JP2000325090A - Dna encoding new aminopeptidase and method for producing the aminopeptidase - Google Patents

Dna encoding new aminopeptidase and method for producing the aminopeptidase

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Publication number
JP2000325090A
JP2000325090A JP2000071879A JP2000071879A JP2000325090A JP 2000325090 A JP2000325090 A JP 2000325090A JP 2000071879 A JP2000071879 A JP 2000071879A JP 2000071879 A JP2000071879 A JP 2000071879A JP 2000325090 A JP2000325090 A JP 2000325090A
Authority
JP
Japan
Prior art keywords
ala
leu
aminopeptidase
ser
val
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.)
Pending
Application number
JP2000071879A
Other languages
Japanese (ja)
Inventor
Hiroki Ninomiya
大記 二宮
Tetsuya Miwa
哲也 三輪
Minao Asano
皆夫 浅野
Nami Nakamura
奈巳 中村
Noriki Nio
式希 丹尾
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.)
Ajinomoto Co Inc
Original Assignee
Ajinomoto Co Inc
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Filing date
Publication date
Application filed by Ajinomoto Co Inc filed Critical Ajinomoto Co Inc
Priority to JP2000071879A priority Critical patent/JP2000325090A/en
Publication of JP2000325090A publication Critical patent/JP2000325090A/en
Pending legal-status Critical Current

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  • Enzymes And Modification Thereof (AREA)
  • Micro-Organisms Or Cultivation Processes Thereof (AREA)

Abstract

PROBLEM TO BE SOLVED: To obtain a new DNA encoding an aminopeptidase having a specific amino acid sequence and derived from a cotyledon of a germinating soybean seed, and capable of giving a decomposition product having a good taste and being rich in glutamic acid and aspartic acid by effectively decomposing a soybean protein. SOLUTION: This DNA is a new DNA encoding a new aminopeptidase having an amino acid sequence represented by the formula and derived from a cotyledon of a germinating soybean seed, and is capable of effectively producing an aminopeptidasae capable of producing a decomposition product rich in glutamic acid and aspartic acid and excellent in taste by effectively decomposing peptides derived from a soybean protein. The DNA is obtained by synthesizing an oligo DNA based on a predetermined amino acid sequence of aminopeptidase GX, obtaining a gene segment by RT-PCR method using an mRNA extracted from the cotyledon of the germinating soybean seed, and the like, as a template and screening a cDNA library, which is produced by using an mRNA of a part such as the cotyledon of the germinating soybean seed, and the like, as a template, by using the gene segment as a probe.

Description

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

【0001】[0001]

【発明の属する技術分野】本発明は、ダイズ由来の新規
なアミノペプチダーゼをコードするDNA、該DNAを
含有する組換え発現ベクター、該組換え発現ベクターに
より形質転換された形質転換体並びに形質転換体を用い
たアミノペプチダーゼの製造方法に関する。TECHNICAL FIELD The present invention relates to a DNA encoding a novel soybean-derived aminopeptidase, a recombinant expression vector containing the DNA, a transformant transformed with the recombinant expression vector, and a transformant. And a method for producing an aminopeptidase using the same.

【0002】[0002]

【従来の技術】ダイズタンパク質のアミノ酸への分解
は、塩酸や硫酸による酸分解、あるいは麹菌等の微生物
由来酵素をはじめとする既存のプロテアーゼによる分解
などにより行われている。2. Description of the Related Art Soybean proteins are decomposed into amino acids by acid decomposition with hydrochloric acid or sulfuric acid, or by existing proteases such as enzymes derived from microorganisms such as Aspergillus or the like.

【0003】しかしながら、酸による分解を行った場
合、天然調味料になり得るようなダイズタンパク質分解
物を得ようとすると、100℃、1〜2日間の反応が必
要であり、高温かつ長時間反応の為、エネルギー消費量
が大きいという問題がある。さらに酸によるタンパク質
の加水分解法は簡便である反面、アミノ酸の過剰(破
壊)分解、中和の為に高塩分となることなどの問題があ
る。[0003] However, in the case of decomposition with an acid, a reaction at 100 ° C for 1 to 2 days is required to obtain a soybean protein decomposition product that can be used as a natural seasoning. Therefore, there is a problem that energy consumption is large. Further, although the method of hydrolyzing proteins with an acid is simple, there are problems such as excessive (destructive) decomposition of amino acids and high salt content due to neutralization.

【0004】そこで上記問題を解決すべく、既存のプロ
テアーゼによる穏和な反応条件での分解が考えられた。
特にタンパク質分解酵素(プロテアーゼ)によるダイズ
タンパク質のアミノ酸への分解は、生物反応を利用する
穏やかな反応条件で進行するため、化学反応を利用する
酸加水分解に代わる方法として実現が期待された。[0004] In order to solve the above-mentioned problem, decomposition under mild reaction conditions with an existing protease was considered.
In particular, the decomposition of soybean protein into amino acids by proteolytic enzymes (proteases) proceeds under mild reaction conditions utilizing a biological reaction, and thus has been expected to be realized as an alternative to acid hydrolysis utilizing a chemical reaction.

【0005】しかしながら、一般にマメ科植物の貯蔵タ
ンパク質は、未変性の状態では、既存のプロテアーゼに
対してかなりの耐性を有している。また、パパイン、サ
チライシンに代表される既存のプロテアーゼはエンドペ
プチダーゼの為、タンパク質をペプチドに分解するが、
これだけでアミノ酸に完全分解することは困難であり、
また得られた製品は苦味を呈するために、調味料として
は使用できないのが実状である。However, legume storage proteins generally have considerable resistance to existing proteases in their native state. In addition, existing proteases represented by papain and subtilisin degrade proteins into peptides due to endopeptidases,
It is difficult to completely decompose into amino acids by this alone,
Moreover, since the obtained product has a bitter taste, it cannot be used as a seasoning.

【0006】さて、このような問題を解決するために、
ペプチドをアミノ酸に分解する酵素であるアミノペプチ
ダーゼ、カルボキシペプチダーゼなどのエキソペプチダ
ーゼの併用が有効と考えられた。Now, in order to solve such a problem,
Combinations of exopeptidases such as aminopeptidase and carboxypeptidase, which are enzymes that decompose peptides into amino acids, were considered effective.

【0007】一方、醤油の醸造に代表される麹菌を用い
たダイズタンパク質の分解において、遊離アミノ酸の増
加にはロイシンアミノペプチダーゼと酸性カルボキシペ
プチダーゼの重要性が示されている(中代忠信、醤研 V
ol.11, No.2, (1985))。しかしながら、同文献に示され
たように、醤油中には酸性アミノ酸を配列に含んだジペ
プチド、トリペプチドが残存し、これらの難分解性が指
摘されている。当該ジペプチド、トリペプチドには、N
末端にグルタミン酸あるいはアスパラギン酸を有したペ
プチドも含まれる。ペプチドの難分解性とは、分解反応
を触媒する酵素、すなわちペプチダーゼの基質特異性が
そのペプチドに対して低いことを意味する。このような
醤油醸造での麹菌由来ペプチダーゼに対する難分解性ペ
プチドの問題のみならず、市販のペプチダーゼ製剤にお
いても、麹菌由来酵素を代表とする微生物酵素では同様
に酸性アミノ酸を配列に含んだジペプチダーゼ、トリペ
プチドに対する分解力は低い。On the other hand, in the degradation of soybean proteins using koji molds typified by soy sauce brewing, the importance of leucine aminopeptidase and acid carboxypeptidase has been shown to increase free amino acids (Tadanobu Nakadai, Shoken V
ol. 11, No. 2, (1985)). However, as shown in the literature, dipeptides and tripeptides containing acidic amino acids in the sequence remain in soy sauce, and their indegradability has been pointed out. The dipeptide and tripeptide include N
Peptides having glutamic acid or aspartic acid at the terminal are also included. The term "hardly decomposable" means that the enzyme that catalyzes the decomposition reaction, that is, peptidase, has low substrate specificity for the peptide. Not only the problem of a peptide that is hardly decomposable against koji mold-derived peptidase in soy sauce brewing, but also in a commercially available peptidase preparation, a dipeptidase containing an acidic amino acid in the sequence in the microbial enzyme represented by the koji mold-derived enzyme, Degrading power for tripeptide is low.

【0008】そこで、本発明者らは上記課題の解決法を
ダイズ子葉中に求めた。すなわち、ダイズは、その発芽
過程に於いて、種子中の貯蔵タンパク質を非常に短時間
にアミノ酸にまで分解する。この現象より、発芽ダイズ
中に貯蔵タンパク質由来の難分解性ペプチドを容易に分
解しうるペプチダーゼが存在することが予想される。本
発明者らは、このようなペプチダーゼ類(酸性アミノ酸
含有ペプチドを効率的に分解するアミノペプチダーゼG
X、及びロイシンアミノペプチダーゼ群)を発芽ダイズ
子葉中より見いだし、ダイズタンパク質の効率的な加水
分解を行うことに成功した(特開平9-294583号)。Therefore, the present inventors have sought a solution for the above-mentioned problem in soybean cotyledons. That is, soybeans degrade storage proteins in seeds into amino acids in a very short time during the germination process. From this phenomenon, it is expected that a peptidase capable of easily decomposing the hardly degradable peptide derived from the storage protein is present in the germinated soybean. The present inventors have proposed such peptidases (aminopeptidase G that efficiently degrades peptides containing acidic amino acids).
X and leucine aminopeptidase group) were found in the germinated soybean cotyledons and succeeded in efficiently hydrolyzing the soybean protein (JP-A-9-294583).

【0009】しかしながら、ダイズアミノペプチダーゼ
GXの発芽ダイズ子葉中での含量は微量であるため、当
酵素を発芽ダイズ子葉抽出液より大量に調製することは
困難であった。However, since the content of soy aminopeptidase GX in the germinated soybean cotyledons is very small, it has been difficult to prepare this enzyme in a larger amount than the germinated soybean cotyledon extract.

【0010】[0010]

【発明が解決しようとする問題】上述の問題点を解決す
る方法の1つとしては、該アミノペプチダーゼ遺伝子を
ダイズ以外の系で遺伝子組換え技術を用いて大量生産さ
せることにより、大量の当該アミノペプチダーゼを取得
する方法が挙げられる。この方法を実現する為には、ま
ず、当該アミノペプチダーゼをコードするcDNAを取
得し、塩基配列を解析し、該アミノペプチダーゼの全ア
ミノ酸配列に関する情報を得ることが必須である。One of the methods for solving the above problems is to produce a large amount of the aminopeptidase gene by using a gene recombination technique in a system other than soybean. A method for obtaining a peptidase is included. In order to realize this method, it is essential to first obtain a cDNA encoding the aminopeptidase, analyze the nucleotide sequence, and obtain information on the entire amino acid sequence of the aminopeptidase.

【0011】次に、該アミノペプチダーゼをコードする
DNAを適当な発現ベクターに組み込み、目的物を大量
に生産する形質転換体を得ることが必須である。Next, it is essential that a DNA encoding the aminopeptidase is incorporated into an appropriate expression vector to obtain a transformant which produces a large amount of the desired product.

【0012】本発明はこのような事情を鑑みてなされた
もので、発芽ダイズ子葉に由来するアミノペプチダーゼ
を天然から単離する方法に代えて、遺伝子組換え技術を
用いて効率的な遺伝子発現並びに該アミノペプチダーゼ
の大量生産を成しえる為の技術を提供する事を目的とす
る。The present invention has been made in view of such circumstances, and instead of using a method of isolating aminopeptidase derived from germinated soybean cotyledons from nature, efficient gene expression and gene recombination using a gene recombination technique have been proposed. It is an object of the present invention to provide a technique for mass-producing the aminopeptidase.

