のβ−ナフ
トキノリン(例えば40g/ml )を含む下記のよう
な組成を有する最少培地寒天平板上に塗抹し、生育する
コロニーの中から変異株を選択する。その1株がH−4
412であり、β−ナフトキノリン抵抗性を有する点で
第1表に示すように、親株のH−3149と明らかに区
別できる。Rifampicin resistance, streptomycin resistance, 6
-Adiuracil resistant) is used as the parent strain. This parent stock is 0. IN)! J Sous-leate buffer (pH
N-methyl-N'-nitro N-nitrosoguanidine was added to the suspension at a final concentration of 0.62 cm/ml, and the suspension was incubated at room temperature for 3.
Let stand for 0 minutes. The mutant strain is selected from the growing colonies by spreading it onto a minimal medium agar plate having the composition shown below, which contains β-naphthoquinoline (for example, 40 g/ml) at a concentration that inhibits the growth of the parent strain. One of them is H-4
412, and as shown in Table 1, it can be clearly distinguished from the parent strain H-3149 in that it has β-naphthoquinoline resistance.

最少培地寒天平板培地組成ニ ゲルコース10g/l、NH1Cj!  Ig/j!。Minimal medium agar plate medium composition Gelcose 10g/l, NH1Cj! Ig/j! .

尿?、2g/l、KH2PO41g/1.KtHPOs
3g/j!、Mg5On・7H200,4g/l。urine? , 2g/l, KH2PO41g/1. KtHPOs
3g/j! , Mg5On.7H200, 4g/l.

Fe50.・7Hz0 10mg/l、MnS○、・4
 H2O4mg/ l 、ビオチン50px/1.ニコ
チン酸5mg/j!、ZnSO4・7H*O1mg/f
Fe50.・7Hz0 10mg/l, MnS○, ・4
H2O 4mg/l, biotin 50px/1. Nicotinic acid 5mg/j! , ZnSO4・7H*O1mg/f
.

Cu5O* ・5H201mg/1.(NH*)sMO
to2<・48201■/l、寒天2%、pH7,0第
    1    表 H−3149++  +  − H4412++ ++  + ++:充分な生育、+:わずかに生育、−二生育せずH
−3149を変異誘導することによって得られたβ−ナ
フトキノリンに抵抗性を有するH−4412は、昭和6
1年5月27日付で工業技術院微生物工業技術研究所(
微工研)にFERMBP−1069として寄託されてい
る。Cu5O* ・5H201mg/1. (NH*)sMO
to2<・48201■/l, agar 2%, pH 7.0 Table 1 H-3149++ + - H4412++ ++ + ++: Sufficient growth, +: Slight growth, -2 No growth H
H-4412, which is resistant to β-naphthoquinoline and was obtained by mutating H-3149, was developed in 1986.
As of May 27, 2015, the Institute of Microbial Technology, Agency of Industrial Science and Technology (
It has been deposited as FERMBP-1069 at the Microtechnical Research Institute.

本発明に使用する培地組成としては使用菌株の    
 ゛利用しろる炭素源、窒素源、無機物その他の必要な
栄養素を程良く含有するものであれば合成培地、天然培
地のいずれも使用できる。The culture medium composition used in the present invention is based on the strain used.
``Both synthetic and natural media can be used as long as they contain appropriate amounts of usable carbon sources, nitrogen sources, inorganic substances, and other necessary nutrients.

すなわち炭素源としてはグルコース、フラクトース、ソ
ルビトール、グリセロール、蔗Ill、 am。That is, carbon sources include glucose, fructose, sorbitol, glycerol, and am.

澱粉加水分解物、糖蜜、果汁などの各種炭水化物、酢酸
、フマール酸、乳酸、コハク酸などの有機酸、さらにエ
タノール、メタノールなどのアルコール類も使用できる
Various carbohydrates such as starch hydrolysates, molasses, and fruit juices, organic acids such as acetic acid, fumaric acid, lactic acid, and succinic acid, and alcohols such as ethanol and methanol can also be used.

窒素源としては、アンモニア、塩化アンモニウム、硫酸
アンモニウム、酢酸アンモニウム、リン酸アンモニウム
などの各種無機酸のアンモニウム塩、尿素、アミン類、
その地合窒素化合物、ならびにペプトン、肉エキス、酵
母エキス、コーン・スチープ・リカー、カゼイン加水分
解物、大豆粕酸加水分解物、各種発酵菌体およびその消
化物などが使用できる。Nitrogen sources include ammonium salts of various inorganic acids such as ammonia, ammonium chloride, ammonium sulfate, ammonium acetate, ammonium phosphate, urea, amines,
The formed nitrogen compounds, peptone, meat extract, yeast extract, corn steep liquor, casein hydrolyzate, soybean meal hydrolyzate, various fermented microbial cells and digested products thereof, etc. can be used.

