JP2007089522A - Method for producing fatty acid composition containing specific highly unsaturated fatty acid in concentrated state - Google Patents
Method for producing fatty acid composition containing specific highly unsaturated fatty acid in concentrated state Download PDFInfo
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- JP2007089522A JP2007089522A JP2005285578A JP2005285578A JP2007089522A JP 2007089522 A JP2007089522 A JP 2007089522A JP 2005285578 A JP2005285578 A JP 2005285578A JP 2005285578 A JP2005285578 A JP 2005285578A JP 2007089522 A JP2007089522 A JP 2007089522A
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- JP
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- Prior art keywords
- fatty acid
- lipase
- specific
- highly unsaturated
- acid
- Prior art date
- Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.)
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Abstract
Description
本発明は、特定の高度不飽和脂肪酸が濃縮された脂肪酸組成物の製造方法、及びこの方法により製造される脂肪酸組成物に関する。 The present invention relates to a method for producing a fatty acid composition in which a specific highly unsaturated fatty acid is concentrated, and a fatty acid composition produced by this method.
高度不飽和脂肪酸のエイコサペンタエン酸(以下「EPA」と称する)、ドコサヘキサエン酸(以下「DHA」と称する)は、特に、動脈硬化症、血栓症などの成人病の予防効果や抗ガン作用、学習能の増強作用などで多くの生理機能を有していることが知られ、医薬品、特定保健用食品への利用で様々な試みがなされている。しかし、最近ではこれらの他の高度不飽和脂肪酸の生理機能にも注目が集っている。 Eicosapentaenoic acid (hereinafter referred to as “EPA”) and docosahexaenoic acid (hereinafter referred to as “DHA”), which are highly unsaturated fatty acids, are particularly effective in preventing and anti-cancer and learning for adult diseases such as arteriosclerosis and thrombosis. It is known that it has many physiological functions, such as a potentiating action, and various attempts have been made for use in pharmaceuticals and foods for specified health use. Recently, however, the physiological functions of these other polyunsaturated fatty acids have attracted attention.
高度不飽和脂肪酸の1種であるアラキドン酸は、血液や肝臓などの重要な器官を構成する脂肪酸の約10%程度を占めており(例えば、ヒト血液のリン脂質中の脂肪酸組成比では、アラキドン酸は11%、エイコサペンタエン酸は1%、ドコサヘキサエン酸は3%)、細胞膜の主要構成成分として膜の流動性の調節に関与し、体内の代謝で様々な機能を示す一方、プロスタグランジン類の直接の前駆体として重要な役割を果たす。特に最近は、乳幼児栄養としてのアラキドン酸の役割、神経活性作用を示す内因性カンナビノイド(2-アラキドノイルモノグリセロール、アナンダミド)の構成脂肪酸として注目されている。通常はリノール酸を富む食品を摂取すればアラキドン酸に変換されるが、成人病患者やその予備軍、乳児、老人では生合成に関与する酵素の働きが低下し、これらアラキドン酸は不足しがちとなるため、油脂(トリグリセリドの構成脂肪酸)として、直接に摂取することが望まれる。 Arachidonic acid, a type of polyunsaturated fatty acid, accounts for about 10% of fatty acids that make up vital organs such as blood and liver (for example, arachidone is a fatty acid composition ratio in phospholipids of human blood). 11% for acid, 1% for eicosapentaenoic acid and 3% for docosahexaenoic acid). It is involved in the regulation of membrane fluidity as a major component of cell membrane, and exhibits various functions in metabolism in the body, while prostaglandins Plays an important role as a direct precursor. Particularly recently, it has been attracting attention as a constituent fatty acid of endogenous cannabinoids (2-arachidonoyl monoglycerol, anandamide) that exhibit a role of arachidonic acid as infant nutrition and a neuroactive activity. Normally, when foods rich in linoleic acid are ingested, it is converted to arachidonic acid, but in ill patients and their reserves, infants and the elderly, the activities of enzymes involved in biosynthesis decrease, and these arachidonic acids tend to be deficient. Therefore, it is desirable to take it directly as fats and oils (triglyceride constituent fatty acids).
EPAやDHAには、魚油という豊富な供給源が存在するが、ジホモ-γ-リノレン酸(DGLA)、アラキドン酸(ARA)及び5,8,11−エイコサペンタエン酸(20:3 n-9)は、従来の油脂供給源から殆ど得ることができず、現在では微生物を発酵して得た高度不飽和脂肪酸を構成脂肪酸として成る油脂(トリグリセリド)が一般に使用されている。例えば、アラキドン酸を構成脂肪酸として成る油脂(トリグリセリド)を産生することのできる種々の微生物を培養して、アラキドン酸を構成脂肪酸として成る油脂(トリグリセリド)を得る方法が提案されている。この中でも、特にモルティエレラ属の微生物を用いることによって、アラキドン酸高含有油脂(トリグリセリド)が得られることが知られている(特開昭63-44891、特開昭63-12290)。さらに同じモルティエレラ属の微生物の変異株を用いてジホモ-γ-リノレン酸、アラキドン酸及び5,8,11−エイコサペンタエン酸(20:3 n-9)を生産する技術が開示されている(特開平5-91887、特開平5-91888)。 EPA and DHA have abundant sources of fish oil, but dihomo-γ-linolenic acid (DGLA), arachidonic acid (ARA) and 5,8,11-eicosapentaenoic acid (20: 3 n-9) Can hardly be obtained from conventional oil sources, and at present, fats and oils (triglycerides) comprising polyunsaturated fatty acids obtained by fermenting microorganisms as constituent fatty acids are generally used. For example, a method has been proposed in which various microorganisms capable of producing fats and oils (triglycerides) containing arachidonic acid as a constituent fatty acid are cultured to obtain fats and oils (triglycerides) containing arachidonic acid as a constituent fatty acid. Of these, it is known that oils and fats (triglycerides) with a high content of arachidonic acid can be obtained by using microorganisms belonging to the genus Mortierella (JP-A 63-44891, JP-A 63-12290). Furthermore, a technique for producing dihomo-γ-linolenic acid, arachidonic acid and 5,8,11-eicosapentaenoic acid (20: 3 n-9) using the same mutant of the microorganism belonging to the genus Mortierella is disclosed ( JP-A-5-91887, JP-A-5-91888).
