JP2003325130A - Method for producing yeast extract - Google Patents

Method for producing yeast extract

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Publication number
JP2003325130A
JP2003325130A JP2002138431A JP2002138431A JP2003325130A JP 2003325130 A JP2003325130 A JP 2003325130A JP 2002138431 A JP2002138431 A JP 2002138431A JP 2002138431 A JP2002138431 A JP 2002138431A JP 2003325130 A JP2003325130 A JP 2003325130A
Authority
JP
Japan
Prior art keywords
enzyme
treated product
yeast
product
derived
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
JP2002138431A
Other languages
Japanese (ja)
Inventor
Yoshihiro Kawabata
兆宏 川端
Rie Kawaguchi
理衣 川口
Tsuyoshi Komai
強 駒井
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.)
T Hasegawa Co Ltd
Original Assignee
T Hasegawa 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 T Hasegawa Co Ltd filed Critical T Hasegawa Co Ltd
Priority to JP2002138431A priority Critical patent/JP2003325130A/en
Publication of JP2003325130A publication Critical patent/JP2003325130A/en
Pending legal-status Critical Current

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Abstract

<P>PROBLEM TO BE SOLVED: To provide a yeast extract having high deliciousness, thickness and saltiness, improved seasoning property and decreased yeast smell. <P>SOLUTION: The yeast extract is produced by treating yeast cells under high pressure, treating with an endo-type protease and then treating with an exo-type protease. <P>COPYRIGHT: (C)2004,JPO

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】本発明は酵母エキスの製造方
法に関し、更に詳しくは旨味、コク味、塩味が強く、呈
味性が改善され、さらに酵母臭の低減された酵母エキス
の製造方法に関する。BACKGROUND OF THE INVENTION 1. Field of the Invention The present invention relates to a method for producing a yeast extract, and more particularly to a method for producing a yeast extract having a strong umami, rich and salty taste, improved taste and further reduced yeast odor.

【0002】[0002]

【従来の技術】酵母エキスは天然調味料として、近年、
肉エキス、野菜エキス、魚介類エキス等とともに、化学
調味料にはない複雑な呈味性、すなわち、旨味、酸味、
苦味、コク味等を有しており、食品素材として広く利用
されている。2. Description of the Related Art Yeast extract has recently been used as a natural seasoning.
Along with meat extract, vegetable extract, seafood extract, etc., complex tastes that chemical seasonings do not have, that is, umami, sourness,
It has bitterness and richness and is widely used as a food material.

【0003】従来、酵母エキスの製造方法としては、自
己消化法、熱水抽出法等による天然分解法や、酵素分解
法、酸・アルカリや塩類等による化学的分解法等がある
が、呈味性の増強や、酵母臭の低減を目的として種々の
提案がなされており、例えば、酵母菌体に3000Kg
/cm2程度以上の超高圧を加えて酵母菌体よりエキス
分を抽出する方法(特開平2−255059号公報)、
酵母の細胞壁を機械的に破砕し、該酵母内の成分を抽出
する方法(特開平5−252894号公報)、細胞壁溶
解酵素を併用させて自己消化を行わせた後に加熱し、菌
体内酵素を失活後、5’−ホスホジエステラーゼ、5’
−アデニル酸デアミナーゼを作用させ、呈味性5’−ヌ
クレオチド含量・遊離アミノ酸含量を共に高める方法
(特開平6−70716号公報)、高圧ホモジナイザー
処理した酵母菌体懸濁液をpH6.5〜8.5の中性〜
弱アルカリ性に調整し、該酵母菌体懸濁液にエンド型プ
ロテアーゼを含む酵素剤を添加し、自己消化させる方法
(特開平9−56361号公報)、自己消化法により酵
母エキスを製造するにあたり、2段階の酵素反応温度条
件を採用して製造する方法(特開平10−179084
号公報)、酵母の水懸濁液を90〜95℃にて30〜6
0分加熱処理した後、40〜70℃にて溶菌酵素、ヌク
レアーゼ、デアミナーゼ及び酵母乾物量に対して1重量
%以上のプロテアーゼからなる酵素を同時に反応させる
方法(特開平10−262605号公報)などが提案さ
れている。Conventionally, as a method for producing a yeast extract, there are a natural decomposition method such as an autolysis method and a hot water extraction method, an enzymatic decomposition method, and a chemical decomposition method such as an acid / alkali or a salt. Various proposals have been made for the purpose of enhancing sexuality and reducing yeast odor.
A method of extracting an extract from the yeast cells by applying an ultrahigh pressure of about / cm 2 or more (JP-A-2-255059),
A method of mechanically crushing the cell wall of yeast and extracting components in the yeast (Japanese Patent Laid-Open No. 252894/1993), autolysis using cell wall lysing enzyme in combination, followed by heating to remove intracellular enzyme After inactivation, 5'-phosphodiesterase, 5 '
-A method of increasing the taste 5'-nucleotide content and the free amino acid content by allowing adenylate deaminase to act (JP-A-6-70716), and a yeast cell suspension treated with a high-pressure homogenizer at pH 6.5 to 8 .5 neutrality ~
A method of adjusting to weakly alkaline, adding an enzyme agent containing an endo-type protease to the yeast cell suspension, and performing self-digestion (JP-A-9-56361), in producing a yeast extract by the self-digestion method, A method of production using two-step enzyme reaction temperature conditions (Japanese Patent Application Laid-Open No. 10-179084).
Gazette), an aqueous suspension of yeast at 90 to 95 ° C. for 30 to 6
After 0 minute heat treatment, a method of simultaneously reacting a lysing enzyme, a nuclease, a deaminase, and an enzyme composed of 1% by weight or more of protease with respect to the dry matter of yeast at 40 to 70 ° C. (JP-A-10-262605) Is proposed.