さらに無機物としては、リン酸第−カリウム。Furthermore, potassium phosphate is an inorganic substance.

リン酸第二カリウム、リン酸マグネシウム、硫酸マグネ
シウム、塩化ナトリウム、硫酸第一鉄、硫酸マンガン、
炭酸カルシウムなどが使用できる。Potassium phosphate, magnesium phosphate, magnesium sulfate, sodium chloride, ferrous sulfate, manganese sulfate,
Calcium carbonate etc. can be used.

本発明に使用する微生物が生育のために特定の栄養素を
必要とする場合には、その栄養素を適当量培地中に存在
させなければならないが、これらの物質は窒素源として
例示した天然物に含まれて添加される場合がある。また
培地中に各種の添加物、例えば各種抗生物質、α−アミ
ノ酪酸、システィン、ロイシン、ロイシン発酵液あるい
はアスパラギン酸、グルタミン酸などを添加することに
よりL−リジン生産量を増加させうる場合がある。If the microorganisms used in the present invention require specific nutrients for growth, the nutrients must be present in appropriate amounts in the culture medium, but these substances are not included in the natural products exemplified as nitrogen sources. It may be added as a result. Furthermore, the amount of L-lysine produced may be increased by adding various additives to the culture medium, such as various antibiotics, α-aminobutyric acid, cysteine, leucine, leucine fermentation broth, aspartic acid, and glutamic acid.

培養は振盪培養あるいは深部通気攪拌培養などの好気的
条件下で行う。培養温度は通常20〜40℃の範囲であ
る。培地のpHは3〜9の範囲で、好ましくは中性付近
に保持することが望ましいが、これ以外の条件下でも使
用菌株が生育すれば実施できる。培地のpH調節は炭酸
カルシウム、尿素。Cultivation is performed under aerobic conditions such as shaking culture or deep aeration agitation culture. The culture temperature is usually in the range of 20 to 40°C. Although it is desirable to maintain the pH of the culture medium in the range of 3 to 9, preferably near neutrality, it can be carried out under other conditions as long as the strain used grows. The pH of the medium was adjusted using calcium carbonate and urea.

酸あるいはアルカリ溶液、pH緩衝剤などによって行う
。培養時間は通常1〜6日間で培養液中にL−リジンが
生成蓄積する。This is done using acid or alkaline solutions, pH buffers, etc. The culture time is usually 1 to 6 days, and L-lysine is produced and accumulated in the culture solution.

培養終了後、培養液より菌体などの沈殿物を除去し、公
知のイオン交換処理法、濃縮法、吸着法、塩析法などを
併用することにより、培養液からし−リジンを回収する
ことができる。After the culture is completed, precipitates such as bacterial cells are removed from the culture solution, and lysine is recovered from the culture solution by using a combination of known ion exchange treatment methods, concentration methods, adsorption methods, salting-out methods, etc. Can be done.

以下、実施例をあげて本発明を具体的に示す。Hereinafter, the present invention will be specifically illustrated by giving examples.

実施例1゜ 種菌としてコリネバクテリウム・グルタミクムH−44
12(FERM  BP−1069)を使用した。Example 1 Corynebacterium glutamicum H-44 as inoculum
12 (FERM BP-1069) was used.

この菌株をグルコース40g/j!、尿素3g/CKH
aPO41,5g#!、KaHPOa 0.5g/A。This strain has 40g/j of glucose! , urea 3g/CKH
aPO41,5g#! , KaHPOa 0.5g/A.

Mg5O<・7Hz○ 0.5g/!、ビオチン50■
/l、ペプトン20g/l、酵母エキス5g/j!から
なる種培地(pH7゜2)20mlを含む303ml容
三角フラスコに接種し、30℃で24時間培養した。こ
の培養液2+111を廃糖蜜100g/j!(グルコー
ス換算)、硫酸アンモニウム40g/β、 K H2P
 040.5g/CMg SO40,5g/j! 、 
CaCO530g/12からなる発酵培地(pH7,2
) 20mlを含む3、OQ+nl容三角フラスコに接
種し、32℃で3日間振盪培養(22Orpm)を行っ
た。このとき培養液中にL−IJリジン塩酸塩47g/
j!蓄積した。Mg5O<・7Hz○ 0.5g/! , biotin 50■
/l, peptone 20g/l, yeast extract 5g/j! It was inoculated into a 303 ml Erlenmeyer flask containing 20 ml of a seed medium (pH 7.2) consisting of the following, and cultured at 30°C for 24 hours. This culture solution 2+111 is mixed with blackstrap molasses 100g/j! (converted to glucose), ammonium sulfate 40g/β, K H2P
040.5g/CMg SO40.5g/j! ,
Fermentation medium (pH 7.2) consisting of CaCO 530g/12
) It was inoculated into a 3,0Q+nl Erlenmeyer flask containing 20ml, and cultured with shaking (22Orpm) at 32°C for 3 days. At this time, 47 g of L-IJ lysine hydrochloride/
j! Accumulated.