【0013】[0013]

【課題を解決するための手段】本研究者らは上記課題を
解決するために鋭意研究を行い、アミノペプチダーゼG
Xの内部アミノ酸配列と相同性の高い、イネESTをプ
ローブに用いることにより、発芽ダイズshootmRNA
より調製したcDNAライブラリーをスクリーニング
し、該アミノペプチダーゼをコードするcDNAを取得
した。Means for Solving the Problems The present inventors have conducted intensive studies in order to solve the above-mentioned problems and found that aminopeptidase G
By using rice EST having high homology to the internal amino acid sequence of X as a probe, germinated soybean shoot mRNA
The cDNA library prepared above was screened to obtain cDNA encoding the aminopeptidase.

【0014】本研究者らは更に研究を進め、この得られ
たcDNAを用いて、該アミノペプチダーゼを生産する
形質転換体を得、これにより該アミノペプチダーゼ活性
を有するタンパク質を得るに至った。The present inventors have further studied and obtained a transformant producing the aminopeptidase using the obtained cDNA, thereby obtaining a protein having the aminopeptidase activity.

【0015】すなわち本発明は、以下の通りである。 (1)配列表配列番号1に記載されるアミノ酸配列を有
する発芽ダイズ子葉由来の新規アミノペプチダーゼをコ
ードするDNA。 (2)配列表配列番号1に記載されるアミノ酸配列に於
いて、1もしくは複数のアミノ酸残基が挿入、付加、欠
失もしくは置換されたアミノ酸配列を有し、かつ、アミ
ノペプチダーゼを活性を有するタンパク質をコードする
DNA。 (3)配列表配列番号2に記載される塩基配列のうち、
塩基番号22から1482までの塩基配列を有する上記(1)
のDNA。 (4)上記(1)〜(3)のいずれかのDNAを含有す
る組換えDNA。 (5)上記(4)の組換えDNAで形質転換された形質
転換体。 (6)上記(5)の形質転換体を培養し、アミノペプチ
ダーゼ活性を有するタンパク質を生産させ、これを回収
することを特徴とするアミノペプチダーゼ活性を有する
タンパク質の製造方法。That is, the present invention is as follows. (1) A DNA encoding a novel aminopeptidase derived from germinated soybean cotyledons having the amino acid sequence set forth in SEQ ID NO: 1 in the Sequence Listing. (2) In the amino acid sequence represented by SEQ ID NO: 1 in the Sequence Listing, the amino acid sequence has one or more amino acid residues inserted, added, deleted or substituted, and has an aminopeptidase activity. DNA encoding a protein. (3) Among the nucleotide sequences described in SEQ ID NO: 2 in the sequence listing,
The above (1) having a base sequence from base numbers 22 to 1482
DNA. (4) A recombinant DNA containing the DNA of any of the above (1) to (3). (5) A transformant transformed with the recombinant DNA of (4). (6) A method for producing a protein having aminopeptidase activity, comprising culturing the transformant of (5) above, producing a protein having aminopeptidase activity, and recovering the protein.

【0016】[0016]

【発明実施の形態】以下、本発明について詳述する。以
後、アミノペプチダーゼGXをGXと記す。BEST MODE FOR CARRYING OUT THE INVENTION Hereinafter, the present invention will be described in detail. Hereinafter, aminopeptidase GX is referred to as GX.

【0017】<1>本発明のDNA 本発明のcDNAの取得方法の具体例としては、例え
ば、すでに決定されているGXのアミノ酸配列に基づい
てオリゴDNAを合成し、発芽ダイズ子葉もしくは他の
部位から抽出したmRNAを鋳型にRT−PCR法で遺
伝子断片を得、それをプローブに発芽ダイズ子葉もしく
は他の部位のmRNAを鋳型に作製したcDNAライブ
ラリーから、ハイブリダイゼーションによりGXのcD
NAを釣り上げるなど、従来、慣用的に行われている方
法が挙げられる。<1> DNA of the Present Invention As a specific example of the method for obtaining the cDNA of the present invention, for example, oligo DNA is synthesized based on the amino acid sequence of GX which has already been determined, and germinated soybean cotyledons or other sites are synthesized. A gene fragment was obtained by RT-PCR using the mRNA extracted from the template as a template, and using the probe as a probe, a cDNA library prepared using mRNA of germinated soybean cotyledons or other sites as a template was subjected to hybridization to obtain GX cD.
Conventionally, a method conventionally used, such as catching NA, may be used.

【0018】また、すでに決定されているGXのアミノ
酸配列と相同性の高い、塩基配列を適当なDNAデータ
ベース、例えばDDBJ、EMBL、GenBankな
どが挙げられる、より検索し、当該する配列をプローブ
に、発芽ダイズ子葉もしくは他の部位から抽出したmR
NAを鋳型に作製したcDNAライブラリーをスクリー
ニングし、GXのcDNAを取得する方法も考えられ
る。Further, a base sequence having high homology to the amino acid sequence of GX which has already been determined is searched from an appropriate DNA database, for example, DDBJ, EMBL, GenBank, etc., and the relevant sequence is used as a probe. MR extracted from germinated soybean cotyledons or other sites
A method of screening a cDNA library prepared using NA as a template to obtain GX cDNA is also conceivable.

【0019】GXのmRNA抽出に用いる発芽ダイズは
そのダイズの種類を問わない。すなわち市販されている
ダイズ、搾油原料として用いられているダイズなど、そ
の栽培産地、品種を限定しない。また、発芽の方法、栽
培条件、発芽の有無、発芽の期間は問わないが、ダイズ
種子を吸水させ、7〜10日間生長させた発芽ダイズを
用いるのが好ましい。The germinated soybean used for GX mRNA extraction is not limited to the type of soybean. That is, the cultivation area and cultivar are not limited, such as commercially available soybean and soybean used as a raw material for oil pressing. The method of germination, the cultivation conditions, the presence or absence of germination, and the period of germination are not limited, but it is preferable to use germinated soybeans which have been made to absorb soybean seeds and grown for 7 to 10 days.

【0020】また、cDNAのプローブは、すでに決定
されているアミノ酸配列を基に、発芽ダイズ子葉もしく
は他の部位から抽出したmRNAを鋳型に、RT−PC
R法等によって作製してもよく、あるいはアミノ酸配列
を基に化学合成しても良い。アミノ酸配列と相同性の高
い塩基配列をプローブに用いる場合、その塩基配列の起
源、遺伝子産物の機能は問わない。すなわち、既知のア
ミノペプチダーゼである必要は無く、また、遺伝子産物
の機能がわかっていなくても良く、EST(Expression
Sequence Tag)でもかまわない。後述の実施例におい
ては、イネの根由来のESTをプローブとして用いた。
なお、cDNAライブラリーの作製は、常法により行う
ことができる。A cDNA probe is prepared by RT-PC using mRNA extracted from germinated soybean cotyledons or other sites as a template based on the amino acid sequence which has already been determined.
It may be prepared by the R method or the like, or may be chemically synthesized based on the amino acid sequence. When a nucleotide sequence having high homology to the amino acid sequence is used as a probe, the origin of the nucleotide sequence and the function of the gene product are not limited. That is, it is not necessary to use a known aminopeptidase, and the function of the gene product may not be known.
Sequence Tag). In the examples described below, ESTs derived from rice roots were used as probes.
In addition, preparation of a cDNA library can be performed by a conventional method.

【0021】かくして配列表配列番号1に記載されるア
ミノ酸配列を有する発芽ダイズ子葉由来の新規アミノペ
プチダーゼをコードするDNAが得られる。なお、本発
明のDNAは、それがコードする蛋白質がアミノペプチ
ダーゼ活性を有する限り、配列表配列番号1に記載され
るアミノ酸配列に於いて、1もしくは複数のアミノ酸残
基が挿入、付加、欠失もしくは置換されたアミノ酸配列
を有するタンパク質をコードするDNAであってもよ
い。Thus, a DNA encoding a novel aminopeptidase derived from germinated soybean cotyledons having the amino acid sequence shown in SEQ ID NO: 1 in the Sequence Listing can be obtained. In the DNA of the present invention, one or more amino acid residues may be inserted, added, or deleted in the amino acid sequence described in SEQ ID NO: 1 as long as the protein encoded by the DNA has aminopeptidase activity. Alternatively, it may be a DNA encoding a protein having a substituted amino acid sequence.

【0022】<2>本発明の組換えDNA 次に、このようにして得たcDNAを発現ベクターに組
み込んで組換えDNAを作製する。用いるベクターは、
特に限定されるものではないが、宿主細胞内で自立複製
可能なものでも、染色体に1コピーもしくは複数のコピ
ーが挿入されるものでも良く、上記DNAすなわちGX
遺伝子を組み込みうる挿入部位を持ち、更にこの組み込
んだDNAを宿主細胞内で発現せしめることを可能とす
る領域が必要である。<2> Recombinant DNA of the Present Invention Next, the thus obtained cDNA is inserted into an expression vector to prepare a recombinant DNA. The vector used is
Although not particularly limited, those capable of autonomous replication in a host cell or those having one or more copies inserted into a chromosome may be used.
It is necessary to have an insertion site into which a gene can be inserted, and a region that allows the inserted DNA to be expressed in a host cell.

【0023】なお、ベクターに組み込むGX遺伝子とし
ては、cDNAだけでなく、cDNAから予想されるG
Xのアミノ酸配列をコードするように設計して合成され
たDNAでも良い。このようなアミノ酸配列を基にした
遺伝子の合成は、DNA自動合成機を利用して合成した
オリゴヌクレオチドをアニール後に連結することなどに
より、容易に行うことができる。The GX gene to be incorporated into the vector includes not only cDNA but also G
It may be a DNA designed and synthesized to encode the amino acid sequence of X. The synthesis of a gene based on such an amino acid sequence can be easily performed by linking oligonucleotides synthesized using an automatic DNA synthesizer after annealing and the like.

【0024】また、GXを発現、異種タンパク質との融
合タンパク質として生産させる方法もある。これは例え
ば、pGEXシステム(アマシャム・ファルマシアバイオテ
ック社製)などを用いることで、GXをグルタチオン−
S−トランスフェラーゼとの融合タンパク質としてエシ
ェリヒア・コリ(E. coli)に生産させることが可能で
ある。There is also a method of expressing GX and producing it as a fusion protein with a heterologous protein. For example, GX can be converted to glutathione by using a pGEX system (manufactured by Amersham-Pharmacia Biotech).
It can be produced in Escherichia coli (E. coli) as a fusion protein with S-transferase.

【0025】GX遺伝子を発現させるプロモーターとし
ては、通常異種タンパク質の発現に用いられる強力なプ
ロモーターを用いることができる。また、GX遺伝子の
下流にはターミネーターを挿入することもできる。例え
ば、trp、tac、lac、trc、λPL、T7等のプロモーター、
tpA、lpp、T4等のターミネーターが挙げられる。As a promoter for expressing the GX gene, a strong promoter usually used for expressing a heterologous protein can be used. Further, a terminator can be inserted downstream of the GX gene. For example, promoters such as trp, tac, lac, trc, λPL, T7,
Terminators such as tpA, lpp, T4 and the like can be mentioned.