【0004】[0004]

【発明が解決しようとする課題】従来提案されている上
述した方法はそれなりの効果はあるが、酵母エキスの呈
味性の増強や酵母臭の低減の点では十分満足できるもの
ではなかった。Although the above-mentioned methods proposed hitherto have some effects, they are not sufficiently satisfactory in terms of enhancing the taste of yeast extract and reducing yeast odor.

【0005】従って、本発明の目的は、旨味やコク味さ
らに塩味が強く、呈味性が改善され、さらに酵母臭の低
減された酵母エキスの製造方法を提供することである。[0005] Therefore, an object of the present invention is to provide a method for producing a yeast extract having a strong umami, a full-bodied taste, a strong salty taste, an improved taste and a reduced yeast odor.

【0006】[0006]

【課題を解決するための手段】本発明者らは上記のごと
き課題を解決すべく、鋭意研究を行った結果、今回、酵
母菌体を高圧処理した後、エンド型プロテアーゼで処理
し、次いでエキソ型プロテアーゼを作用させることによ
り、旨味やコク味が強く、呈味性が改善され、さらに酵
母臭の低減された酵母エキスが得られることを見出し本
発明を完成するに至った。Means for Solving the Problems As a result of intensive studies to solve the above problems, the present inventors have found that this time, yeast cells were treated with high pressure, treated with endo-type protease, and then exogenous. It has been found that a yeast extract having a strong umami and rich taste, improved taste and reduced yeast odor can be obtained by the action of a type protease, and the present invention has been completed.

【0007】かくして、本発明によれば、酵母菌体を、
例えば、0〜0.8MPaの範囲内で高圧処理した後、
エンド型プロテアーゼで処理し、次いでエキソ型プロテ
アーゼを作用させることを特徴とする酵母エキスの製造
方法が提供される。Thus, according to the present invention, yeast cells are
For example, after high-pressure treatment within the range of 0 to 0.8 MPa,
There is provided a method for producing a yeast extract, which comprises treating with an endo-type protease and then allowing the exo-type protease to act.

【0008】以下、本発明について更に詳細に説明す
る。The present invention will be described in more detail below.

【0009】[0009]

【発明の実施の形態】本発明に用いられる酵母は、可食
性のものであれば特に制限はなく、例えば、パン酵母、
ビール酵母、アルコール酵母、清酒用酵母など通常の食
品工業に用いられているものを単独または組合せで任意
に使用することができる。このような酵母の例として
は、サッカロミセス属、キャンディダ属等に属する酵母
などを例示することができる。BEST MODE FOR CARRYING OUT THE INVENTION The yeast used in the present invention is not particularly limited as long as it is edible, for example, baker's yeast,
What is used in normal food industry, such as brewer's yeast, alcohol yeast, and sake yeast, can be used alone or in combination. Examples of such yeasts include yeasts belonging to the genera Saccharomyces and Candida.

【0010】本発明の酵母エキスの製造方法は、上述し
た酵母菌体を高圧処理した後、エンド型プロテアーゼで
処理し、次いでエキソ型プロテアーゼを作用させること
を特徴とする。The method for producing a yeast extract of the present invention is characterized in that the above-mentioned yeast cells are subjected to a high pressure treatment, then treated with an endo-type protease, and then treated with an exo-type protease.

【0011】まず、酵母菌体を高圧処理する方法につい
て説明する。例えば、酵母菌体1重量部に対して水0.
8〜2.0重量部を添加し、オートクレーブなどの適宜
な加圧装置に充填して高圧処理する。高圧処理の条件と
しては、例えば、0〜0.8MPa、好ましくは0.1
〜0.2MPaの範囲内の圧力で、100〜180℃、
好ましくは100〜120℃の温度条件下に、5〜30
分、好ましくは15〜20分の条件を例示することがで
きる。高圧処理することにより細胞内のタンパク質、核
酸等のエキス分を抽出しやすることができ、後述するプ
ロテアーゼ処理の効率を高めることができる。First, a method for high-pressure treatment of yeast cells will be described. For example, water of 0.
8 to 2.0 parts by weight is added, and the mixture is filled in an appropriate pressure device such as an autoclave and subjected to high pressure treatment. The conditions for the high pressure treatment are, for example, 0 to 0.8 MPa, preferably 0.1
At a pressure in the range of ~ 0.2 MPa, 100-180 ° C,
Preferably, 5 to 30 under a temperature condition of 100 to 120 ° C.
Minutes, preferably 15 to 20 minutes. By performing the high-pressure treatment, the extract components such as intracellular proteins and nucleic acids can be easily extracted, and the efficiency of the protease treatment described below can be increased.