対照として、同一の条件で同時に培養した親株のH−3
149のLIJジン塩酸塩の生成量は43g/lであっ
た。As a control, the parent strain H-3 was cultured at the same time under the same conditions.
The amount of LIJ gin hydrochloride produced in 149 was 43 g/l.

発明の効果 本発明方法によれば、L−リジンを工業的に安価に供給
することができる。Effects of the Invention According to the method of the present invention, L-lysine can be supplied industrially at low cost.

手続補正書(自発) 昭和62年 7月 ls″日 1、事件の表示 昭和61年特許願第156775号 2、発明の名称 L−リジンの製造法 3、補正をする者 事件との関係  特許出願人 郵便番号 100 住所 東京都千代田区大手町−丁目6番1号名称 (1
02)協和醗酵工業株式会社明細書の発明の詳細な説明
の欄 5、補正の内容 の次に「、特公昭55−44597Jを加入する。Procedural amendment (spontaneous) July ls'' day 1, 1985, case description 1988 Patent Application No. 156775 2, title of invention: Process for producing L-lysine 3, person making the amendment Relationship with the case Patent application Postal code 100 Address 6-1 Otemachi-chome, Chiyoda-ku, Tokyo Name (1
02) In Column 5 of the detailed description of the invention in the specification of Kyowa Hakko Kogyo Co., Ltd., next to the contents of the amendment, ``, Japanese Patent Publication No. 55-44597J is added.

(2)同書第10頁22行のrMgsOnJをriJg
sO4・7tlzOjに訂正する。(2) riJg rMgsOnJ on page 10, line 22 of the same book.
Corrected to sO4・7tlzOj.

(3)同書第10頁最下行の「3日」を「4日」に訂正
する。(3) "3rd" on the bottom line of page 10 of the same book is corrected to "4th".

(4)同書第11頁1〜5行の「このとき・・・・・・
・・・43g/βであった。」を次の文章に訂正する。(4) On page 11 of the same book, lines 1-5, “At this time...
...It was 43g/β. ” to the following sentence.

[培養終了後、L−1ジンの生成量を酸性銅ニンヒドリ
ン反応を用いる比色法によって測定した。その結果、培
養液中のl、  IJリジン成量は塩酸塩として52g
/Ilであった。対照として、同一の条件で同様にして
培養した親株H−3149のL−IJリジン成量は、塩
酸塩として44g/j!であった。[After the cultivation was completed, the amount of L-1 gin produced was measured by a colorimetric method using acidic copper ninhydrin reaction. As a result, the amount of l, IJ lysine in the culture solution was 52g as hydrochloride.
/Il. As a control, the L-IJ lysine production of the parent strain H-3149, which was similarly cultured under the same conditions, was 44 g/j as hydrochloride! Met.

H−4412株を用いて得た培養液11を遠心分離し、
得られた上清液を硫酸でpH1,5に調整した後、強酸
性イオン交換樹脂ダイヤイオン5K−IB(H“型)(
三菱化成工業社製)のカラムに通し、L−リジンを吸着
させ、カラムを水洗後、2規定のアンモニア水で溶出し
て、L−リジン画分を集めた。集めた両分を濃縮し、得
られたa槽液を塩酸でpH2,0に調整した後、エタノ
ールを添加しながら冷却することによりL−リジン塩酸
塩を晶出させ、結晶41gを得た。」Centrifuging the culture solution 11 obtained using the H-4412 strain,
After adjusting the obtained supernatant liquid to pH 1.5 with sulfuric acid, strongly acidic ion exchange resin Diaion 5K-IB (H" type) (
The mixture was passed through a column (manufactured by Mitsubishi Chemical Industries, Ltd.) to adsorb L-lysine, and after washing the column with water, it was eluted with 2N aqueous ammonia to collect the L-lysine fraction. Both collected fractions were concentrated, and the obtained tank a solution was adjusted to pH 2.0 with hydrochloric acid, and then cooled while adding ethanol to crystallize L-lysine hydrochloride to obtain 41 g of crystals. ”