【0026】また、翻訳の効率化のために、SD配列の
種類、数、SD配列と開始コドンの間の領域の塩基組
成、配列、長さをGX遺伝子の発現に最適になるように
するとよい。In order to improve the efficiency of translation, the type and number of the SD sequence, and the base composition, sequence and length of the region between the SD sequence and the initiation codon may be optimized for GX gene expression. .

【0027】GX発現に必要なプロモーターから翻訳開
始点までの領域は、従来公知のPCR法や化学合成法な
どにより調製することができる。この配列の一例を配列
番号3に示す。The region from the promoter required for GX expression to the translation start point can be prepared by a conventionally known PCR method, chemical synthesis method or the like. An example of this sequence is shown in SEQ ID NO: 3.

【0028】本発明の組換えDNAは、所望の発現系に
応じた公知の発現ベクターに、前記GX遺伝子を含むD
NAを従来公知の方法によって挿入することにより得る
ことが可能である。ここで用いる発現ベクターは多コピ
ーのものであることが望ましい。[0028] The recombinant DNA of the present invention can be prepared by adding a GX gene to a known expression vector according to a desired expression system.
It can be obtained by inserting NA by a conventionally known method. The expression vector used here is desirably a multicopy copy.

【0029】本発明の組換えDNAの調製に用いること
のできる公知のベクターとしてはpUC18、pHSG299等が挙
げられる。pUC18に本発明のDNAを組み込んで得られ
た本発明の組換えDNAの一具体例としては、pUCTRPGX
1-8がある。Known vectors that can be used for preparing the recombinant DNA of the present invention include pUC18, pHSG299 and the like. One specific example of the recombinant DNA of the present invention obtained by incorporating the DNA of the present invention into pUC18 is pUCTRPGX
There is 1-8.

【0030】<3>本発明の形質転換体 次に、前記組換えDNAが挿入されて得られた種々の形
質転換体について説明する。<3> Transformant of the Present Invention Next, various transformants obtained by inserting the above-mentioned recombinant DNA will be described.

【0031】該形質転換体となりうる細胞としては、E.
coli等の細菌が挙げられる。E.coliの一具体例として
は、JM109株(recA、endA1、gyrA96、thi、hsdR17、sup
E44、relA1、Δ(lac-proAB)/F' [traD36、proAB+、lacI
q、lacZΔM15])がある。The cells which can be the transformant include E. coli.
bacteria such as E. coli. As a specific example of E. coli, JM109 strain (recA, endA1, gyrA96, thi, hsdR17, sup
E44, relA1, Δ (lac-proAB) / F '(traD36, proAB +, lacI
q, lacZΔM15]).

【0032】この他の形質転換体となりうる細胞には、
枯草菌、酵母、麹菌等があり、これらのタンパク質分泌
能を利用して、GXを培地中に生産させる方法も考えら
れる。上記のような微生物の他、カイコ培養細胞などの
培養細胞を用いてもよい。Other potential transformants include the following cells:
There are Bacillus subtilis, yeast, Aspergillus and the like, and a method of producing GX in a medium by utilizing the protein secretion ability is also conceivable. In addition to the microorganisms described above, cultured cells such as silkworm cultured cells may be used.

【0033】次いで、上記組換えベクターを宿主細胞内
に導入し、形質転換体を得る。組換え発現ベクターの宿
主細胞内への導入方法は、従来の慣用的に用いられてい
る方法により行うことができる。コンピテントセル法、
プロトプラスト法、リン酸カルシウム共沈法、エレクト
ロポレーション法、マイクロインジェクション法、リポ
ソーム融合法等、種々のものが挙げられる。Next, the above recombinant vector is introduced into a host cell to obtain a transformant. The method for introducing the recombinant expression vector into the host cell can be carried out by a conventional and commonly used method. Competent cell method,
Various methods such as a protoplast method, a calcium phosphate coprecipitation method, an electroporation method, a microinjection method, and a liposome fusion method are exemplified.

【0034】<4>アミノペプチダーゼの製造法 このようにして得られた形質転換体を培養することによ
り、培養物中にGXを産生させる。これを公知の方法で
単離し、場合によっては精製することにより、目的とす
る酵素が得られる。<4> Method for Producing Aminopeptidase GX is produced in the culture by culturing the thus obtained transformant. This is isolated by a known method and, if necessary, purified to obtain the desired enzyme.

【0035】E.coliを宿主とした場合には、不活性なG
X会合体、すなわちタンパク質封入体としてGX遺伝子
産物を得た後、これを適当な方法で活性化することも可
能であり、活性再生後、活性型タンパク質を公知の方法
で分離精製することにより、目的の酵素を得てもよい。When E. coli is used as a host, inactive G
After obtaining a GX gene product as an X-aggregate, that is, a protein inclusion body, it is also possible to activate this by an appropriate method. After regenerating the activity, the active protein can be separated and purified by a known method. The desired enzyme may be obtained.

【0036】形質転換体を培養する為の培地は公知であ
り、例えば、E.coliではLB培地などの栄養培地や、M9培
地などの最小培地に炭素源、窒素源、ビタミン源等を添
加して用いることができる。形質転換体の培養は、宿主
に応じて、通常16〜42℃、好ましくは25〜37℃で5〜168
時間、好ましくは8〜72時間行う。振盪培養と静置培養
のいずれも可能であるが、必要に応じて攪拌、通気を行
ってもよい。また、GX発現のために誘導型プロモータ
ーを用いた場合は、培地にプロモーター誘導剤を添加し
て培養をおこなうこともできる。Culture media for culturing transformants are known. For example, in E. coli, a carbon source, a nitrogen source, a vitamin source, etc. are added to a nutrient medium such as an LB medium or a minimum medium such as an M9 medium. Can be used. Culture of the transformant is carried out usually at 16 to 42 ° C, preferably at 25 to 37 ° C, for 5 to 168, depending on the host.
It is carried out for an hour, preferably for 8 to 72 hours. Both shaking culture and stationary culture are possible, but stirring and aeration may be performed as necessary. When an inducible promoter is used for GX expression, the culture can be carried out by adding a promoter inducer to the medium.

【0037】GXの単離、精製方法としては、形質転換
体の抽出物より、公知の塩析、等電点沈殿法もしくは溶
媒沈殿法等の沈殿法、透析、限外濾過もしくはゲル濾過
等の分子量差を利用する方法、イオン交換クロマトグラ
フィー等の特異的親和性を利用する方法、疎水クロマト
グラフィー、逆相クロマトグラフィー等の疎水度の差を
利用する方法やその他アフィニティークロマトグラフィ
ー、SDSポリアクリルアミド電気泳動法、等電点電気
泳動法などが挙げられ、これらを組み合わせることによ
り精製が可能である。GX can be isolated and purified from the extract of the transformant by known methods such as salting out, isoelectric point precipitation or solvent precipitation, dialysis, ultrafiltration or gel filtration. A method using a difference in molecular weight, a method using a specific affinity such as ion exchange chromatography, a method using a difference in hydrophobicity such as hydrophobic chromatography and reverse phase chromatography, other affinity chromatography, and SDS polyacrylamide electricity Electrophoresis, isoelectric focusing, etc., can be mentioned, and purification can be performed by combining them.

【0038】[0038]

【実施例】以下、本発明を実施例に基づいて説明する。DESCRIPTION OF THE PREFERRED EMBODIMENTS The present invention will be described below with reference to embodiments.

【0039】[実施例1 GX cDNAのクローニン
グ]以下に、本実施例について<1>GXの内部アミノ
酸配列の決定、<2>GXと相同性の高い塩基配列の検
索、<3>ダイズにおけるGX発現部位の解析、<4>
イネEST R2219_2Aをプローブにした発芽ダイズshoot
由来cDNAライブラリーのスクリーニングについて分
説する。[Example 1 Cloning of GX cDNA] In the following, <1> determination of the internal amino acid sequence of GX, <2> search for a base sequence highly homologous to GX, and <3> GX in soybean Analysis of expression site, <4>
Germinated soybean shoot using rice EST R2219_2A as a probe
The screening of the derived cDNA library will now be described.

【0040】<1>GXの内部アミノ酸配列の決定 発芽ダイズ子葉より精製したGXタンパクを還元カルボ
キシメチル化後、リシルエンドペプチダーゼ(EC.3.4.2
1.50和光純薬)処理した。生じたペプチドフラグメント
をμRPC C2/C18 SC2.1/10カラム(ファルマシア社製)を用
いて分取した。各々のフラグメントにつきプロテインシ
ークエンサーでアミノ酸配列を解析したところ、計10
ヶ所のアミノ酸配列を決定することに成功した。<1> Determination of GX internal amino acid sequence GX protein purified from germinated soybean cotyledons is subjected to reductive carboxymethylation, and then lysyl endopeptidase (EC. 3.4.2).
1.50 Wako Pure Chemical Industries, Ltd.) The resulting peptide fragment was fractionated using a μRPC C2 / C18 SC2.1 / 10 column (Pharmacia). When the amino acid sequence of each fragment was analyzed using a protein sequencer, a total of 10
We have succeeded in determining the amino acid sequences at three locations.

【0041】<2>GXと相同性の高い塩基配列の検索 先に決定したアミノ酸配列をDDBJ(DNA DATA BASE
of JAPAN)のホモロジー検索にかけたところ、配列表配
列番号4記載のペプチドフラグメントNo.8に相同性の高
い、イネ根由来EST R2219_2Aが見つかった。この、イネ
のR2219_2AはイネのGXである可能性が高く、以後、こ
のイネR2219_2Aをプローブに、ダイズGXのクローニン
グを試みた。クローニングにあたり、ダイズのどの部位
で発現が顕著であるか検討した。<2> Search for base sequence having high homology to GX The amino acid sequence determined previously was compared with DDBJ (DNA DATA BASE).
of JAPAN), a rice root-derived EST R2219_2A having high homology to peptide fragment No. 8 described in SEQ ID NO: 4 in the sequence listing was found. It is highly probable that the rice R2219_2A is rice GX, and thereafter, cloning of soybean GX was attempted using the rice R2219_2A as a probe. At the time of cloning, it was examined at which site in soybean the expression was remarkable.

【0042】<3>ダイズにおけるGX発現部位の解析 プローブとするイネR2219_2AcDNAの部分断片はRT
ーPCR法により、以下のように得た。R2219_2AcDN
Aの一部を、イネ根総RNAを鋳型にRT−PCR法に
て増幅した。R2219_2A増幅用のプライマーはセンスプラ
イマーとしてR22192AU(配列表配列番号5)、アンチセ
ンスプライマーとしてR22192AD(配列表配列番号6)を
用いた。なお、増幅した領域はペプチドNo.8に対応する
部分を含んでなるものである。<3> Analysis of GX Expression Site in Soybean A partial fragment of rice R2219_2A cDNA used as a probe was RT
-Obtained by the PCR method as follows. R2219_2AcDN
A portion of A was amplified by RT-PCR using rice root total RNA as a template. As a primer for amplifying R2219_2A, R22192AU (SEQ ID NO: 5) was used as a sense primer, and R22192AD (SEQ ID NO: 6) was used as an antisense primer. The amplified region includes a portion corresponding to peptide No. 8.