【0012】次いで、この高圧処理物をエンド型プロテ
アーゼで処理する。本発明で使用することができるエン
ド型プロテアーゼとしては、特に制限されず動植物由
来、微生物由来のエンド型プロテアーゼを少なくとも1
種類以上使用することができ、例えば、細菌由来のサー
モライシン、麹菌由来のデューテロライシン、放線菌由
来の中性プロテアーゼ、植物由来のパパイン、ブロメラ
イン、動物由来のトリプシン、ペプシン、カテプシン類
などを挙げることができる。具体的には、例えば、プロ
テアーゼN(アマノエンザイム社製)、ニュートラーゼ
(ノボノルディスクバイオインダストリー社製)、オリ
エンターゼ10NL(エイチビィアイ社製)などの細菌
由来のサーモライシン;スミチームFP(新日本化学工
業社製)、オリエンターゼONS(エイチビィアイ社
製)、プロテアーゼM(アマノエンザイム社製)などの
麹菌由来のデューテロライシン;アクチナーゼAS(科
研ファルマ社製)などの放線菌由来中性プロテアーゼ;
パパインW−40(アマノエンザイム社製)、ブロメラ
イン(日本バイオコン社製)などの植物由来の中性プロ
テアーゼ;トリプシンPTN(ノボノルディスクバイオ
インダストリー社製)、ペプシン(日本バイオコン社
製)などの動物由来のプロテアーゼ;イカ肝臓由来カテ
プシンDなどのカテプシン類を挙げることができる。Next, this high-pressure treated product is treated with endo-type protease. The endo-type protease that can be used in the present invention is not particularly limited, and at least one endo-type protease derived from plants and animals and derived from microorganisms is used.
More than one kind can be used, for example, bacteria-derived thermolysin, koji mold-derived deuterolysin, actinomycete-derived neutral protease, plant-derived papain, bromelain, animal-derived trypsin, pepsin, cathepsins and the like. You can Specifically, for example, bacterial-derived thermolysin such as Protease N (manufactured by Amano Enzyme), Neutrase (manufactured by Novo Nordisk Bioindustry), Orientase 10NL (manufactured by HBII); Sumiteam FP (Nippon Kagaku Kogyo) Deuterolysin derived from Aspergillus oryzae such as orientase ONS (manufactured by HBI) or Protease M (manufactured by Amano Enzyme); actinase AS (manufactured by Kaken Pharma) or other neutral protease derived from actinomycetes;
Plant-derived neutral proteases such as papain W-40 (manufactured by Amano Enzyme) and bromelain (manufactured by Nippon Biocon); animal origins such as trypsin PTN (manufactured by Novo Nordisk Bioindustry) and pepsin (manufactured by Nippon Biocon) Proteases; cathepsin such as squid liver-derived cathepsin D.

【0013】エンド型プロテアーゼの使用量は、力価な
どにより一概には言えないが、例えば、酵母菌体の重量
を基準として0.1〜100U/gの範囲を例示するこ
とができる。The amount of the endo-type protease to be used cannot be generally stated depending on the titer and the like, but for example, it can be exemplified in the range of 0.1 to 100 U / g based on the weight of the yeast.

【0014】エンド型プロテアーゼによる処理条件は、
特に制限されず使用する酵素の至適条件に合わせて行う
ことができるが、通常、例えば、4〜8のpHの範囲に
調整し、25〜70℃の温度範囲で、1〜24時間処理
する方法を例示することができる。The treatment conditions with endo-type protease are as follows:
It is not particularly limited and can be carried out in accordance with the optimum conditions of the enzyme to be used, but it is usually adjusted to a pH range of 4 to 8 and treated at a temperature range of 25 to 70 ° C. for 1 to 24 hours. The method may be illustrated.