これまで、多彩な効果を示してきた高度不飽和脂肪酸ではあるが、例え微生物で作った油脂であっても、この油脂(トリグリセリド)中に含まれるアラキドン酸等の高度不飽和脂肪酸は40%を程度である。この有用性を広めるためにはもっと高度不飽和脂肪酸の濃度を高め、少量で使える形にする必要がある。このため高純度の高度不飽和脂肪酸が期待されている。 Up to now, polyunsaturated fatty acids have shown various effects, but even for fats and oils made with microorganisms, 40% of highly unsaturated fatty acids such as arachidonic acid contained in these fats and oils (triglycerides). Degree. In order to spread this usefulness, it is necessary to increase the concentration of highly unsaturated fatty acids so that they can be used in small amounts. For this reason, highly pure highly unsaturated fatty acids are expected.
これら高度不飽和脂肪酸の純度を工業的に高める手段としては、大規模な高速液体クロマトグラフィー(HPLC)を用いる方法(Y.Yamamura, et.al., J.Am. Oil Chem. Soc., 74, 1435(1997))や銀との錯体形成を利用する方法(山口ら、油化学 40, 959(1991))が考案されている。しかし、製造コストの点から工業的な精製方法として採用されていない。高度不飽和脂肪酸は熱や酸化に対して非常に不安定であることから温和な条件下で反応が進行する酵素(リパーゼ)の利用も注目され、2種のリパーゼを組合せてマグロ油から90%のDHA(Y.Shimada, et.al., J.Am. Oil Chem. Soc., 74, 1441(1997))をボラージ油から98%の純度のγ−リノレン酸(18:3 n-6)(Y.Shimada, et.al., J.Am. Oil Chem. Soc., 72, 1323(1995); Y.Shimada, et.al., J.Am. Oil Chem. Soc., 75, 1581(1998))を精製している。アラキドン酸についても島田ら(島田ら 科学と工業 73, 125-130(1999))がリパーゼの非選択的加水分解と選択的なリパーゼのエステル化を組合せ検討している。その結果、n-6系高度不飽和脂肪酸が96%にまで濃縮精製されたが、アラキドン酸は81%の純度にとどまっている。これは原料油脂に混在するアラキドン酸の他のn-6系高度不飽和脂肪酸も同時に濃縮されたためである。また、n-6系高度不飽和脂肪酸やn-9系高度不飽和脂肪酸の中には、まだ、単一種の高度不飽和脂肪酸のみを濃縮する方法について検討されていないものもある。 As a means of industrially increasing the purity of these highly unsaturated fatty acids, a method using large-scale high performance liquid chromatography (HPLC) (Y. Yamamura, et.al., J. Am. Oil Chem. Soc., 74 , 1435 (1997)) and a method using a complex formation with silver (Yamaguchi et al., Oil Chemistry 40, 959 (1991)) has been devised. However, it has not been adopted as an industrial purification method from the viewpoint of production cost. Since polyunsaturated fatty acids are very unstable to heat and oxidation, the use of enzymes (lipases) that react under mild conditions is also attracting attention. 90% of tuna oil is a combination of two lipases. Of DHA (Y. Shimada, et.al., J. Am. Oil Chem. Soc., 74, 1441 (1997)) from borage oil to 98% pure γ-linolenic acid (18: 3 n-6) (Y. Shimada, et.al., J. Am. Oil Chem. Soc., 72, 1323 (1995); Y. Shimada, et.al., J. Am. Oil Chem. Soc., 75, 1581 ( 1998)). As for arachidonic acid, Shimada et al. (Shimada et al. Science and Industry 73, 125-130 (1999)) are examining non-selective hydrolysis of lipase and selective esterification of lipase. As a result, n-6 polyunsaturated fatty acids were concentrated and purified to 96%, but arachidonic acid remained at a purity of 81%. This is because other n-6 polyunsaturated fatty acids other than arachidonic acid mixed in the raw oil and fat were concentrated at the same time. Some n-6 highly unsaturated fatty acids and n-9 highly unsaturated fatty acids have not yet been studied for a method of concentrating only one kind of highly unsaturated fatty acid.
このように、単一種の高度不飽和脂肪酸が高純度となるような方法については、まだ充分な検討がなされていない。
一方、市場においては、使用量を少なくするとともに、余分な脂肪酸の混入を避け、コンパクトな商品設計をするために高純度の単一種の高度不飽和脂肪酸を含有する油脂が求められている。すなわち、単一種の高度不飽和脂肪酸を高純度とする方法の検討、およびその方法により得られた高度不飽和脂肪酸を含有する油脂が求められていた。
Thus, sufficient examination has not yet been made about a method in which a single type of highly unsaturated fatty acid has high purity.