【0043】RT−PCRにはTakara RNA PCR kitを用
いた。このときのPCRの条件は94℃、5min→55℃、1m
in→72℃、1minを1cycle行い、続いて、94℃、1min→55
℃、1min→72℃、1minを25サイクル行うものであっ
た。For the RT-PCR, Takara RNA PCR kit was used. The PCR conditions at this time were 94 ° C, 5min → 55 ° C, 1m
1 cycle of in → 72 ℃, 1min, then 94 ℃, 1min → 55
C., 1 min → 72 ° C., 1 min for 25 cycles.

【0044】次に上述のイネR2219_2AcDNAを用い
て、ノーザンハイブリダイゼーション法により、ダイズ
RNAにイネR2219_2Aと相同性のある配列があるか調べ
た。Next, using the above-mentioned rice R2219_2A cDNA, a soybean RNA was examined for a sequence homologous to rice R2219_2A by Northern hybridization.

【0045】取得したR2219_2AcDNAをプローブに、
ダイズの各部位から抽出した総RNAに対して、ノーザ
ンブロッティングを行った。使用したダイズの部位は、
発芽3日目子葉、発芽7日目子葉、発芽7日目shoot、
未熟子葉、さや、本葉であった。Using the obtained R2219_2A cDNA as a probe,
Northern blotting was performed on total RNA extracted from each part of soybean. The soybean parts used were
Germination day 3 cotyledon, germination day 7 cotyledon, germination day 7 shoot,
Immature cotyledons, pods, true leaves.

【0046】その結果、ハイブリダイゼーションの温度
を55℃又は60℃、stringency washの洗浄液を0.5×SS
C、0.1%SDSでハイブリダイゼーションと同じ温度で
洗浄したとき、発芽7日目shootに明瞭にシグナルが検
出された。また、その大きさは約1.5kbpと算出された。As a result, the hybridization temperature was 55 ° C. or 60 ° C., and the washing solution of the stringency wash was 0.5 × SS.
C, When washed with 0.1% SDS at the same temperature as the hybridization, a signal was clearly detected in the shoot on day 7 of germination. The size was calculated to be about 1.5 kbp.

【0047】この結果より、発芽ダイズshoot中には、
イネR2219_2Aとある程度の相同性を有するmRNAが存
在すると結論され、またそれが、GXであることが強く
期待されたので、このイネR2219_2AcDNAをプローブ
に、60℃でのハイブリダイゼーション、及びstringency
washのハイブリダイゼーションの条件で発芽7日目ダ
イズshootmRNAより調製したcDNAライブラリー
をスクリーニングし、GX cDNAの取得を試みた。From the results, it can be seen that during the germination soybean shoot,
It was concluded that there was an mRNA having some homology with rice R2219_2A, and it was strongly expected that it was GX. Therefore, using this rice R2219_2A cDNA as a probe, hybridization at 60 ° C and stringency were performed.
On the 7th day of germination, a cDNA library prepared from soybean shoot mRNA was screened under the conditions of wash hybridization to obtain GX cDNA.

【0048】<4>イネEST をプローブにした発芽
ダイズshoot由来cDNAライブラリーのスクリーニン
グ 常法に従い、調製した発芽7日目のダイズshoot poly A
RNAより調製したcDNAライブラリー7.2×104 pf
uを上記条件でスクリーニングしたところ、7個のハイ
ブリダイズするクローンを得た。各クローンの塩基配列
を決定したところ、クローンの1つに、配列表配列番号
4に記載のGX内部アミノ酸配列を含み、配列表配列番
号1に記載の487残基のアミノ酸からなるポリペプチ
ドをコードする、配列表配列番号2に記載の全GX塩基
配列を含むクローンが見つかった。<4> Screening of cDNA library derived from germinated soybean shoot using rice EST as probe A soybean shoot poly A prepared on the 7th day of germination prepared according to a conventional method.
CDNA library prepared from RNA 7.2 × 104 pf
When u was screened under the above conditions, seven hybridizing clones were obtained. When the nucleotide sequence of each clone was determined, one of the clones contained a GX internal amino acid sequence described in SEQ ID NO: 4 and encoded a polypeptide consisting of 487 amino acids described in SEQ ID NO: 1 in Sequence Listing. A clone containing the entire GX base sequence described in SEQ ID NO: 2 was found.

【0049】この塩基配列は、先に決定したGX内部ア
ミノ酸配列10ヶ所を、全てコードしていることから、
目的のGX cDNAであると考えられたので、次に、
このcDNAを用いて、E. coliによってGXタンパク
を生産させることとした。This base sequence encodes all of the 10 GX internal amino acid sequences previously determined.
Since it was considered to be the desired GX cDNA,
GX protein was produced by E. coli using this cDNA.

【0050】[実施例2 GXのE. coliでの生産]実
施例1で得られたGX cDNAをE. coliで機能する発
現ベクターに組み込み、この発現プラスミドを保持する
形質転換体を培養し、菌体内にGX活性を検出した。こ
の際、得られたGX cDNAの配列と同時に、E. coli
でのコドンの使用頻度を考慮して、N末端から2残基目
のAlaから5残基目のLeuまで、すなわち、Ala、Ala、Ly
s、Leuの4残基について、コドンを変更したものについ
ても発現プラスミドを作製し、その発現量を比較した。Example 2 Production of GX in E. coli The GX cDNA obtained in Example 1 was incorporated into an expression vector that functions in E. coli, and a transformant carrying this expression plasmid was cultured. GX activity was detected in the cells. At this time, simultaneously with the sequence of the obtained GX cDNA,
In consideration of the frequency of codon usage in Ala, from Ala at the second residue from the N-terminal to Leu at the fifth residue, ie, Ala, Ala, Ly
Expression plasmids were also prepared for the four residues s and Leu in which codons were changed, and the expression levels were compared.

【0051】以下、本実施例について、<1>発現プラ
スミドの構築、<2>該発現プラスミドを用いたE. col
iの形質転換体の作製と培養、<3>GX活性測定につ
いて分説する。Hereinafter, in this example, <1> construction of an expression plasmid and <2> E. coli using the expression plasmid
The preparation and culture of the transformant i and the measurement of <3> GX activity will be described separately.

【0052】<1>発現プラスミドの構築 (1)GX cDNAの配列そのままの発現プラスミド
の構築 GX遺伝子を転写するプロモーターは、培地中にトリプ
トファンの欠乏で容易に転写が誘導されるtrpプロモー
ターを用いることにした。マダイ・トランスグルタミナ
ーゼ(TG)遺伝子を高発現したプラスミドpTTG-22
(特開平6-225775号)は、trpプロモーターを用いてお
り、マダイTG遺伝子の上流の配列は、E.coliにおいて
異種タンパク質が高発現するようにデザインされてい
る。また、微生物由来トランスグルタミナーゼ(MT
G)遺伝子を高発現させたプラスミドpUCTRPMTG(+)D2
(欧州特許出願公開0889133号)は、このマダイTGの
発現プラスミドのtrpプロモーターを含む上流配列を用
いており(配列表配列番号3)、更に、多コピープラス
ミドpUC19に組み込むことにより、MTGが高発現する
ようになっている。<1> Construction of Expression Plasmid (1) Construction of Expression Plasmid as it is with GX cDNA As the promoter for transcribing the GX gene, a trp promoter whose transcription is easily induced by lack of tryptophan in the medium is used. I made it. Plasmid pTTG-22 highly expressing the red sea bream transglutaminase (TG) gene
(JP-A-6-225775) uses a trp promoter, and the sequence upstream of the red sea bream TG gene is designed to highly express a heterologous protein in E. coli. Microbial transglutaminase (MT
G) Plasmid pUCTRPMTG (+) D2 overexpressing gene
(European Patent Application Publication No. 0889133) uses an upstream sequence containing the trp promoter of the expression plasmid of red sea bream TG (SEQ ID NO: 3 in the Sequence Listing). It is supposed to.

【0053】GX cDNAの上流に、trpプロモーター
を結合させるために、PCRによりDNAフラグメント
の結合を行った。まず、図1のように、MTG発現プラ
スミドpUCTRPMTG(+)D2のtrpプロモーターを含む領域
(配列表配列番号3)と、GXcDNAの部分領域をP
CRで増幅した。trpプロモーター増幅用プライマーはT
RP-N2(配列表配列番号7)、TRP-C2(配列表配列番号
8)、またGX部分増幅用プライマーはGX-N1(配列表
配列番号9)、GX-C(配列表配列番号10)であり、TR
P-N2、GX-N1はセンスプライマー、TRP-C2、GX-Cはアン
チセンスプライマーである。また、GX-N1は、trpプロモ
ーターを含む配列と結合させるための11塩基の配列を
GXの開始コドンの直前に付加させるようにデザインし
てあり、この配列は、TRP-C2中の配列と相補的である。DNA fragments were ligated by PCR in order to bind the trp promoter upstream of the GX cDNA. First, as shown in FIG. 1, the region containing the trp promoter of the MTG expression plasmid pUCTRPMTG (+) D2 (SEQ ID NO: 3 in the Sequence Listing) and the partial region of the GX cDNA were
Amplified with CR. The primer for amplifying the trp promoter is T
RP-N2 (SEQ ID NO: 7), TRP-C2 (SEQ ID NO: 8), and primers for partial amplification of GX are GX-N1 (SEQ ID NO: 9) and GX-C (SEQ ID NO: 10). And TR
P-N2 and GX-N1 are sense primers, and TRP-C2 and GX-C are antisense primers. GX-N1 is designed so that an 11-base sequence for binding to a sequence containing the trp promoter is added immediately before the start codon of GX, and this sequence is complementary to the sequence in TRP-C2. It is a target.

【0054】まず、プラスミドpUCTRPMTG(+)D2に対して
プライマーTRP-N2とTRP-C2、また、GX cDNA全長
を含むプラスミド、pR2219iに対してプライマーGX-N1と
GX-Cで、PCRをそれぞれ、94℃、2minの後に、94℃、
30sec→50℃、5sec→72℃、30secを25サイクル行った。
各PCR産物をフェノール/クロロホルム処理後エタノ
ール沈殿を行い、100μLのdH2Oに溶解した。First, the primers TRP-N2 and TRP-C2 for the plasmid pUCTRPMTG (+) D2, and the primer GX-N1 for the plasmid containing the full length GX cDNA and pR2219i
In GX-C, PCR was performed at 94 ° C,
25 cycles of 30 sec → 50 ° C., 5 sec → 72 ° C., 30 sec were performed.
Each PCR product was subjected to phenol / chloroform treatment, followed by ethanol precipitation, and dissolved in 100 μL of dH2O.

【0055】各PCR産物から1μLづつとって混ぜ、9
4℃で10minの熱変性後、プライマーTRP-N2とGX-Cで、P
CRを94℃、30sec→55℃、5sec→72℃、1minの条件で2
5サイクル行った。Take 1 μL of each PCR product and mix.
After heat denaturation at 4 ° C for 10 minutes, primers TRP-N2 and GX-C
CR at 94 ℃, 30sec → 55 ℃, 5sec → 72 ℃, 1min 2
Five cycles were performed.

【0056】2回目のPCR産物をフェノール/クロロ
ホルムで抽出後、エタノール沈殿下ものを、EcoRIとKpn
Iで消化し、pUC18にサブクローニングし、pUCTRPGXN1-8
を得(図1)、シークエンスを確認した。After extracting the second PCR product with phenol / chloroform, the product under ethanol precipitation was extracted with EcoRI and Kpn.
Digested with I, subcloned into pUC18, pUCTRPGXN1-8
Was obtained (FIG. 1), and the sequence was confirmed.