【0015】本発明では、上述したエンド型プロテアー
ゼで処理した後、該処理物をさらにエキソ型プロテアー
ゼで処理する。本発明で使用することができるエキソ型
プロテアーゼとしては、特に制限されず動植物由来、微
生物由来のエキソ型プロテアーゼを少なくとも1種類以
上使用することができ、例えば、麹菌由来の酸性カルボ
キシペプチダーゼ、酵母由来の酸性カルボキシペプチダ
ーゼ、イカ肝臓由来のカルボキシペプチダーゼ、小麦由
来のカルボキシペプチダーゼ、および麹菌由来のアミノ
ペプチダーゼ、細菌由来のアミノペプチダーゼ、マイタ
ケ由来のアミノペプチダーゼなどを挙げることができ
る。具体的には、例えば、カルボキシペプチダーゼP
(シグマアルドリッチ社製)、スミチームFLPA(新
日本化学工業社製)、プロテアーゼM(アマノエンザイ
ム社製)などの麹菌由来の酸性カルボキシペプチダー
ゼ;カルボキシペプチダーゼY(シグマアルドリッチ社
製)などの酵母由来の酸性カルボキシペプチダーゼ;イ
カ肝臓カルボキシペプチダーゼなどの動物由来の酸性カ
ルボキシペプチダーゼ;カルボキシペプチダーゼW(ぺ
んてる社製)、マイタケ由来アミノペプチダーゼなどの
植物由来の酸性ペプチダーゼ;サカナーゼ(科研ファル
マ社製)などの麹菌由来のアミノペプチダーゼ;アクセ
ラーゼ(萬有通商社製)などの細菌由来のアミノペプチ
ダーゼなどを例示することができる。In the present invention, after treated with the above-mentioned endo-type protease, the treated product is further treated with an exo-type protease. The exo-type protease that can be used in the present invention is not particularly limited, and at least one or more animal- or plant-derived exo-type proteases derived from microorganisms can be used. For example, acid carboxypeptidase derived from koji mold, yeast-derived Examples thereof include acid carboxypeptidase, squid liver-derived carboxypeptidase, wheat-derived carboxypeptidase, and koji mold-derived aminopeptidase, bacterial-derived aminopeptidase, maitake-derived aminopeptidase, and the like. Specifically, for example, carboxypeptidase P
(Manufactured by Sigma-Aldrich), Sumiteam FLPA (manufactured by Shin Nippon Chemical Industry Co., Ltd.), protease M (manufactured by Amano Enzyme) and other acidic carboxypeptidases derived from koji mold; carboxypeptidase Y (manufactured by Sigma-Aldrich) and other yeast-derived acidic Carboxypeptidase; animal-derived acidic carboxypeptidase such as squid liver carboxypeptidase; plant-derived acidic peptidase such as carboxypeptidase W (manufactured by Pentel), maitake-derived aminopeptidase; amino acid derived from Aspergillus oryzae such as sacanase (manufactured by Kaken Pharma Co.) Examples thereof include peptidases; aminopeptidases derived from bacteria such as accelerators (manufactured by Manyutsusho Co., Ltd.).

【0016】エキソ型プロテアーゼの使用量は、力価な
どにより一概には言えないが、例えば、酵母菌体の重量
を基準として0.1〜100U/gの範囲を例示するこ
とができる。The amount of exo-type protease used cannot be generally determined depending on the titer and the like, but for example, it can be exemplified in the range of 0.1 to 100 U / g based on the weight of yeast cells.

【0017】エキソ型プロテアーゼによる処理条件は、
特に制限されず使用する酵素の至適条件に合わせて行う
ことができるが、通常、例えば、カルボキシペプチダー
ゼであれば、2.5〜5のpHの範囲に調整し、又、ア
ミノペプチダーゼであれば、6〜8.5のpHの範囲に
調整し、20〜60℃の温度範囲で、1〜24時間処理
する方法を例示することができる。The treatment conditions with exo-type protease are as follows:
It is not particularly limited and can be carried out in accordance with the optimum conditions of the enzyme to be used, but usually, for example, in the case of carboxypeptidase, it is adjusted to a pH range of 2.5 to 5, and in the case of aminopeptidase, , A pH range of 6 to 8.5, and a temperature range of 20 to 60 ° C. for 1 to 24 hours.