On the other hand, in the market, there is a demand for fats and oils containing a single type of highly unsaturated fatty acid of high purity in order to reduce the amount used, avoid mixing of extra fatty acids, and design a compact product. That is, the examination of the method of making a single kind of highly unsaturated fatty acid highly pure, and the fats and oils containing the highly unsaturated fatty acid obtained by the method have been desired.
本発明は、このようなコンパクトな商品設計を実現するために、リパーゼを選択し、リパーゼ反応の組合せによってアラキドン酸に代表される高度不飽和脂肪酸を高純度化する方法およびそれを含有する組成物およびそれらを含有する食品や健康食品を提供するものである。
単一種の高度不飽和脂肪酸を高純度で含む脂肪酸組成物を得るため、例えば、真菌類が生産し炭素数20以上かつ2重結合を2個以上含む高度不飽和脂肪酸を20%以上含有する油脂(トリグリセリド)を原料にして、選択性が厳密なリパーゼのエステル化反応を中心に、数段の反応を組み合わせることにより得ることができた。
In order to realize such a compact product design, the present invention selects a lipase and highly purifies highly unsaturated fatty acid typified by arachidonic acid by a combination of lipase reactions, and a composition containing the same And foods and health foods containing them.
In order to obtain a fatty acid composition containing a single type of highly unsaturated fatty acid with high purity, for example, an oil and fat produced by fungi and containing 20% or more of a highly unsaturated fatty acid containing 20 or more carbon atoms and 2 or more double bonds (Triglyceride) was used as a raw material, and it could be obtained by combining several stages of reaction, focusing on the esterification reaction of lipase with strict selectivity.
すなわち、リパーゼの脂肪酸に対する反応性を見極めることが大切であり、混在し除去したい脂肪酸と濃縮したい脂肪酸との反応性の差が大きなリパーゼを選択することが中心であり、この選択したリパーゼによるエステル化と非特異的リパーゼによるトリグリセリドの分解、尿素包括法を組み合わせることで高純度の単一種の高度不飽和脂肪酸を含む油脂の製造方法を完成した。 In other words, it is important to determine the reactivity of lipase to fatty acids, and it is mainly to select lipases that have a large difference in reactivity between fatty acids that are mixed and removed and fatty acids that are to be concentrated. The production method of fats and oils containing a single highly polyunsaturated fatty acid with high purity was completed by combining triglyceride degradation with non-specific lipase and urea inclusion method.
従って、本発明は、例えば微生物(特に真菌類)が生産する油脂(トリグリセリド)を原料にして、選択性が厳密なリパーゼのエステル化反応を中心に、数段の反応を組み合わせることにより得られる高純度の単一種の高度不飽和脂肪酸を含む油脂の製造方法ならびにこれら油脂を含む組成物を提供する。 Therefore, the present invention can be obtained by combining several stages of reaction, focusing mainly on esterification of lipase with strict selectivity, using, for example, fats and oils (triglycerides) produced by microorganisms (particularly fungi) as raw materials. Provided are a method for producing fats and oils containing a single type of highly unsaturated fatty acid having a purity, and a composition containing these fats and oils.
従って、本発明は、特定の高度不飽和脂肪酸の比率が50%以上である脂肪酸組成物の製造方法において、
(1)前記特定の高度不飽和脂肪酸に対する特異性が、他の高度不飽和脂肪酸に対する特異性よりも低いリパーゼ(特異的リパーゼ)を、脂肪アルコールの存在下で、前記特定の高度不飽和脂肪酸を含んで成る脂肪酸組成物に作用させることにより、前記特定の高度不飽和脂肪酸以外の脂肪酸を選択的にエステル化し;
(2)前記工程(1)で生じたエステルを除去して、前記特定の高度不飽和脂肪酸が濃縮された脂肪酸組成物を得;そして
(3)前記工程(1)において使用したリパーゼと同じリパーゼ又は異なるリパーゼを道いて、前記工程(1)及び(2)を反復する;
ことを含んで成る方法を提供する。
Therefore, the present invention provides a method for producing a fatty acid composition in which the ratio of a specific highly unsaturated fatty acid is 50% or more,
(1) A lipase (specific lipase) having a specificity for the specific polyunsaturated fatty acid is lower than that for the other polyunsaturated fatty acid, and the specific polyunsaturated fatty acid in the presence of a fatty alcohol. Selectively esterifying fatty acids other than the specific polyunsaturated fatty acids by acting on the fatty acid composition comprising;
(2) removing the ester produced in the step (1) to obtain a fatty acid composition enriched with the specific polyunsaturated fatty acid; and (3) the same lipase as the lipase used in the step (1). Or go through different lipases and repeat steps (1) and (2) above;
A method comprising the above is provided.
上記の方法において、前記工程(1)で用いられる脂肪酸組成物は、例えば、下記の工程:
(a)前記特定の高度不飽和脂肪酸の含有する脂肪酸組成物を用意し;
(b)尿素包括法により飽和脂肪酸を除去して、高度不飽和脂肪酸が濃縮された脂肪酸組成物を得る
により得る。
In the above method, the fatty acid composition used in the step (1) is, for example, the following step:
(A) preparing a fatty acid composition containing the specific highly unsaturated fatty acid;
(B) A saturated fatty acid is removed by the urea inclusion method to obtain a fatty acid composition enriched with highly unsaturated fatty acids.