【0057】次に、pR2219iに含まれる、GX遺伝子の
C末端を、KpnI、XbaIで切り出し、上記pUCTRPGXN1-8へ
サブクローニングすることで、trpプロモーターによる
GX発現プラスミドpUCTRPGX1-8を完成させた(図
2)。Next, the C-terminal of the GX gene contained in pR2219i was cut out with KpnI and XbaI and subcloned into the above-mentioned pUCTRPGXN1-8, thereby completing the GX expression plasmid pUCTRPGX1-8 using the trp promoter (FIG. 2). ).

【0058】(2)コドンを変更したGX発現プラスミ
ドの構築 (1)と同様の方法でプラスミドを構築した。但しGX
cDNAのN末端部分断片をPCRで増幅する際のセ
ンスプライマーに、GX-N2(配列表配列番号11)を用
いた。GX-N2はN末端から2から5残基までのAla、Al
a、Lys、Leuに相当するコドンをGCG GCG AAG CTAからGC
T GCT AAA CTGへ変更してある。(2) Construction of GX Expression Plasmid with Codon Changed A plasmid was constructed in the same manner as in (1). However, GX
GX-N2 (SEQ ID NO: 11 in the Sequence Listing) was used as a sense primer when amplifying the N-terminal partial fragment of the cDNA by PCR. GX-N2 is Ala, Al from 2 to 5 residues from N-terminal.
Codons corresponding to a, Lys and Leu were converted from GCG GCG AAG CTA to GC
Changed to T GCT AAA CTG.

【0059】まず、プラスミドpUCTRPMTG(+)D2に対して
プライマーTRP-N2とTRP-C2、また、pR2219iに対してプ
ライマーGX-N2とGX-Cで、PCRをそれぞれ、94℃、2mi
nの後に、94℃、30sec→50℃、5sec→72℃、30secを25
サイクル行った。各PCR産物をフェノール/クロロホ
ルム処理後エタノール沈殿を行い、100μLのdH2Oに溶解
した。First, PCR was performed at 94 ° C. and 2 mi with the primers TRP-N2 and TRP-C2 for the plasmid pUCTRPMTG (+) D2 and the primers GX-N2 and GX-C for the pR2219i, respectively.
After n, 94 ℃, 30sec → 50 ℃, 5sec → 72 ℃, 30sec 25
Cycled. Each PCR product was subjected to phenol / chloroform treatment, followed by ethanol precipitation, and dissolved in 100 μL of dH2O.

【0060】各PCR産物から1μLづつとって混ぜ、9
4℃で10minの熱変性後、プライマーTRP-N2とGX-Cで、P
CRを94℃、30sec→55℃、5sec→72℃、1minの条件で2
5サイクル行った。Mix 1 μL of each PCR product and mix.
After heat denaturation at 4 ° C for 10 minutes, primers TRP-N2 and GX-C
CR at 94 ℃, 30sec → 55 ℃, 5sec → 72 ℃, 1min 2
Five cycles were performed.

【0061】2回目のPCR産物をフェノール/クロロ
ホルムで抽出後、エタノール沈殿したものを、EcoRIとK
pnIで消化し、pUC18にサブクローニングし、pUCTRPGXN2
-1を得(図3)、シークエンスを確認した。After the second PCR product was extracted with phenol / chloroform and ethanol-precipitated, EcoRI and K
digested with pnI, subcloned into pUC18, pUCTRPGXN2
-1 was obtained (FIG. 3), and the sequence was confirmed.

【0062】次に、pR2219iに含まれる、GX遺伝子の
C末端を、KpnI、XbaIで切り出し、上記pUCTRPGXN2-1へ
サブクローニングすることで、trpプロモーターによる
GX発現プラスミドpUCTRPGX2-1を完成させた(図
4)。Next, the CX terminus of the GX gene contained in pR2219i was cut out with KpnI and XbaI and subcloned into the above pUCTRPGXN2-1 to complete the GX expression plasmid pUCTRPGX2-1 using the trp promoter (FIG. 4). ).

【0063】<2>該発現プラスミドを用いたE. coli
の形質転換体の作製と培養 コンピテントセル法によりpUCTRPGX1-8、pUCTRPGX2-1及
びpUC19をE. coli JM109に導入し、形質転換体を150μg
/mLのアンピシリンを含む寒天培地で選択した。なお、p
UCTRPGX2-1で形質転換したE.coliをAJ13564と命名し
た。このE.coli株は工業技術院生命工学工業技術研究所
に受託番号FERM P-17131として寄託され、その後、平成
12年2月14日にブダペスト条約に基づく寄託へ移管
され、受託番号FERM BP-7027として同機関に寄託されて
いる。各形質転換体を150μg/mLのアンピシリンを含む2
×YT培地に接種し、37℃で5hr培養した。この前培養液1
mLを150μg/mLのアンピシリンを含む50mLのM9-カザミノ
酸培地に移し、本培養とした。本培養は37℃で18hr行っ
た。<2> E. coli using the expression plasmid
Preparation and culture of transformants of pUCTRPGX1-8, pUCTRPGX2-1 and pUC19 were introduced into E. coli JM109 by the competent cell method, and 150 μg of the transformant was introduced.
Selection was performed on an agar medium containing 1 / mL ampicillin. Note that p
E. coli transformed with UCTRPGX2-1 was named AJ13564. This E. coli strain was deposited at the National Institute of Advanced Industrial Science and Technology under the accession number FERM P-17131, and was subsequently transferred to the deposit under the Budapest Treaty on February 14, 2000, and the accession number FERM BP- It has been deposited with the institution as 7027. Each transformant contains 150 μg / mL ampicillin 2
XYT medium was inoculated and cultured at 37 ° C. for 5 hours. This preculture 1
mL was transferred to 50 mL of M9-casamino acid medium containing 150 μg / mL ampicillin, and this was used as main culture. The main culture was performed at 37 ° C. for 18 hours.

【0064】培養終了後、遠心により集菌した菌体を、
菌体破砕用バッファー(50mM Tris-HCl(pH8.0)、5mM EDT
A)に懸濁し、超音波破砕をBranson MODEL-Sonifier 25
0のマイクロチップを用い、output control 7,duty cyc
le 50%で約10min行った。この破砕処理液を、12000rpm
で10min遠心して、上清を菌体内可溶性画分とし、ま
た、沈殿を不溶性画分として、SDS−ポリアクリルア
ミドゲル電気泳動を行った。その結果、pUCTRPGX1-8/JM
109の可溶性画分、及びpUCTRPGX2-1/JM109の可溶性画分
と不溶性画分に、GXと同一分子量を有するタンパク質
の発現が認められた。特にコドンを変更したpUCTRPGX2-
1/JM109については高発現が観察され、コドン変更によ
る効果は明らかであった。なお、生産培地には、3−β
−インドールアクリル酸を加えなくとも十分な高発現が
得られた。After completion of the culture, the cells collected by centrifugation are
Cell disruption buffer (50 mM Tris-HCl (pH 8.0), 5 mM EDT
A) Suspended and sonicated with a Branson MODEL-Sonifier 25
Output control 7, duty cyc
le 50% for about 10 min. This crushed liquid is 12000 rpm
, And the supernatant was used as a soluble fraction in the cells, and the precipitate was used as an insoluble fraction, followed by SDS-polyacrylamide gel electrophoresis. As a result, pUCTRPGX1-8 / JM
Expression of a protein having the same molecular weight as GX was observed in the soluble fraction of 109 and the soluble and insoluble fractions of pUCTRPGX2-1 / JM109. In particular, pUCTRPGX2- with codon changed
High expression was observed for 1 / JM109, and the effect of the codon change was apparent. The production medium contains 3-β
-Sufficient high expression was obtained without adding indoleacrylic acid.

【0065】<3>GX活性の測定 GX活性は、ジペプチドGlu-Gluの分解による、遊離グ
ルタミン酸量の増加で測定した。50mM HEPES(pH8.0)、5m
M Glu-Gluを含む活性測定溶液に、酵素溶液を加え、37
℃で5-10min反応させ、2%になるように酢酸を加えて反
応を止め、グルタミン酸アッセイkit(生化学工業)
を用いて、遊離グルタミン酸量を測定した。活性は1分
間に1μmolのグルタミン酸を遊離する活性を1unitとし
た。pUCTRPGX1-8/JM109、pUCTRPGX2-1/JM109、pUC19/JM
109の可溶性画分、すなわち菌体破砕上清のGX活性を
測定し、比活性を求めたところ、pUCTRPGX1-8/JM109で
は0.91U/mg、 pUCTRPGX2-1/JM109では2.88U/mg、 pUC19
/JM109では0.04U/mgとなり、菌体内に蓄積したGXタン
パクが活性を有することを確認した。また、コドンを変
更することにより約3倍のGXタンパクが蓄積すること
が確認された。<3> Measurement of GX activity GX activity was measured by an increase in the amount of free glutamic acid due to degradation of the dipeptide Glu-Glu. 50mM HEPES (pH8.0), 5m
Add the enzyme solution to the activity measurement solution containing M Glu-Glu, and add
Incubate at 5 ℃ for 5-10min, add acetic acid to 2% to stop the reaction, glutamate assay kit (Seikagaku Corporation)
Was used to measure the amount of free glutamic acid. The activity was defined as the activity of releasing 1 μmol of glutamic acid per minute as 1 unit. pUCTRPGX1-8 / JM109, pUCTRPGX2-1 / JM109, pUC19 / JM
The GX activity of the soluble fraction of 109, i.e., the supernatant of the disrupted cells was measured and the specific activity was determined. 0.91 U / mg for pUCTRPGX1-8 / JM109, 2.88 U / mg for pUCTRPGX2-1 / JM109, pUC19
In the case of / JM109, it was 0.04 U / mg, and it was confirmed that the GX protein accumulated in the cells had activity. In addition, it was confirmed that GX protein was accumulated about three times by changing the codon.

【0066】[0066]

【発明の効果】本発明によれば、タンパク質及びペプチ
ドを含む原料から、酸性アミノ酸含量の高い、分解の進
んだ加水分解物を生産するのに適したアミノペプチダー
ゼGXのアミノ酸配列をコードするcDNAが得られ
る。このcDNAをもとに、E. coliなどで組換え体ア
ミノペプチダーゼを量産できる。また、上記cDNAを
用いれば、E.coli以外の宿主でもアミノペプチダーゼG
Xを生産することが可能である。さらに、生産させたG
XをプロテアーゼFlavourzyme(登録商標)(Novo Nordi
sk A/S)およびProtease M(登録商標)(Amano Pharmac
eutical)のような商業的に入手可能なプロテアーゼと
組み合わせることにより、ダイズタンパク質より、グル
タミン酸ならびにアスパラギン酸含量の高い、呈味性の
優れた分解物を創出することが可能である。According to the present invention, a cDNA encoding an amino acid sequence of aminopeptidase GX suitable for producing a hydrolyzate having a high acid amino acid content and a high degree of degradation is obtained from a raw material containing proteins and peptides. can get. Based on this cDNA, recombinant aminopeptidase can be mass-produced in E. coli or the like. Further, if the above cDNA is used, aminopeptidase G can be used in hosts other than E. coli.
X can be produced. In addition, G
X is the protease Flavorzyme® (Novo Nordi
sk A / S) and Protease M® (Amano Pharmac
In combination with a commercially available protease such as eutical), it is possible to create a deodorant having a higher content of glutamic acid and aspartic acid and a better taste than soybean protein.