【0018】本発明の一実施態様を例示すれば、酵母菌
体1重量部に水0.8〜2.0重量部を添加して、約
0.1〜約0.2MPaの圧力条件下、約100〜約1
20℃で約10〜約20分間高圧処理した後冷却し、上
述のエンド型プロテアーゼを添加して、約30〜約60
℃で約60分〜約24時間酵素処理を行う。酵素処理
後、pHを2.5〜5.0に調整した後、上述のエキソ
型プロテアーゼを添加して、約20〜約60℃で約60
分〜約24時間酵素処理を行う。酵素処理後、pHを調
製し、約90〜約100℃で約5〜約20分間酵素失活
した後冷却し、遠心分離、濾紙濾過等の適宜な分離手段
を採用して分離することにより清澄な酵母エキスを得る
ことができる。得られた酵母エキスは所望により適宜な
濃縮手段を採用して濃縮液の形態とすることもできる。
本発明の酵母エキスは、通常そのまま液状で利用する
が、所望により該エキスにデキストリン、加工澱粉、サ
イクロデキストリン、アラビアガム等の賦形剤を添加し
て粉末状とすることもできる。As an example of one embodiment of the present invention, 0.8 to 2.0 parts by weight of water is added to 1 part by weight of yeast cells, and a pressure condition of about 0.1 to about 0.2 MPa is applied. About 100 to about 1
After high-pressure treatment at 20 ° C. for about 10 to about 20 minutes, the mixture is cooled, and the above-mentioned endoprotease is added to about 30 to about 60.
Enzyme treatment is performed at 60 ° C. for about 60 minutes to about 24 hours. After the enzyme treatment, the pH is adjusted to 2.5 to 5.0, and then the above-mentioned exo-type protease is added, and the pH is adjusted to about 60 at about 20 to about 60 ° C.
The enzyme treatment is performed for about 24 minutes to about 24 hours. After the enzyme treatment, the pH is adjusted, the enzyme is inactivated at about 90 to about 100 ° C. for about 5 to about 20 minutes, then cooled, and clarified by separating using an appropriate separating means such as centrifugation or filter paper filtration. The yeast extract can be obtained. The obtained yeast extract may be in the form of a concentrated liquid by adopting an appropriate concentration means, if desired.
The yeast extract of the present invention is usually used in a liquid state as it is, but if desired, an excipient such as dextrin, modified starch, cyclodextrin, gum arabic or the like may be added to the extract to give a powder form.

【0019】以下、本発明を実施例および比較例により
具体的に説明する。Hereinafter, the present invention will be specifically described with reference to Examples and Comparative Examples.

【0020】[0020]

【実施例】実施例1 酵母菌体100gに対し、200gの水を加え懸濁した
後、オートクレーブにて120℃、0.2MPaにて、
15分間加温、加圧処理した(以下、加圧処理物Aと称
する)。この加圧処理Aを60℃まで冷却し、5000
u/gのオリエンターゼ90N(エイチビィアイ社製の
エンド型プロテアーゼ)10mgを添加し60℃におい
て5時間反応した(以下、酵素処理物Bと称する)。こ
の酵素処理物BのpHを0.1N塩酸にて4.0に調製
後、40℃にて50u/gのプロテアーゼM(アマノエ
ンザイム社製のエキソ型プロテアーゼ)0.05 gを添
加し、40℃において20時間反応した(以下、酵素処
理物Cと称する;本発明品1)。Example 1 To 100 g of yeast cells, 200 g of water was added and suspended, and then autoclaved at 120 ° C. and 0.2 MPa.
It was heated and pressure-treated for 15 minutes (hereinafter referred to as pressure-treated product A). This pressure treatment A is cooled to 60 ° C.
10 mg of orientase 90N (endo-type protease manufactured by HBI) was added at u / g and reacted at 60 ° C. for 5 hours (hereinafter referred to as enzyme-treated product B). The pH of this enzyme-treated product B was adjusted to 4.0 with 0.1N hydrochloric acid, and then 0.05 g of 50 u / g of protease M (exo-type protease manufactured by Amano Enzyme) was added at 40 ° C. to 40 The reaction was carried out at 0 ° C for 20 hours (hereinafter referred to as enzyme-treated product C; product 1 of the present invention).

【0021】(ゲルろ過曲線の比較)上記工程における加
圧処理物A、一段階目のエンド型プロテアーゼ処理後の
酵素処理物Bおよび二段階目のエキソ型プロテアーゼ処
理後の酵素処理物C(本発明品1)をSuperdex
peptide(アマシャムファルマシア社製)を用い
たゲルろ過クロマトグラフィーに供し、分子量分布を測
定した。図.1にクロマトグラムを示すが、加圧処理物
Aと酵素処理物Bでは分子量1000〜500Daのペ
プチドが多量に生成し、酵素処理物C(本発明品1)で
は分子量500Da以下のペプチド・アミノ酸が多量に
生成した。このことから酵母菌体を加圧処理すること
で、両方のプロテアーゼが作用し、多量の呈味成分が生
成することが確認された。(Comparison of Gel Filtration Curves) Pressurized product A in the above step, enzymatically processed product B after the first step endo-type protease treatment and enzymatically processed product C after the second step exo-type protease treatment (main Invention 1) is superdex
Peptide (manufactured by Amersham Pharmacia) was used for gel filtration chromatography to measure the molecular weight distribution. Fig. The chromatogram is shown in Fig. 1. In the pressure-treated product A and the enzyme-treated product B, a large amount of peptides having a molecular weight of 1000 to 500 Da is produced, and in the enzyme-treated product C (invention product 1), peptides / amino acids having a molecular weight of 500 Da or less are produced. Generated in large quantities. From this, it was confirmed that by pressurizing the yeast cells, both proteases act and a large amount of taste components are produced.