Claims (1)

【特許請求の範囲】[Claims] コリネ型グルタミン酸生産菌に属し、β−ナフトキノリ
ンに抵抗性を有し、かつL−リジン生産能を有する微生
物を培地に培養し、培養物中にL−リジンを生成蓄積さ
せ、該培養物からL−リジンを採取することを特徴とす
るL−リジンの製造法。A microorganism belonging to coryneform glutamate-producing bacteria, resistant to β-naphthoquinoline, and capable of producing L-lysine is cultured in a medium, L-lysine is produced and accumulated in the culture, and L-lysine is produced and accumulated in the culture. - A method for producing L-lysine, which comprises collecting lysine.
JP15677586A 1986-07-03 1986-07-03 Production of l-lysine Granted JPS6312292A (en)

Priority Applications (6)

Application Number Priority Date Filing Date Title
JP15677586A JPS6312292A (en) 1986-07-03 1986-07-03 Production of l-lysine
MX711587A MX168303B (en) 1986-07-03 1987-06-29 A PROCEDURE FOR PRODUCING L-LYSINE
FR8709309A FR2601035B1 (en) 1986-07-03 1987-07-01 PROCESS FOR THE PREPARATION OF L-LYSINE
CN 87104553 CN1022931C (en) 1986-07-03 1987-07-01 Process for producing L-lysine
HU300487A HU200797B (en) 1986-07-03 1987-07-02 Process for producing l-lysine
AU75059/87A AU597387B2 (en) 1986-07-03 1987-07-02 A process for producing L-lysine

Applications Claiming Priority (1)

Application Number Priority Date Filing Date Title
JP15677586A JPS6312292A (en) 1986-07-03 1986-07-03 Production of l-lysine

Publications (2)

Publication Number Publication Date
JPS6312292A true JPS6312292A (en) 1988-01-19
JPH0555114B2 JPH0555114B2 (en) 1993-08-16

Family

ID=15635042

Family Applications (1)

Application Number Title Priority Date Filing Date
JP15677586A Granted JPS6312292A (en) 1986-07-03 1986-07-03 Production of l-lysine

Country Status (6)

Country Link
JP (1) JPS6312292A (en)
CN (1) CN1022931C (en)
AU (1) AU597387B2 (en)
FR (1) FR2601035B1 (en)
HU (1) HU200797B (en)
MX (1) MX168303B (en)

Cited By (2)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US6000931A (en) * 1995-05-19 1999-12-14 Matsushita Electric Industrial Co., Ltd. Gas safety control system
JP2010516274A (en) * 2007-01-24 2010-05-20 シージェイ チェイルジェダン コーポレイション Method for producing fermentation products from carbon sources containing glycerol using corynebacteria

Families Citing this family (4)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
JP3006939B2 (en) * 1991-10-21 2000-02-07 協和醗酵工業株式会社 Method for producing L-lysine
KR100830289B1 (en) * 2007-01-18 2008-05-16 씨제이제일제당 (주) Corynebacterium glutamicum variety producing l-arginine and method for fabricating the same
WO2011111073A2 (en) * 2010-03-11 2011-09-15 Anand Bhadalakar PROCESS FOR BIOGENESIS OF L-LYSINE FROM ε-CAPROLACTAM OR ε-CAPROLACTAM DEGRADATION OR RELATED INTERMEDIATES
CN102399834A (en) * 2011-11-03 2012-04-04 中粮生物化学(安徽)股份有限公司 Method for preparing lysine

Family Cites Families (2)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
JPS594993B2 (en) * 1976-12-29 1984-02-02 味の素株式会社 Production method of L-lysine by fermentation method
GB2103617B (en) * 1981-08-10 1986-05-21 Kyowa Hakko Kogyo Kk Production of l-lysine by fermentation and new micro-organisms obtained by protoplast fusion

Cited By (2)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US6000931A (en) * 1995-05-19 1999-12-14 Matsushita Electric Industrial Co., Ltd. Gas safety control system
JP2010516274A (en) * 2007-01-24 2010-05-20 シージェイ チェイルジェダン コーポレイション Method for producing fermentation products from carbon sources containing glycerol using corynebacteria

Also Published As

Publication number Publication date
CN1022931C (en) 1993-12-01
MX168303B (en) 1993-05-17
HUT44080A (en) 1988-01-28
HU200797B (en) 1990-08-28
AU7505987A (en) 1988-01-07
CN87104553A (en) 1988-05-04
AU597387B2 (en) 1990-05-31
FR2601035A1 (en) 1988-01-08
FR2601035B1 (en) 1989-12-08
JPH0555114B2 (en) 1993-08-16

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