【0067】[0067]

【配列表】 Sequence Listing <110> 味の素株式会社(Ajinomoto Co., Inc.) <120> 新規アミノペプチダーゼをコードするDNA及び該アミノペプチダーゼの 製造方法 <130> Y1G0282 <150> JP 11-68255 <151> 1999-3-15 <160> 11 <210> 1 <211> 487 <212> PRT <213> Glycine max <400> 1 Met Ala Ala Lys Leu Asp Thr His Ala Val Ala Ser Asp Leu Ile Asp 1 5 10 15 Phe Leu Asn Ala Ser Pro Thr Ala Phe His Ala Val Asp Glu Ala Lys 20 25 30 Arg Arg Leu Arg Ser Ala Gly Tyr His Gln Leu Ser Glu Arg Glu Val 35 40 45 Trp Glu Leu Gln Pro Gly Asn Lys Tyr Phe Phe Thr Arg Asn His Ser 50 55 60 Thr Ile Val Ala Phe Ala Ile Gly Lys Lys Tyr Val Ala Gly Asn Gly 65 70 75 80 Phe Tyr Ile Ile Gly Ala His Thr Asp Ser Pro Cys Leu Lys Leu Lys 85 90 95 Pro Val Thr Lys Val Val Lys Ala Gly Ile Leu Glu Val Gly Val Gln 100 105 110 Thr Tyr Gly Gly Gly Leu Trp His Thr Trp Phe Asp Arg Asp Leu Thr 115 120 125 Val Ala Gly Arg Val Ile Val Arg Glu Glu Asn Ala Gly Ser Val Ser 130 135 140 Tyr Ser His Arg Leu Val Arg Ile Glu Glu Pro Ile Met Arg Ile Pro 145 150 155 160 Thr Leu Ala Ile His Leu Asp Lys Thr Val Asn Asp Gly Phe Lys Phe 165 170 175 Asn Asn Glu Asn His Leu Ile Pro Ile Leu Ala Thr Ser Leu Lys Gly 180 185 190 Glu Leu Asn Lys Val Ser Ser Glu Asn Gly Pro Val Glu Ser Gly Asn 195 200 205 Gln Thr Asp Gly Lys Lys Ala Asn Asp Lys Thr Gly Thr Ser Asn Thr 210 215 220 Lys His His Leu Leu Leu Leu Gln Leu Leu Ala Ser Lys Leu Gly Cys 225 230 235 240 Glu Pro Asp Asp Ile Cys Asp Phe Glu Leu Gln Ala Cys Asp Thr Gln 245 250 255 Pro Ser Thr Ile Ala Gly Ala Ala Lys Glu Phe Ile Phe Ser Gly Arg 260 265 270 Leu Asp Asn Leu Cys Met Ser Phe Cys Ser Leu Lys Ala Leu Ile Asp 275 280 285 Ala Thr Ser Ser Asp Ser Ser Leu Glu Glu Glu Ser Gly Val Arg Met 290 295 300 Val Ala Leu Phe Asp His Glu Glu Val Gly Ser Asn Ser Ala Gln Gly 305 310 315 320 Ala Gly Ser Pro Val Met Leu Asn Ala Val Thr Arg Val Thr Asn Ser 325 330 335 Phe Ser Ser Asn Pro Asn Leu Leu Glu Lys Ala Ala Gln Leu Ser Tyr 340 345 350 Leu Val Ser Ala Asp Met Ala His Ala Leu His Pro Asn Tyr Met Asp 355 360 365 Lys His Glu Ala Asn His Gln Pro Lys Leu His Gly Gly Leu Val Ile 370 375 380 Lys Thr Asn Ala Ser Gln Arg Tyr Ala Thr Asn Val Val Thr Ser Phe 385 390 395 400 Ile Phe Arg Glu Ile Ala Ser Lys His Lys Leu Pro Val Gln Asp Phe 405 410 415 Val Val Arg Asn Asp Met Ser Cys Gly Ser Thr Ile Gly Pro Ile Leu 420 425 430 Ala Ser Gly Val Gly Ile Arg Thr Val Asp Val Gly Ala Pro Gln Leu 435 440 445 Ser Met His Ser Ile Arg Glu Ile Cys Ala Val Asp Asp Val Lys Tyr 450 455 460 Ser Tyr Glu His Phe Lys Ala Phe Tyr Gln Glu Phe Ser His Val Asp 465 470 475 480 Gly Lys Met Val Val Asp Ile 485[Sequence Listing] Sequence Listing <110> Ajinomoto Co., Inc. <120> DNA encoding a novel aminopeptidase and method for producing the aminopeptidase <130> Y1G0282 <150> JP 11-68255 <151 > 1999-3-15 <160> 11 <210> 1 <211> 487 <212> PRT <213> Glycine max <400> 1 Met Ala Ala Lys Leu Asp Thr His Ala Val Ala Ser Asp Leu Ile Asp 1 5 10 15 Phe Leu Asn Ala Ser Pro Thr Ala Phe His Ala Val Asp Glu Ala Lys 20 25 30 Arg Arg Leu Arg Ser Ala Gly Tyr His Gln Leu Ser Glu Arg Glu Val 35 40 45 Trp Glu Leu Gln Pro Gly Asn Lys Tyr Phe Phe Thr Arg Asn His Ser 50 55 60 Thr Ile Val Ala Phe Ala Ile Gly Lys Lys Tyr Val Ala Gly Asn Gly 65 70 75 80 Phe Tyr Ile Ile Gly Ala His Thr Asp Ser Pro Cys Leu Lys Leu Lys 85 90 95 Pro Val Thr Lys Val Val Lys Ala Gly Ile Leu Glu Val Gly Val Gln 100 105 110 Thr Tyr Gly Gly Gly Leu Trp His Thr Trp Phe Asp Arg Asp Leu Thr 115 120 125 Val Ala Gly Arg Val Ile Val Arg Glu Glu Asn Ala Gly Ser Val Ser 130 135 140 Tyr Ser His Arg Le u Val Arg Ile Glu Glu Pro Ile Met Arg Ile Pro 145 150 155 160 Thr Leu Ala Ile His Leu Asp Lys Thr Val Asn Asp Gly Phe Lys Phe 165 170 175 Asn Asn Glu Asn His Leu Ile Pro Ile Leu Ala Thr Ser Leu Lys Gly 180 185 190 Glu Leu Asn Lys Val Ser Ser Glu Asn Gly Pro Val Glu Ser Gly Asn 195 200 205 Gln Thr Asp Gly Lys Lys Ala Asn Asp Lys Thr Gly Thr Ser Asn Thr 210 215 220 Lys His His Leu Leu Leu Leu Gln Leu Leu Ala Ser Lys Leu Gly Cys 225 230 235 240 Glu Pro Asp Asp Ile Cys Asp Phe Glu Leu Gln Ala Cys Asp Thr Gln 245 250 255 Pro Ser Thr Ile Ala Gly Ala Ala Lys Glu Phe Ile Phe Ser Gly Arg 260 265 270 270 Leu Asp Asn Leu Cys Met Ser Phe Cys Ser Leu Lys Ala Leu Ile Asp 275 280 285 Ala Thr Ser Ser Asp Ser Ser Leu Glu Glu Glu Ser Gly Val Arg Met 290 295 300 Val Ala Leu Phe Asp His Glu Glu Val Gly Ser Asn Ser Ala Gln Gly 305 310 315 320 Ala Gly Ser Pro Val Met Leu Asn Ala Val Thr Arg Val Thr Asn Ser 325 330 335 Phe Ser Ser Asn Pro Asn Leu Leu Glu Lys Ala Ala Gln Leu Ser Tyr 340 345 350 Leu Val Ser Ala A sp Met Ala His Ala Leu His Pro Asn Tyr Met Asp 355 360 365 Lys His Glu Ala Asn His Gln Pro Lys Leu His Gly Gly Leu Val Ile 370 375 380 Lys Thr Asn Ala Ser Gln Arg Tyr Ala Thr Asn Val Val Thr Ser Phe 385 390 395 400 Ile Phe Arg Glu Ile Ala Ser Lys His Lys Leu Pro Val Gln Asp Phe 405 410 415 Val Val Arg Asn Asp Met Ser Cys Gly Ser Thr Ile Gly Pro Ile Leu 420 425 430 Ala Ser Gly Val Gly Ile Arg Thr Val Asp Val Gly Ala Pro Gln Leu 435 440 445 Ser Met His Ser Ile Arg Glu Ile Cys Ala Val Asp Asp Val Lys Tyr 450 455 460 Ser Tyr Glu His Phe Lys Ala Phe Tyr Gln Glu Phe Ser His Val Asp 465 470 475 480 Gly Lys Met Val Val Asp Ile 485