【0022】(遊離アミノ酸含量の比較)ニンヒドリン発
色法により、反応液中の遊離アミノ酸含量を測定した。
加圧処理物A、酵素処理物Bおよび酵素処理物C(本発
明品1)の結果を図.2に示すが、二段階の酵素反応に
より酵母菌体より遊離アミノ酸が多量に遊離することが
確認された。(Comparison of Free Amino Acid Content) The free amino acid content in the reaction solution was measured by the ninhydrin coloring method.
The results of pressure-treated product A, enzyme-treated product B, and enzyme-treated product C (invention product 1) are shown in FIG. As shown in Fig. 2, it was confirmed that a large amount of free amino acids was released from the yeast cells by the two-step enzymatic reaction.

【0023】(呈味、香気比較)加圧処理物A、酵素処理
物Bおよび酵素処理物C(本発明品1)の水可溶部を分
離し、5%溶液に希釈し専門パネラー10名により官能
評価を行った。その結果、専門パネラー10名全員が、
呈味、香気とも酵素処理物C(本発明品1)は、加圧処
理物Aおよび酵素処理物Bと比較し、非常に強い旨味、
こく味、塩味が感じられると評価した。(Comparison of taste and aroma) The water-soluble portion of the pressure-treated product A, the enzyme-treated product B and the enzyme-treated product C (product 1 of the present invention) was separated and diluted with a 5% solution to prepare 10 specialized panelists. The sensory evaluation was performed by. As a result, all 10 professional panelists
The enzyme-treated product C (invention product 1) in both taste and aroma has a very strong umami as compared with the pressure-treated product A and the enzyme-treated product B.
It was evaluated that a rich and salty taste was felt.

【0024】比較例1(実施例1において加圧処理を行
っていない例) 酵母菌体100gに対し、200gの水を加え懸濁した
後、60℃に加温した(以下、酵素未処理物Dと称す
る)。これに5000u/gのオリエンターゼ90N
(エイチビィアイ社製)10mgを添加し60℃におい
て5時間反応した。この反応液のpHを0.1N塩酸に
て4.0に調製後、40℃にて50u/gのプロテアー
ゼM(アマノエンザイム社製) 0.05 gを添加し、
40℃において20時間反応した(以下、酵素処理物E
と称する)。Comparative Example 1 (example in which pressure treatment was not carried out in Example 1) 200 g of water was added to 100 g of yeast cells and suspended, and then the suspension was heated to 60 ° C. (hereinafter, enzyme-untreated product). Called D). 5000u / g of Orientase 90N
10 mg (manufactured by HBI) was added and reacted at 60 ° C. for 5 hours. After adjusting the pH of this reaction solution to 4.0 with 0.1N hydrochloric acid, 0.05 g of 50 u / g Protease M (manufactured by Amano Enzyme) was added at 40 ° C.,
Reacted at 40 ° C for 20 hours (hereinafter referred to as enzyme-treated product E
Called)).

【0025】(ゲルろ過曲線の比較)酵素未処理物Dと酵
素処理物EをSuperdex peptide(アマ
シャムファルマシア社製)を用いたゲルろ過クロマトグ
ラフィーに供し、分子量分布を測定した。図.3にクロ
マトグラムを示すが、酵素未処理物Dと酵素処理物Eで
はほとんど変化がなく、プロテアーゼが作用していない
ことが確認された。(Comparison of gel filtration curves) The enzyme-untreated product D and the enzyme-treated product E were subjected to gel filtration chromatography using Superdex peptide (manufactured by Amersham Pharmacia) to measure the molecular weight distribution. Fig. A chromatogram is shown in Fig. 3, and there was almost no change between the enzyme-untreated product D and the enzyme-treated product E, and it was confirmed that the protease did not act.

【0026】(遊離アミノ酸含量の比較)ニンヒドリン発
色法により、反応液中の遊離アミノ酸含量を測定した。
その結果を図.4に示すが、酵素反応によりほとんど変
化が見られなかった。(Comparison of Free Amino Acid Content) The free amino acid content in the reaction solution was measured by the ninhydrin coloring method.
The results are shown in Fig. As shown in Fig. 4, almost no change was observed due to the enzymatic reaction.

【0027】(呈味、香気比較)酵素未処理物Dと酵素処
理物Eの水可溶部を分離し、5%溶液に希釈し専門パネ
ラー10名にて官能評価を行った。その結果、専門パネ
ラー全員が呈味、香気とも酵素未処理物Dと酵素処理物
Eでは差が感じられないと評価した。(Taste and aroma comparison) The water-soluble parts of the enzyme-untreated product D and the enzyme-treated product E were separated, diluted with a 5% solution, and subjected to sensory evaluation by 10 specialized panelists. As a result, all the expert panelists evaluated that there was no difference in taste and aroma between the enzyme-untreated product D and the enzyme-treated product E.