上記の方法において、前記工程(a)における原料となる脂肪酸組成物は、前記特定の高度不飽和脂肪酸を含有するエステルのリパーゼ分解又は鹸化により得る。この、エステルは、例えば、前記特定の高度不飽和脂肪酸を含有するモノグリセライド、ジグリセライド及びトリグリセライドから成る群から選択されるグリセライドであり、典型的にはトリグリセライドである。前記工程(a)において使用するリパーゼは、例えば、前記特定の高度不飽和脂肪酸とその他の脂肪酸との間で基質特異性の差が少ないリパーゼである。 In the above method, the fatty acid composition as a raw material in the step (a) is obtained by lipase decomposition or saponification of an ester containing the specific highly unsaturated fatty acid. The ester is, for example, a glyceride selected from the group consisting of monoglycerides, diglycerides and triglycerides containing the specific highly unsaturated fatty acid, and is typically triglyceride. The lipase used in the step (a) is, for example, a lipase with little difference in substrate specificity between the specific polyunsaturated fatty acid and other fatty acids.
前記特異的にエステル化するために使用する脂肪アルコールは、好ましくは炭素原子数8〜16個の脂肪アルコールであり、例えば炭素原子数12個のラウリルアルコールである。
前記特定の高度不飽和脂肪酸は、例えば、n-6系高度不飽和脂肪酸、例えばアラキドン酸、ジホモ−γ−リノレン酸;n-9系高度不飽和脂肪酸、例えばミード酸である。
The fatty alcohol used for the specific esterification is preferably a fatty alcohol having 8 to 16 carbon atoms, such as lauryl alcohol having 12 carbon atoms.
The specific highly unsaturated fatty acid is, for example, an n-6 highly unsaturated fatty acid such as arachidonic acid, dihomo-γ-linolenic acid; an n-9 highly unsaturated fatty acid such as mead acid.
前記特定の高度不飽和脂肪酸は、例えばアラキドン酸であり、この場合、前記工程(3)で使用する特異的リパーゼは、ブルクホルデリア・セパシア由来(旧分類ではシュードモナス・スペーシス(Pseudomonas sp.)由来)のリパーゼである。得られた高度不飽和脂肪酸組成物中のアラキドン酸の比率は85%以上、好ましくは90%以上、更に好ましくは95%以上である。 The specific polyunsaturated fatty acid is, for example, arachidonic acid. In this case, the specific lipase used in the step (3) is derived from Burkholderia cepacia (formerly Pseudomonas sp.). ) Lipase. The ratio of arachidonic acid in the obtained highly unsaturated fatty acid composition is 85% or more, preferably 90% or more, and more preferably 95% or more.
他の例では、前記特定の高度不飽和脂肪酸が、ジホモ−γ−リノレン酸であり、この場合、前記工程(1)で使用する特異的リパーゼは、シュードモナス・アエルギノサ(Pseudomonas aeruginosa)由来のリパーゼ及び/又はカンジダ・ルゴサ(Candida rugosa)由来のリパーゼである。得られた高度不飽和脂肪酸組成物中のジホモ−γ−リノレン酸の比率が50%以上であり、好ましくは80%以上であり、更に好ましくは89%以上である。 In another example, the specific polyunsaturated fatty acid is dihomo-γ-linolenic acid, in which case the specific lipase used in step (1) is a lipase derived from Pseudomonas aeruginosa and It is a lipase derived from Candida rugosa. The ratio of dihomo-γ-linolenic acid in the obtained highly unsaturated fatty acid composition is 50% or more, preferably 80% or more, and more preferably 89% or more.
更に他の例では、前記特定の高度不飽和脂肪酸が、ミード酸であり、この場合、前記工程(1)で使用する特異的リパーゼは、ブルクホルデリア・セパシア(旧分類ではシュードモナス・スペーシス)由来のリパーゼである。得られた高度不飽和脂肪酸組成物中のミードの比率は50%以上であり、好ましくは80%以上であり、更に好ましくは90%以上である。 In yet another example, the specific polyunsaturated fatty acid is mead acid, and in this case, the specific lipase used in the step (1) is derived from Burkholderia cepacia (Pseudomonas space in the old classification). Lipase. The proportion of mead in the obtained highly unsaturated fatty acid composition is 50% or more, preferably 80% or more, more preferably 90% or more.
本発明は更に、前記の方法により得られる、アラキドン酸含有脂肪酸組成物、ジホモ−γ−リノレン酸含有脂肪酸組成物及びミード酸含有脂肪酸組成物を提供する。本発明は更に、前記脂肪酸組成物を含んで成る食品、例えば健康食品、サプリメント、を提供する。 The present invention further provides an arachidonic acid-containing fatty acid composition, dihomo-γ-linolenic acid-containing fatty acid composition, and mead acid-containing fatty acid composition obtained by the above method. The present invention further provides foods comprising the fatty acid composition, such as health foods and supplements.
本発明において、高度不飽和脂肪酸とは、18個〜24個の炭素原子を有す、2個以上の二重結合を有する脂肪酸であり、好ましくは20個〜22個の炭素原子を有し、3個〜4個の二重結合を有する脂肪酸を意味する。
本発明の方法において出発原料として使用する、特定の(目的とする)高度不飽和脂肪酸を含有する脂肪酸組成物は、例えば脂肪酸エステルの鹸化又はリパーゼ分解により得られる。脂肪酸エステルは実用的には、グリセライド、モノグリセライド、ジグリセライド又はトリグリセライドであり、最も実用的には、トリグリセライドを主成分とする天然油脂である。
In the present invention, polyunsaturated fatty acids are fatty acids having 18 to 24 carbon atoms and having two or more double bonds, preferably 20 to 22 carbon atoms, It means a fatty acid having 3 to 4 double bonds.