【0068】 <210> 2 <211> 1657 <212> DNA <213> Glycine max <220> <221> CDS <222> 22..1482 <400> 2 aaaattaaaa tctgaaaaac a atg gcg gcg aag cta gac acc cac gcc gtg 51 Met Ala Ala Lys Leu Asp Thr His Ala Val 1 5 10 gct tcc gat ctg atc gac ttc ctc aac gct tct cca acg gct ttc cac 99 Ala Ser Asp Leu Ile Asp Phe Leu Asn Ala Ser Pro Thr Ala Phe His 15 20 25 gcc gtc gac gag gca aag agg cgt ttg cgt agc gcg ggg tac cac caa 147 Ala Val Asp Glu Ala Lys Arg Arg Leu Arg Ser Ala Gly Tyr His Gln 30 35 40 ctc tct gag agg gaa gtg tgg gaa ctg caa ccg ggc aac aag tac ttc 195 Leu Ser Glu Arg Glu Val Trp Glu Leu Gln Pro Gly Asn Lys Tyr Phe 45 50 55 ttc acc aga aat cac tcc acc atc gtc gcc ttc gcc atc ggc aaa aag 243 Phe Thr Arg Asn His Ser Thr Ile Val Ala Phe Ala Ile Gly Lys Lys 60 65 70 tac gtt gct gga aat gga ttc tac ata att ggg gct cac acg gat agt 291 Tyr Val Ala Gly Asn Gly Phe Tyr Ile Ile Gly Ala His Thr Asp Ser 75 80 85 90 cct tgt ctc aaa ctc aag cct gtc acc aag gtt gtt aag gct ggg att 339 Pro Cys Leu Lys Leu Lys Pro Val Thr Lys Val Val Lys Ala Gly Ile 95 100 105 ttg gag gtt ggt gtc caa acc tat gga ggt ggt ctg tgg cac aca tgg 387 Leu Glu Val Gly Val Gln Thr Tyr Gly Gly Gly Leu Trp His Thr Trp 110 115 120 ttt gat cga gac ttg act gtg gcg ggg agg gtc atc gtg cgg gaa gag 435 Phe Asp Arg Asp Leu Thr Val Ala Gly Arg Val Ile Val Arg Glu Glu 125 130 135 aat gct ggt tct gtt tcg tac tca cat cgc ctt gtt aga att gag gaa 483 Asn Ala Gly Ser Val Ser Tyr Ser His Arg Leu Val Arg Ile Glu Glu 140 145 150 cct ata atg cga ata ccg act ttg gca att cac ttg gac aag act gtt 531 Pro Ile Met Arg Ile Pro Thr Leu Ala Ile His Leu Asp Lys Thr Val 155 160 165 170 aat gat gga ttc aaa ttt aac aac gag aat cac ctt att ccc atc ttg 579 Asn Asp Gly Phe Lys Phe Asn Asn Glu Asn His Leu Ile Pro Ile Leu 175 180 185 gca aca tcg ctg aag ggt gag ctc aat aaa gtg tcc tct gaa aat ggt 627 Ala Thr Ser Leu Lys Gly Glu Leu Asn Lys Val Ser Ser Glu Asn Gly 190 195 200 cct gtt gaa agt gga aat cag acc gat gga aag aaa gca aat gat aaa 675 Pro Val Glu Ser Gly Asn Gln Thr Asp Gly Lys Lys Ala Asn Asp Lys 205 210 215 aca ggc acc agc aat acg aag cat cac ctt ctt ctt cta cag ttg ctt 723 Thr Gly Thr Ser Asn Thr Lys His His Leu Leu Leu Leu Gln Leu Leu 220 225 230 gca agc aag ctt ggg tgt gaa cca gat gac ata tgt gat ttt gaa ttg 771 Ala Ser Lys Leu Gly Cys Glu Pro Asp Asp Ile Cys Asp Phe Glu Leu 235 240 245 250 caa gct tgc gat aca caa cca agt act att gct gga gct gca aag gaa 819 Gln Ala Cys Asp Thr Gln Pro Ser Thr Ile Ala Gly Ala Ala Lys Glu 255 260 265 ttc att ttt tca gga cgg ctt gat aat ctc tgc atg tca ttt tgc tcg 867 Phe Ile Phe Ser Gly Arg Leu Asp Asn Leu Cys Met Ser Phe Cys Ser 270 275 280 ctg aag gca tta ata gat gct aca tct tct gac agc agt ctt gag gaa 915 Leu Lys Ala Leu Ile Asp Ala Thr Ser Ser Asp Ser Ser Leu Glu Glu 285 290 295 gag tca ggt gtt aga atg gtg gct tta ttt gac cat gag gaa gtt gga 963 Glu Ser Gly Val Arg Met Val Ala Leu Phe Asp His Glu Glu Val Gly 300 305 310 tct aac tct gcc caa gga gct ggc tct cct gtt atg cta aat gct gtg 1011 Ser Asn Ser Ala Gln Gly Ala Gly Ser Pro Val Met Leu Asn Ala Val 315 320 325 330 act agg gtt acc aat tcc ttc agc tcc aat ccc aac ctt ctg gag aaa 1059 Thr Arg Val Thr Asn Ser Phe Ser Ser Asn Pro Asn Leu Leu Glu Lys 335 340 345 gca gca caa tta agc tac ctt gta tct gcc gac atg gca cat gca cta 1107 Ala Ala Gln Leu Ser Tyr Leu Val Ser Ala Asp Met Ala His Ala Leu 350 355 360 cac cca aat tac atg gac aag cat gaa gca aac cat cag ccc aaa cta 1155 His Pro Asn Tyr Met Asp Lys His Glu Ala Asn His Gln Pro Lys Leu 365 370 375 cat gga gga ctt gtc att aaa acc aat gca agc caa cgc tat gca acc 1203 His Gly Gly Leu Val Ile Lys Thr Asn Ala Ser Gln Arg Tyr Ala Thr 380 385 390 aat gtt gtc aca tcc ttc ata ttc agg gag ata gca tca aaa cat aaa 1251 Asn Val Val Thr Ser Phe Ile Phe Arg Glu Ile Ala Ser Lys His Lys 395 400 405 410 ctt ccc gtt cag gac ttt gtg gtg cgc aat gac atg tca tgt ggt tca 1299 Leu Pro Val Gln Asp Phe Val Val Arg Asn Asp Met Ser Cys Gly Ser 415 420 425 acc att ggt cct att ctt gct agt ggc gta ggt att cgc act gtt gat 1347 Thr Ile Gly Pro Ile Leu Ala Ser Gly Val Gly Ile Arg Thr Val Asp 430 435 440 gta ggt gca ccg cag ttg tca atg cat agc ata cga gaa att tgt gct 1395 Val Gly Ala Pro Gln Leu Ser Met His Ser Ile Arg Glu Ile Cys Ala 445 450 455 gtt gat gat gtg aag tat tca tat gag cac ttc aaa gca ttt tac caa 1443 Val Asp Asp Val Lys Tyr Ser Tyr Glu His Phe Lys Ala Phe Tyr Gln 460 465 470 gaa ttc tct cat gtt gat ggt aag atg gtc gtg gat ata tag gaatatctc 1494 Glu Phe Ser His Val Asp Gly Lys Met Val Val Asp Ile 475 480 485 taatcacgaa atcctcatta atcctttgct ctagaagctg ttgctgaaat ggtcgtgttt 1554 cgtaatttag taccattata atgccgacgt tattatgatg aaattttcaa taaaattaga 1614 ctccctgaat gaaatattag caactaaaaa aaaaaaaaaa aaa 1657<210> 2 <211> 1657 <212> DNA <213> Glycine max <220> <221> CDS <222> 22..1482 <400> 2 aaaattaaaa tctgaaaaac a atg gcg gcg aag cta gac acc cac gcc gtg 51 Met Ala Ala Lys Leu Asp Thr His Ala Val 1 5 10 gct tcc gat ctg atc gac ttc ctc aac gct tct cca acg gct ttc cac 99 Ala Ser Asp Leu Ile Asp Phe Leu Asn Ala Ser Pro Thr Ala Phe His 15 20 25 gcc gtc gac gag gca aag agg cgt ttg cgt agc gcg ggg tac cac caa 147 Ala Val Asp Glu Ala Lys Arg Arg Leu Arg Ser Ala Gly Tyr His Gln 30 35 40 ctc tct gag agg gaa gtg tgg gag ccg caa g aag tac ttc 195 Leu Ser Glu Arg Glu Val Trp Glu Leu Gln Pro Gly Asn Lys Tyr Phe 45 50 55 ttc acc aga aat cac tcc acc atc gtc gcc ttc gcc atc ggc aaa aag 243 Phe Thr Arg Asn His Ser Thr Ile Val Ala Phe Ala Ile Gly Lys Lys 60 65 70 tac gtt gct gga aat gga ttc tac ata att ggg gct cac acg gat agt 291 Tyr Val Ala Gly Asn Gly Phe Tyr Ile Ile Gly Ala His Thr Thr Asp Ser 75 80 85 90 cct tgt ctc aaa ctc aag cct gtc acc aag gtt gtt aag gct ggg att 339 Pro C ys Leu Lys Leu Lys Pro Val Thr Lys Val Val Lys Ala Gly Ile 95 100 105 ttg gag gtt ggt gtc caa acc tat gga ggt ggt ctg tgg cac aca tgg 387 Leu Glu Val Gly Val Gln Thr Tyr Gly Gly Gly Leu Trp His Thr Trp 110 115 120 ttt gat cga gac ttg act gtg gcg ggg agg gtc atc gtg cgg gaa gag 435 Phe Asp Arg Asp Leu Thr Val Ala Gly Arg Val Ile Val Arg Glu Glu 125 130 135 aat gct ggt tct gtt tcg tac tca cat cgc ctt gtt aga att gag gaa 483 Asn Ala Gly Ser Val Ser Tyr Ser His Arg Leu Val Arg Ile Glu Glu 140 145 150 cct ata atg cga ata ccg act ttg gca att cac ttg gac aag act gtt 531 Pro Ile Met Arg Ile Pro Thr Leu Ala Ile His Leu Asp Lys Thr Val 155 160 165 170 aat gat gga ttc aaa ttt aac aac gag aat cac ctt att ccc atc ttg 579 Asn Asp Gly Phe Lys Phe Asn Asn Glu Asn His Leu Ile Pro Ile Leu 175 180 185 gca aca tcg ctg aag ggt gag ctc aat aaa gtg tcc tct gaa aat ggt 627 Ala Thr Ser Leu Lys Gly Glu Leu Asn Lys Val Ser Ser Glu Asn Gly 190 195 200 cct gtt gaa agt gga aat cag acc gat gga aat aaa gca aat g aa a 675 Pro Val Glu Ser Gly Asn Gln Thr Asp Gly Lys Lys Ala Asn Asp Lys 205 210 215 aca ggc acc agc aat acg aag cat cac ctt ctt ctt cta cag ttg ctt 723 Thr Gly Thr Ser Asn Thr Lys His His Leu Leu Leu Leu Gln Leu Leu 220 225 230 gca agc aag ctt ggg tgt gaa cca gat gac ata tgt gat ttt gaa ttg 771 Ala Ser Lys Leu Gly Cys Glu Pro Asp Asp Ile Cys Asp Phe Glu Leu 235 240 245 250 caa gct tgc gat aca ca cca agt act att gct gga gct gca aag gaa 819 Gln Ala Cys Asp Thr Gln Pro Ser Thr Ile Ala Gly Ala Ala Lys Glu 255 260 265 ttc att ttt tca gga cgg ctt gat aat ctc tgc atg tca ttt tgc tcg 867 Phe Ile Ser Gly Arg Leu Asp Asn Leu Cys Met Ser Phe Cys Ser 270 275 280 ctg aag gca tta ata gat gct aca tct tct gac agc agt ctt gag gaa 915 Leu Lys Ala Leu Ile Asp Ala Thr Ser Ser Asp Ser Ser Leu Glu Glu 285 290 295 gag tca ggt gtt aga atg gtg gct tta ttt gac cat gag gaa gtt gga 963 Glu Ser Gly Val Arg Met Val Ala Leu Phe Asp His Glu Glu Val Gly 300 305 310 tct aac tct gcc caa gga gct ggc tct cct gtt atg ct a aat gct gtg 1011 Ser Asn Ser Ala Gln Gly Ala Gly Ser Pro Val Met Leu Asn Ala Val 315 320 325 330 act agg gtt acc aat tcc ttc agc tcc aat ccc aac ctt ctg gag aaa 1059 Thr Arg Val Thr Asn Ser Phe Ser Ser Asn Pro Asn Leu Leu Glu Lys 335 340 345 gca gca caa tta agc tac ctt gta tct gcc gac atg gca cat gca cta 1107 Ala Ala Gln Leu Ser Tyr Leu Val Ser Ala Asp Met Ala His Ala Leu 350 355 360 cac cca aat tac atg gac aag cat gaa gca aac cat cag ccc aaa cta 1155 His Pro Asn Tyr Met Asp Lys His Glu Ala Asn His Gln Pro Lys Leu 365 370 375 cat gga gga ctt gtc att aaa acc aat gca agc caa cgc tat gca acc 1203 His Gly Gly Leu Val Ile Lys Thr Asn Ala Ser Gln Arg Tyr Ala Thr 380 385 390 aat gtt gtc aca tcc ttc ata ttc agg gag ata gca tca aaa cat aaa 1251 Asn Val Val Thr Ser Ser Phe Ile Phe Arg Glu Ile Ala Ser Lys His Lys 395 400 405 410 ctt ccc gtt cag gac ttt gtg gtg cgc aat gac atg tca tgt ggt tca 1299 Leu Pro Val Gln Asp Phe Val Val Arg Asn Asp Met Ser Cys Gly Ser 415 420 425 acc att ggt cct att ctt gct agt ggc gta ggt att cgc act gtt gat 1347 Thr Ile Gly Pro Ile Leu Ala Ser Gly Val Gly Ile Arg Thr Val Asp 430 435 440 gta ggt gca ccg cag ttg tca atg cat agc ata cga gaa att tgt gct 1395 Val Gly Ala Pro Gln Leu Ser Met His Ser Ile Arg Glu Ile Cys Ala 445 450 455 gtt gat gat gtg aag tat tca tat gag cac ttc aaa gca ttt tac caa 1443 Val Asp Asp Val Lys Tyr Ser Tyr Glu His Phe Lys Ala Phe Tyr Gln 460 465 470 gaa ttc tct cat gtt gat ggt aag atg gtc gtg gat ata tag gaatatctc 1494 Glu Phe Ser His Val Asp Gly Lys Met Val Val Asp Ile 475 480 485 taatcacgaa atcctcatta atcctttgct ctagaagctg ttgctgaaat ggtcgtgttt 1554 cgtaatttag taccattata atgccgacgt tattatgatg aaattttcaa taaaattaga 1614 ctccctgaat gaaatattag caactaaaaa aaaaaaaaaa aaa 1657