【0028】実施例2 酵母菌体100gに対し、200gの水を加え懸濁した
後、オートクレーブにて130℃、0.26MPaに
て、15分間加温、加圧処理した(以下、加圧処理物F
と称する)。この加圧処理物Fを60℃まで冷却し、1
0000u/gの放線菌由来の中性エンド型プロテアー
ゼ5mgを添加し60℃において5時間反応した(以
下、酵素処理物Gと称する)。この酵素処理物GのpH
を0.1N塩酸にて4.0に調製後、40℃にて小麦由
来の酸性カルボキシペプチダーゼ(50u/g)0.0
5gを添加し、40℃において20時間反応した(以
下、酵素処理物Hと称する;本発明品2)。Example 2 To 100 g of yeast cells, 200 g of water was added and suspended, and then heated and pressurized in an autoclave at 130 ° C. and 0.26 MPa for 15 minutes (hereinafter, pressure treatment). Object F
Called)). This pressurized product F is cooled to 60 ° C. and
5 mg of an actinomycete-derived neutral endoprotease of 0000 u / g was added and reacted at 60 ° C. for 5 hours (hereinafter, referred to as enzyme-treated product G). PH of this enzyme-treated product G
Was adjusted to 4.0 with 0.1N hydrochloric acid, and then wheat-derived acid carboxypeptidase (50 u / g) 0.0
5 g was added and reacted at 40 ° C. for 20 hours (hereinafter, referred to as enzyme-treated product H; product 2 of the present invention).

【0029】(ゲルろ過曲線の比較)上記工程による加圧
処理物F、一段階目のエンド型プロテアーゼ処理後の酵
素処理物Gおよび二段階目のエキソ型プロテアーゼ処理
後の酵素処理物H(本発明品2)をSuperdex
peptide(アマシャムファルマシア社製)を用いた
ゲルろ過クロマトグラフィーに供し、分子量分布を測定
した。図.5にクロマトグラムを示すが、加圧処理物F
と酵素処理物Gでは分子量1000〜500Daのペプ
チドが多量に生成し、酵素処理物H(本発明品2)では
分子量500Da以下のペプチド・アミノ酸が多量に生
成した。このことから酵母菌体を加圧処理することで、
両方のプロテアーゼが作用し、多量の呈味成分が生成す
ることが確認された。(Comparison of Gel Filtration Curves) Pressurized product F by the above process, enzyme-treated product G after the first step endo-type protease treatment and enzyme-treated product H after the second step exo-type protease treatment ( Invention 2) is superdex
Peptide (manufactured by Amersham Pharmacia) was used for gel filtration chromatography to measure the molecular weight distribution. Fig. The chromatogram is shown in Fig. 5, and the pressure-treated product F
The enzyme-treated product G produced a large amount of peptides having a molecular weight of 1000 to 500 Da, and the enzyme-treated product H (product 2 of the present invention) produced a large amount of peptides / amino acids having a molecular weight of 500 Da or less. From this, by pressurizing the yeast cells,
It was confirmed that both proteases act and a large amount of taste components are produced.

【0030】(遊離アミノ酸含量の比較)ニンヒドリン発
色法により、反応液中の遊離アミノ酸含量を測定した。
加圧処理物F、酵素処理物Gおよび酵素処理物H(本発
明品2)の結果を図.6に示すが、二段階の酵素反応に
より酵母菌体より遊離アミノ酸が多量に遊離することが
確認された。(Comparison of Free Amino Acid Content) The free amino acid content in the reaction solution was measured by the ninhydrin coloring method.
The results of the pressure-treated product F, the enzyme-treated product G, and the enzyme-treated product H (invention product 2) are shown in FIG. As shown in 6, it was confirmed that a large amount of free amino acids was released from the yeast cells by the two-step enzymatic reaction.

【0031】(呈味、香気比較)加圧処理物F、酵素処理
物Gおよび酵素処理物Hの水可溶部を分離し、5%溶液
に希釈し専門パネラー10名にて官能評価を行った。そ
の結果、専門パネラー全員が呈味、香気とも酵素処理物
H(本発明品2)の方が加圧処理物Fおよび酵素処理物
Gと比較し、非常に強い旨味、こく味、塩味が感じられ
ると評価した。(Comparison of taste and aroma) The water-soluble parts of the pressure-treated product F, the enzyme-treated product G and the enzyme-treated product H were separated, diluted with a 5% solution and subjected to a sensory evaluation by 10 professional panelists. It was As a result, all the expert panelists taste and smell the enzyme-treated product H (invention product 2) more strongly than the pressure-treated product F and the enzyme-treated product G, and feel a very strong umami, rich taste, and salty taste. It was evaluated as being able to.

【0032】[0032]

【発明の効果】本発明によれば、旨味やコク味および塩
味が強く、呈味性が改善され、さらに酵母臭の低減され
た酵母エキスの製造方法を提供することができる。EFFECTS OF THE INVENTION According to the present invention, it is possible to provide a method for producing a yeast extract which has a strong umami taste, a rich taste and a salty taste, an improved taste and a reduced yeast odor.