The fatty acid composition containing a specific (target) highly unsaturated fatty acid used as a starting material in the method of the present invention can be obtained, for example, by saponification or lipase decomposition of a fatty acid ester. The fatty acid ester is practically a glyceride, a monoglyceride, a diglyceride or a triglyceride, and most practically a natural fat / oil mainly composed of triglyceride.
原料油脂としての微生物が生産する油脂(トリグリセリド)
高度不飽和脂肪酸を構成脂肪酸として成る油脂(トリグリセリド)を産生しうる微生物を培養する。ここでいう微生物としては、炭素数が20以上で二重結合は2以上のn-6系、n-9系またはn-3系の高度不飽和脂肪酸の少なくとも1種の高度不飽和脂肪酸を主にトリグリセリドの構成脂肪酸として産生する微生物が望ましい。
Fats and oils (triglycerides) produced by microorganisms as raw oils and fats
A microorganism capable of producing oils and fats (triglycerides) comprising highly unsaturated fatty acids as constituent fatty acids is cultured. The microorganism here is mainly composed of at least one highly unsaturated fatty acid of n-6 series, n-9 series or n-3 series, which has 20 or more carbon atoms and 2 or more double bonds. In particular, microorganisms that produce triglycerides as constituent fatty acids are desirable.
そして、炭素数が20以上で二重結合は2以上のn-6系、n-9系またはn-3系の高度不飽和脂肪酸としては、ジホモ-γ-リノレン酸(DGLA;8,11,14-エイコサトリエン酸)、アラキドン酸(ARA;5,8,11,14-エイコサテトラエン酸)、7,10,13,16-ドコサテトラエン酸(22:4n-6)、DPAω6(4,7,10,13,16-ドコサペンタエン酸)、8,11-エイコサジエン酸、ミード酸(5,8,11-エイコサトリエン酸)、8,11,14,17-エイコサテトラエン酸(20:4 n-3)、EPA(5,8,11,14,17-エイコサペンタエン酸)、DPAn-3(7,10,13,16,19-ドコサペンタエン酸)、及びDHA(4,7,10,13,16,19-ドコサヘキサエン酸)を挙げることができる。 Further, as an n-6 series, n-9 series or n-3 series highly unsaturated fatty acid having 20 or more carbon atoms and two or more double bonds, dihomo-γ-linolenic acid (DGLA; 8, 11, 14-eicosatrienoic acid), arachidonic acid (ARA; 5,8,11,14-eicosatetraenoic acid), 7,10,13,16-docosatetraenoic acid (22: 4n-6), DPAω6 ( 4,7,10,13,16-docosapentaenoic acid), 8,11-eicosadienoic acid, mead acid (5,8,11-eicosatrienoic acid), 8,11,14,17-eicosatetraene Acid (20: 4 n-3), EPA (5,8,11,14,17-eicosapentaenoic acid), DPAn-3 (7,10,13,16,19-docosapentaenoic acid), and DHA ( 4,7,10,13,16,19-docosahexaenoic acid).
従って、本発明においては、高度不飽和脂肪酸を構成脂肪酸として成る油脂(トリグリセリド)を産生しうる微生物であればすべて使用することができる。例えば、アラキドン酸を構成脂肪酸として成る油脂(トリグリセリド)の生産能を有する微生物としては、モルティエレラ(Mortierella)属、コニディオボラス(Conidiobolus)属、フィチウム(Pythium)属、フィトフトラ(Phytophthora)属、ペニシリューム(Penicillium)属、クロドスポリューム(Cladosporium)属、ムコール(Mucor)属、フザリューム(Fusarium)属、アスペルギルス(Aspergillus)属、ロードトルラ(Rhodotorula)属、エントモフトラ(Entomophthora)属、エキノスポランジウム(Echinosporangium)属、サプロレグニア(Saprolegnia)属に属する微生物を挙げることができる。 Therefore, in the present invention, any microorganism can be used as long as it can produce fats and oils (triglycerides) composed of highly unsaturated fatty acids as constituent fatty acids. For example, as the microorganism capable of producing fats and oils comprising arachidonic acid as a constituent fatty acid (triglyceride), Mortierella (Mortierella) genus, Koni audio bolus (Conidiobolus) genus Fichiumu (Pythium) genus Phytophthora (Phytophthora) genus, Penishiryumu (Penicillium) genus, Clos de sports Liu beam (Cladosporium) genus, Mucor (Mucor) genus, Fuzaryumu (Fusarium) genus Aspergillus (Aspergillus) genus, Rhodotorula (Rhodotorula) genus, Entomofutora (Entomophthora) genus, echinochrome aminocephalosporanic indium (Echinosporangium) genus And microorganisms belonging to the genus Saprolegnia .
モルティエレラ(Mortierella)属モルティエレラ(Mortierella)亜属に属する微生物では、例えばモルティエレラ・エロンガタ(Mortierella elongata)、モルティエレラ・エキシグア(Mortierella exigua)、モルティエレラ・フィグロフィラ(Mortierella hygrophila)、モルティエレラ・アルピナ(Mortierella alpina)等を挙げることができる。具体的にはモルティエレラ・エロンガタ(Mortierella elongata)IFO8570、モルティエレラ・エキシグア(Mortierella exigua)IFO8571、モルティエレラ・フィグロフィラ(Mortierella hygrophila)IFO5941、モルティエレラ・アルピナ(Mortierella alpina)IFO8568、ATCC16266、ATCC32221、ATCC42430、CBS219.35、CBS224.37、CBS250.53、CBS343.66、CBS527.72、CBS529.72、CBS608.70、CBS754.68等の菌株を挙げることができる。 In the Mortierella (Mortierella) belonging to the genus Mortierella (Mortierella) microorganisms belonging to the subgenus, for example Mortierella elongata (Mortierella elongata), Mortierella exigua (Mortierella exigua), Mortierella Figurofira (Mortierella hygrophila), Mortierella alpina ( Mortierella alpina ). More specifically, Mortierella elongata IFO8570, Mortierella exigua IFO8571, Mortierella hygrophila IFO5941, Mortierella alpina 221266266, CC41, 266266CC Examples include CBS219.35, CBS224.37, CBS250.53, CBS343.66, CBS527.72, CBS529.72, CBS608.70, CBS754.68 and the like.