【0069】 <210> 3 <211> 357 <212> DNA <213> Artificial Sequence <220> <221> promoter <222> 0..357 <400> 3 cgcccaatac gcaaaccgcc tctccccgcg cgttggccgc ttcattaatg cagctggcac 60 gacaggtttc ccgactggaa agcgggcagt gagcgcaacg caattaatgt gagttagctc 120 actcattagg caccccaggc tttacacttt atgcttccgg atcgtatgtt gtgtggaatt 180 gtgagcggat aacaatttca cacaggaaac agctatgacc atgattacgc caagcttgca 240 tgcctgcagg tcgccctttc gtcttcaaga attcccctgt tgacaattaa tcatcgaact 300 agttaactag tacgcaagtt cacgtaaaaa gggtatcgat tagtaaggag gtttaaa 357<210> 3 <211> 357 <212> DNA <213> Artificial Sequence <220> <221> promoter <222> 0..357 <400> gagttagctc 120 actcattagg caccccaggc tttacacttt atgcttccgg atcgtatgtt gtgtggaatt 180 gtgagcggat aacaatttca cacaggaaac agctatgacc atgattacgc caagcttgca 240 tgcctgcagg tcgcctag tag cctca tg tga tg tca tca tg tg tga tg tga tg tga tg

【0070】 <210> 4 <211> 20 <212> PRT <213> Glycine max <400> 4 Ser Ala Gly Tyr His Gln Leu Ser Glu Arg Glu Val Trp Glu Leu Gln Pro Gly 1 5 10 15 Asn Lys 20<210> 4 <211> 20 <212> PRT <213> Glycine max <400> 4 Ser Ala Gly Tyr His Gln Leu Ser Glu Arg Glu Val Trp Glu Leu Gln Pro Gly 1 5 10 15 Asn Lys 20

【0071】 <210> 5 <211> 25 <212> DNA <213> Artificial Sequence <220> <223> Description of Artificial Sequence : primer <400> 5 ctacacctga ctcatcgatc cacta 25<210> 5 <211> 25 <212> DNA <213> Artificial Sequence <220> <223> Description of Artificial Sequence: primer <400> 5 ctacacctga ctcatcgatc cacta 25

【0072】 <210> 6 <211> 25 <212> DNA <213> Artificial Sequence <220> <223> Description of Artificial Sequence : primer <400> 6 caggcttgag cttcagggat ggact 25<210> 6 <211> 25 <212> DNA <213> Artificial Sequence <220> <223> Description of Artificial Sequence: primer <400> 6 caggcttgag cttcagggat ggact 25

【0073】 <210> 7 <211> 20 <212> DNA <213> Artificial Sequence <220> <223> Description of Artificial Sequence : primer <400> 7 cgcccaatac gcaaaccgcc 20<210> 7 <211> 20 <212> DNA <213> Artificial Sequence <220> <223> Description of Artificial Sequence: primer <400> 7 cgcccaatac gcaaaccgcc 20

【0074】 <210> 8 <211> 27 <212> DNA <213> Artificial Sequence <220> <223> Description of Artificial Sequence : primer <400> 8 tttaaacctc cttactaatc gataccc 27<210> 8 <211> 27 <212> DNA <213> Artificial Sequence <220> <223> Description of Artificial Sequence: primer <400> 8 tttaaacctc cttactaatc gataccc 27

【0075】 <210> 9 <211> 32 <212> DNA <213> Artificial Sequence <220> <223> Description of Artificial Sequence : primer <400> 9 ggaggtttaa aatggcggcg aagctagaca cc 32<210> 9 <211> 32 <212> DNA <213> Artificial Sequence <220> <223> Description of Artificial Sequence: primer <400> 9 ggaggtttaa aatggcggcg aagctagaca cc 32

【0076】 <210> 10 <211> 21 <212> DNA <213> Artificial Sequence <220> <223> Description of Artificial Sequence : primer <400> 10 gttgcagttc ccacaattcc c 21<210> 10 <211> 21 <212> DNA <213> Artificial Sequence <220> <223> Description of Artificial Sequence: primer <400> 10 gttgcagttc ccacaattcc c 21

【0077】 <210> 11 <211> 32 <212> DNA <213> Artificial Sequence <220> <223> Description of Artificial Sequence : primer <400> 11 ggaggtttaa aatggctgct aaactggaca cc 32<210> 11 <211> 32 <212> DNA <213> Artificial Sequence <220> <223> Description of Artificial Sequence: primer <400> 11 ggaggtttaa aatggctgct aaactggaca cc 32

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

【図1】 プラスミドpUCTRPGXN1-8の構築図である。FIG. 1 is a diagram showing the construction of plasmid pUCTRPGXN1-8.

【図2】 GX発現プラスミドpUCTRPGX1-8の構築図で
ある。FIG. 2 is a construction diagram of a GX expression plasmid pUCTRPGX1-8.

【図3】 プラスミドpUCTRPGXN2-1の構築図である。FIG. 3 is a construction diagram of plasmid pUCTRPGXN2-1.

【図4】 GX発現プラスミドpUCTRPGX2-1の構築図で
ある。FIG. 4 is a construction diagram of a GX expression plasmid pUCTRPGX2-1.

フロントページの続き (51)Int.Cl.7 識別記号 FI テーマコート゛(参考) C12N 9/48 A23L 1/238 101D // A23L 1/238 101 C12N 5/00 A (72)発明者 浅野 皆夫 神奈川県川崎市川崎区鈴木町1−1 味の 素株式会社食品総合研究所内 (72)発明者 中村 奈巳 神奈川県川崎市川崎区鈴木町1−1 味の 素株式会社食品総合研究所内 (72)発明者 丹尾 式希 神奈川県川崎市川崎区鈴木町1−1 味の 素株式会社食品総合研究所内 Fターム(参考) 4B024 AA05 BA14 CA04 DA06 EA04 GA11 GA19 HA01 HA12 4B039 LC06 LG26 4B050 CC03 DD13 FF13E LL02 4B065 AA26X AA88Y AB01 AC14 BA02 BA25 BB28 CA33 CA42Continued on the front page (51) Int.Cl. 7 Identification symbol FI Theme coat II (reference) C12N 9/48 A23L 1/238 101D // A23L 1/238 101 C12N 5/00 A (72) Inventor Minao Asano Kanagawa 1-1, Suzuki-cho, Kawasaki-ku, Kawasaki-ku, Ajinomoto Co., Ltd. (72) Inventor Nami Nakamura 1-1, Suzuki-cho, Kawasaki-ku, Kawasaki, Kanagawa, Japan Ajinomoto Co., Ltd. (72) Invention Participant Shiki Tanio 1-1, Suzukicho, Kawasaki-ku, Kawasaki-shi, Kanagawa Prefecture F-term in Ajinomoto Co., Inc.Food Research Institute (reference) AB01 AC14 BA02 BA25 BB28 CA33 CA42

Claims (6)

【特許請求の範囲】[Claims] 【請求項1】 配列表配列番号1に記載されるアミノ酸
配列を有する発芽ダイズ子葉由来の新規アミノペプチダ
ーゼをコードするDNA。1. A DNA encoding a novel aminopeptidase derived from germinated soybean cotyledons having the amino acid sequence set forth in SEQ ID NO: 1 in the sequence listing. 【請求項2】 配列表配列番号1に記載されるアミノ酸
配列に於いて、1もしくは複数のアミノ酸残基が挿入、
付加、欠失もしくは置換されたアミノ酸配列を有し、か
つ、アミノペプチダーゼを活性を有するタンパク質をコ
ードするDNA。2. An amino acid sequence represented by SEQ ID NO: 1 in which one or more amino acid residues are inserted,
A DNA which has an added, deleted or substituted amino acid sequence and encodes a protein having aminopeptidase activity. 【請求項3】 配列表配列番号2に記載される塩基配列
のうち、塩基番号22から1482の塩基配列を有する請求項
1に記載のDNA。3. The DNA according to claim 1, which has a base sequence from base numbers 22 to 1482 in the base sequence shown in SEQ ID NO: 2 in the sequence listing. 【請求項4】 請求項1〜3のいずれかに記載のDNA
を含有する組換えDNA。4. The DNA according to any one of claims 1 to 3,
A recombinant DNA containing 【請求項5】 請求項4に記載の組換えDNAで形質転
換された形質転換体。A transformant transformed with the recombinant DNA according to claim 4. 【請求項6】 請求項5に記載の形質転換体を培養し、
アミノペプチダーゼ活性を有するタンパク質を生産さ
せ、これを回収することを特徴とするアミノペプチダー
ゼ活性を有するタンパク質の製造方法。6. culturing the transformant according to claim 5,
A method for producing a protein having an aminopeptidase activity, comprising producing a protein having an aminopeptidase activity and recovering the protein.
JP2000071879A 1999-03-15 2000-03-15 Dna encoding new aminopeptidase and method for producing the aminopeptidase Pending JP2000325090A (en)

Priority Applications (1)

Application Number Priority Date Filing Date Title
JP2000071879A JP2000325090A (en) 1999-03-15 2000-03-15 Dna encoding new aminopeptidase and method for producing the aminopeptidase

Applications Claiming Priority (3)

Application Number Priority Date Filing Date Title
JP6825599 1999-03-15
JP11-68255 1999-03-15
JP2000071879A JP2000325090A (en) 1999-03-15 2000-03-15 Dna encoding new aminopeptidase and method for producing the aminopeptidase

Publications (1)

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JP2000325090A true JP2000325090A (en) 2000-11-28

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ID=26409476

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Country Link
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Cited By (3)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
WO2004105503A1 (en) 2003-05-27 2004-12-09 Ajinomoto Co., Inc. Method of improving taste and/or flavor of food or drink
US7087422B2 (en) 2001-03-19 2006-08-08 Ajinomoto Co., Inc. Aminopeptidase and the genes thereof
JP2009521943A (en) * 2006-01-04 2009-06-11 ノボザイムス アクティーゼルスカブ Soy sauce production method

Cited By (5)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US7087422B2 (en) 2001-03-19 2006-08-08 Ajinomoto Co., Inc. Aminopeptidase and the genes thereof
WO2004105503A1 (en) 2003-05-27 2004-12-09 Ajinomoto Co., Inc. Method of improving taste and/or flavor of food or drink
JPWO2004105503A1 (en) * 2003-05-27 2006-07-20 味の素株式会社 Method for improving taste and / or flavor of food and drink
JP4529183B2 (en) * 2003-05-27 2010-08-25 味の素株式会社 Method for improving taste and / or flavor of food and drink
JP2009521943A (en) * 2006-01-04 2009-06-11 ノボザイムス アクティーゼルスカブ Soy sauce production method

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