【0033】[0033]

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

【図1】加圧処理物A、酵素処理物Bおよび酵素処理物
Cのゲルろ過クロマトグラフィーによる分子量分布を示
した図面である。FIG. 1 is a drawing showing molecular weight distributions of a pressure-treated product A, an enzyme-treated product B, and an enzyme-treated product C by gel filtration chromatography.

【図2】加圧処理物A、酵素処理物Bおよび酵素処理物
Cの遊離アミノ酸量を示す図面である。FIG. 2 is a drawing showing the amounts of free amino acids of pressure-treated product A, enzyme-treated product B, and enzyme-treated product C.

【図3】加圧処理物Dと酵素処理物Eのゲルろ過クロマ
トグラフィーによる分子量分布を示した図面である。FIG. 3 is a drawing showing the molecular weight distributions of pressure-treated product D and enzyme-treated product E by gel filtration chromatography.

【図4】加圧処理物Dと酵素処理物Eの遊離アミノ酸量
を示した図面である。FIG. 4 is a drawing showing the amounts of free amino acids of pressure-treated product D and enzyme-treated product E.

【図5】加圧処理物F、酵素処理物Gおよび酵素処理物
Hのゲルろ過クロマトグラフィーによる分子量分布を示
した図面である。FIG. 5 is a drawing showing the molecular weight distributions of pressure-treated product F, enzyme-treated product G, and enzyme-treated product H by gel filtration chromatography.

【図6】加圧処理物F、酵素処理物Gおよび酵素処理物
Hの遊離アミノ酸量を示す図面である。FIG. 6 is a drawing showing the amounts of free amino acids of the pressure-treated product F, the enzyme-treated product G, and the enzyme-treated product H.

Claims (2)

【特許請求の範囲】[Claims] 【請求項1】酵母菌体を高圧処理した後、エンド型プロ
テアーゼで処理し、次いでエキソ型プロテアーゼを作用
させることを特徴とする酵母エキスの製造方法。1. A method for producing a yeast extract, which comprises treating a yeast cell with a high pressure, treating with an endo-type protease, and then allowing an exo-type protease to act thereon. 【請求項2】高圧処理が0〜0.8MPaの範囲内の圧
力である請求項1記載の製造方法。2. The manufacturing method according to claim 1, wherein the high-pressure treatment is performed at a pressure within a range of 0 to 0.8 MPa.
JP2002138431A 2002-05-14 2002-05-14 Method for producing yeast extract Pending JP2003325130A (en)

Priority Applications (1)

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Family

ID=29699872

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Cited By (7)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
JP2007049989A (en) * 2005-07-20 2007-03-01 Nippon Paper Chemicals Co Ltd Yeast extract and method for producing the same
JP2007049984A (en) * 2005-07-20 2007-03-01 Nippon Paper Chemicals Co Ltd Yeast extract and method for producing the same
JP2007049988A (en) * 2005-07-20 2007-03-01 Nippon Paper Chemicals Co Ltd Yeast extract and method for producing the same
JP2010090065A (en) * 2008-10-08 2010-04-22 Nihon Kolmar Co Ltd Cosmetic product
WO2012011402A1 (en) 2010-07-22 2012-01-26 キッコーマン株式会社 Yeast extract containing lactic acid
WO2017114403A1 (en) * 2015-12-28 2017-07-06 Novozymes A/S Method for producing a yeast extract
CN113906145A (en) * 2019-05-29 2022-01-07 欧励有限公司 Yeast extract rich in trehalose

Cited By (11)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
JP2007049989A (en) * 2005-07-20 2007-03-01 Nippon Paper Chemicals Co Ltd Yeast extract and method for producing the same
JP2007049984A (en) * 2005-07-20 2007-03-01 Nippon Paper Chemicals Co Ltd Yeast extract and method for producing the same
JP2007049988A (en) * 2005-07-20 2007-03-01 Nippon Paper Chemicals Co Ltd Yeast extract and method for producing the same
JP4543010B2 (en) * 2005-07-20 2010-09-15 日本製紙ケミカル株式会社 Method for producing yeast extract
JP4543018B2 (en) * 2005-07-20 2010-09-15 日本製紙ケミカル株式会社 Method for producing yeast extract
JP2010090065A (en) * 2008-10-08 2010-04-22 Nihon Kolmar Co Ltd Cosmetic product
WO2012011402A1 (en) 2010-07-22 2012-01-26 キッコーマン株式会社 Yeast extract containing lactic acid
WO2017114403A1 (en) * 2015-12-28 2017-07-06 Novozymes A/S Method for producing a yeast extract
CN108473938A (en) * 2015-12-28 2018-08-31 诺维信公司 Method for producing yeast extract
CN113906145A (en) * 2019-05-29 2022-01-07 欧励有限公司 Yeast extract rich in trehalose
JP2022535695A (en) * 2019-05-29 2022-08-10 オーリー ゲー・エム・ベー・ハー Yeast extract rich in trehalose

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