例えば、DHAを産生しうる微生物として、クリプテコデニウム(Crypthecodenium)属、スラウトキトリウム(Thrautochytrium)属、シゾキトリウム(Schizochytrium)属、ウルケニア(Ulkenia)属、ジャポノキトリウム(Japonochytrium)属又はハリフォトリス(Haliphthoros)属に属する微生物を挙げることもできる。 For example, a microorganism capable of producing DHA, Crypthecodinium Kode hexafluorophosphate (Crypthecodenium) genus scan Lau Toki thorium (Thrautochytrium) genus Schizochytrium (Schizochytrium) genus Ulkenia (Ulkenia) genus, Japo eaves thorium (Japonochytrium) genus or needles Photo Squirrel Mention may also be made of microorganisms belonging to the genus ( Haliphthoros ).
これらの菌株はいずれも、大阪市の財団法人醗酵研究所(IFO)、及び米国のアメリカン・タイプ・カルチャー・コレクション(American Type Culture Collection, ATCC)及び、Centrralbureau voor Schimmelcultures(CBS)からなんら制限なく入手することができる。また本発明の研究グループが土壌から分離した菌株モルティエレラ・エロンガタSAM0219(微工研菌寄第8703号)(微工研条寄第1239号)を使用することもできる。 All of these strains are obtained from Osaka City Foundation for Fermentation (IFO), American Type Culture Collection (ATCC), and Centrralbureau voor Schimmelcultures (CBS) without any restrictions. can do. In addition, the strain Mortierella elongata SAM0219 (Mikken Kenyoku No. 8703) (Mikken Kenjyo No. 1239) isolated from soil by the research group of the present invention can also be used.
本発明に使用される菌株を培養する為には、その菌株の胞子、菌糸、又は予め培養して得られた種培養液あるいは種培養より回収した菌体を、液体培地又は固体培地に接種し本培養する。液体培地の場合に、炭素源としてはグルコース、フラクトース、キシロース、サッカロース、マルトース、可溶性デンプン、糖蜜、グリセロール、マンニトール、糖化澱粉等の一般的に使用されているものが、いずれも使用できるが、これらに限られるものではない。 In order to culture the strain used in the present invention, a spore, mycelium of the strain, or a seed culture solution obtained by culturing in advance or a cell recovered from the seed culture is inoculated into a liquid medium or a solid medium. Main culture. In the case of a liquid medium, as carbon sources, generally used ones such as glucose, fructose, xylose, saccharose, maltose, soluble starch, molasses, glycerol, mannitol, saccharified starch, etc. can be used. It is not limited to.
窒素源としてはペプトン、酵母エキス、麦芽エキス、肉エキス、カザミノ酸、コーンスティープリカー、大豆タンパク、脱脂ダイズ、綿実カス等の天然窒素源の他に、尿素等の有機窒素源、ならびに硝酸ナトリウム、硝酸アンモニウム、硫酸アンモニウム等の無機窒素源を用いることができるが、特に大豆から得られる窒素源、具体的には大豆、脱脂大豆、大豆フレーク、食用大豆タンパク、おから、豆乳、きな粉等が挙げられるが、特に、脱脂大豆に熱変性を施したもの、より好ましくは脱脂大豆を約70〜90℃で熱処理し、さらにエタノール可溶成分を除去したものを単独または複数で、あるいは前記窒素源と組み合わせて使用することができる。 Nitrogen sources include natural nitrogen sources such as peptone, yeast extract, malt extract, meat extract, casamino acid, corn steep liquor, soy protein, defatted soybean, cottonseed residue, etc., organic nitrogen sources such as urea, and sodium nitrate Inorganic nitrogen sources such as ammonium nitrate and ammonium sulfate can be used, particularly nitrogen sources obtained from soybeans, specifically soybeans, defatted soybeans, soybean flakes, edible soybean proteins, okara, soy milk, kinako flour, etc. However, especially those obtained by subjecting defatted soybeans to heat denaturation, more preferably heat treatment of defatted soybeans at about 70 to 90 ° C. and further removal of ethanol-soluble components, alone or in combination, or in combination with the nitrogen source Can be used.
この他必要に応じて、リン酸イオン、カリウムイオン、ナトリウムイオン、マグネシウムイオン、カルシウムイオン以外に、鉄、銅、亜鉛、マンガン、ニッケル、コバルト等の金属イオンやビタミン等を微量栄養源として使用できる。これらの培地成分は微生物の生育を害しない濃度であれば特に制限はない。実用上、一般に炭素源は総添加量は0.1〜40重量%、好ましくは1〜25重量%、窒素源の総添加量は2〜15重量%、好ましくは2〜10重量%とするのが望ましく、より好ましくは初発の炭素源添加量を1〜5重量%、初発の窒素源添加量を3〜8重量%として、培養途中に炭素源及び窒素源を、さらにより好ましくは炭素源のみを流加して培養する。 In addition to phosphate ions, potassium ions, sodium ions, magnesium ions, and calcium ions, metal ions such as iron, copper, zinc, manganese, nickel, and cobalt, vitamins, etc. can be used as trace nutrient sources as needed. . These medium components are not particularly limited as long as they do not impair the growth of microorganisms. In practice, the total amount of carbon source is generally 0.1 to 40% by weight, preferably 1 to 25% by weight, and the total amount of nitrogen source is 2 to 15% by weight, preferably 2 to 10% by weight. More preferably, the initial carbon source addition amount is 1 to 5% by weight, the initial nitrogen source addition amount is 3 to 8% by weight, and the carbon source and nitrogen source are flowed during the cultivation, and still more preferably only the carbon source is allowed to flow. And incubate.
なお、不飽和脂肪酸の収率を増加せしめるために、不飽和脂肪酸の前駆体として、例えば、ヘキサデカン若しくはオクタデカンのごとき炭化水素;オレイン酸若しくはリノール酸のごとき脂肪酸又はその塩、復は脂肪酸エステル、例えばエチルエステル、グリセリン脂肪酸エステル、ソルビタン脂肪酸エステル;又はオリーブ油、大豆油、なたね油、綿実油若しくはヤシ油のごとき油脂類を単独で、又は組み合わせて使用できる。基質の添加量は培地に対して0.001〜10%、好ましくは0.5〜10%である。またこれらの基質を唯一の炭素源として培養してもよい。 In order to increase the yield of unsaturated fatty acid, as a precursor of unsaturated fatty acid, for example, a hydrocarbon such as hexadecane or octadecane; a fatty acid such as oleic acid or linoleic acid or a salt thereof; Ethyl esters, glycerin fatty acid esters, sorbitan fatty acid esters; or oils and fats such as olive oil, soybean oil, rapeseed oil, cottonseed oil or coconut oil can be used alone or in combination. The amount of the substrate added is 0.001 to 10%, preferably 0.5 to 10%, based on the medium. These substrates may be cultured as the sole carbon source.
高度不飽和脂肪酸を産生する微生物の培養温度は使用する微生物によりことなるが、5〜40℃、好ましくは20〜30℃とし、また20〜30℃にて培養して菌体を増殖せしめた後5〜20℃にて培養を続けて不飽和脂肪酸を生産せしめることもできる。このような温度管理によっても、生成脂肪酸中の高度不飽和脂肪酸の割合を上昇せしめることができる。培地のpHは4〜10、好ましくは5〜9として、通気攪拌培養、振盪培養、固体培養、又は静置液体培養を行う。本培養は通常2〜30日間、好ましくは5〜20日間、より好ましくは5〜15日間行う。 The culture temperature of microorganisms producing highly unsaturated fatty acids varies depending on the microorganisms used, but is 5-40 ° C, preferably 20-30 ° C, and after culturing at 20-30 ° C to grow the cells. Unsaturated fatty acids can also be produced by continuing the culture at 5 to 20 ° C. Such a temperature control can also increase the proportion of highly unsaturated fatty acids in the produced fatty acids. The pH of the medium is 4 to 10, preferably 5 to 9, and aeration stirring culture, shaking culture, solid culture, or stationary liquid culture is performed. The main culture is usually performed for 2 to 30 days, preferably 5 to 20 days, more preferably 5 to 15 days.
モルティエレラ属モルティエレラ亜属に属する微生物は、アラキドン酸を主たる構成脂肪酸として成る油脂(トリグリセリド)を産生しうる微生物として知られているが、本発明者らは、上記菌株に変異処理を施すことによって、ジホモ-γ-リノレン酸を主たる構成脂肪酸としてなる油脂(トリグリセリド)を産生しうる微生物(特開平5-91887)や、n-9系高度不飽和脂肪酸を主たる構成脂肪酸としてなる油脂(トリグリセリド)を産生しうる微生物を(特開平5-91888)得ている。さらに、高濃度の炭素源に耐性を有する微生物(WO 98/39468)も得ており、これら微生物は、モルティエレラ属モルティエレラ亜属の微生物である。しかし、本発明はモルティエレラ属モルティエレラ亜属に属する微生物に限定しているわけではなく、高度不飽和脂肪酸を構成脂肪酸として成る油脂(トリグリセリド)を産生しうる微生物を用いることができる。 Although microorganisms belonging to the genus Mortierella subgenus Mortierella are known as microorganisms capable of producing fats and oils (triglycerides) composed mainly of arachidonic acid, the present inventors apply mutation treatment to the above strains. , A microorganism capable of producing a fat (triglyceride) comprising dihomo-γ-linolenic acid as a main constituent fatty acid (Japanese Patent Laid-Open No. 5-91887), and a fat (triglyceride) comprising a n-9 polyunsaturated fatty acid as a main constituent fatty acid Has been obtained (JP-A-5-91888). Furthermore, microorganisms (WO 98/39468) having resistance to a high concentration of carbon source have also been obtained, and these microorganisms are microorganisms of the genus Mortierella. However, the present invention is not limited to microorganisms belonging to the genus Mortierella genus Mortierella, and microorganisms capable of producing fats and oils (triglycerides) comprising highly unsaturated fatty acids as constituent fatty acids can be used.
上記のように培養した微生物から、粗油を得る方法として、培養終了後、培養液をそのままかあるいは殺菌、濃縮、酸性化などの処理を施した後、自然沈降、遠心分離および/又は濾過などの常用の固液分離手段により培養菌体を得る。固液分離を助けるために、凝集剤や濾過助剤を添加してもよい。凝集剤としては、例えば、塩化アルミニウム、塩化カルシウム、アルギン、キトサンなどを使用できる。濾過助剤としては、例えば、珪藻土を使用できる。培養菌体は好ましくは、水洗、破砕、乾燥する。乾燥は、凍結乾燥、風乾、流動層乾燥、凍結乾燥などによって行うことができる。 As a method for obtaining crude oil from microorganisms cultured as described above, after culturing, the culture solution is left as it is or after treatment such as sterilization, concentration, and acidification, and then natural sedimentation, centrifugation, and / or filtration, etc. The cultured cells are obtained by conventional solid-liquid separation means. In order to assist solid-liquid separation, a flocculant or a filter aid may be added. As the flocculant, for example, aluminum chloride, calcium chloride, algin, chitosan and the like can be used. As a filter aid, for example, diatomaceous earth can be used. The cultured cells are preferably washed, crushed and dried. Drying can be performed by freeze drying, air drying, fluidized bed drying, freeze drying, or the like.
乾燥菌体から粗油を得る手段としては、有機溶剤による抽出法や圧搾法を用いることができるが、好ましくは窒素気流下で有機溶剤によって抽出する。有機溶剤としてはエタノール、ヘキサン、メタノール、エタノール、クロロホルム、ジクロロメタン、石油エーテル、アセトン等を用いることができ、またメタノールと石油エーテルの交互抽出やクロロホルム−メタノール−水の一層系の溶媒も用いることができる。しかしながら、粗油の取得に用いる抽出法を上記の方法に限定しているわけではなく、菌体内の油脂を効率的に抽出する手法はすべて使用することができる。例えば、超臨界抽出法なども有効な手段として使用することができる。 As a means for obtaining crude oil from dried cells, an extraction method with an organic solvent or a pressing method can be used, but extraction with an organic solvent is preferably performed under a nitrogen stream. As the organic solvent, ethanol, hexane, methanol, ethanol, chloroform, dichloromethane, petroleum ether, acetone, or the like can be used. Alternate extraction of methanol and petroleum ether or a single solvent of chloroform-methanol-water can also be used. it can. However, the extraction method used for obtaining the crude oil is not limited to the above-described method, and all methods for efficiently extracting the fats and oils in the cells can be used. For example, a supercritical extraction method or the like can also be used as an effective means.
有機溶剤や超臨界流体で抽出された抽出物から減圧下などの条件下で有機溶剤や超臨界流体成分を除去することにより、目的とする粗油を得ることができる。また、上記の方法に代えて湿菌体を用いてい抽出を行うことができる。この場合にはメタノール、エタノール、アセトン等の水に対して相溶性の溶媒、又はこれらと水及び/又は他の溶媒とからなる水に対して相溶性の混合溶媒を使用する。その他の手順は上記と同様である。
また、粗油だけでなく精製油脂をエステル交換の基質として用いることもできる。油脂精製工程として、脱ガム、脱酸、脱臭、脱色、カラム処理、分子蒸留、ウィンタリングなどの常法の工程を用いることができる。
The target crude oil can be obtained by removing the organic solvent and the supercritical fluid component from the extract extracted with the organic solvent and the supercritical fluid under conditions such as reduced pressure. Moreover, it can replace with said method and can extract using a wet microbial cell. In this case, a solvent compatible with water, such as methanol, ethanol, acetone, or the like, or a mixed solvent compatible with water composed of these and water and / or other solvents is used. Other procedures are the same as described above.
Moreover, not only crude oil but refined fats and oils can also be used as a substrate for transesterification. Conventional steps such as degumming, deoxidation, deodorization, decolorization, column treatment, molecular distillation, and wintering can be used as the oil refining step.
グリセライドからの脂肪酸組成物原料の調製
トリグリセライドなどのグリセライドから脂肪酸組成物原料を調製するには、例えば、鹸化又はリパーゼ分解等の方法を用いればよい。
(a)鹸化
鹸化は、水酸化ナトリウムなどの無機塩基を用いて常法に従って行えばよい。
Preparation of fatty acid composition raw material from glyceride To prepare a fatty acid composition raw material from glycerides such as triglyceride, a method such as saponification or lipase decomposition may be used.
(A) Saponification Saponification may be performed according to a conventional method using an inorganic base such as sodium hydroxide.
(b)リパーゼ分解法
この工程に用いるリパーゼは効率的に高度不飽和脂肪酸を多量に含む油脂を分解し、遊離の脂肪酸を効率的に生成する酵素であれば、特に問題なく使える。リパーゼによる加水分解反応の条件は以下の通りである。反応に加える水と原料油脂(TG)の量比は原料油脂に対して水は1/2以上であればよく、より好ましくは等量から5倍量の間、さらに好ましくは、等量から2倍量がよい。加水分解する温度も、使うリパーゼが作用できる温度であればよい。例えば、15から80℃の温度範囲があげられる。より好ましくは25-60℃、さらに好ましくは25-50℃がよい。酵素の添加量は予備的に検討し、目的の脂肪酸が遊離できる量であればよい。
(B) Lipase decomposition method The lipase used in this step can be used without any particular problem as long as it is an enzyme that efficiently decomposes fats and oils containing a large amount of highly unsaturated fatty acids and efficiently generates free fatty acids. The conditions for the hydrolysis reaction with lipase are as follows. The amount ratio of water and raw oil (TG) to be added to the reaction should be 1/2 or more of the raw oil and fat, more preferably between the equivalent amount and 5 times the amount, further preferably from the equivalent amount to 2 Double amount is good. The temperature for hydrolysis may be any temperature at which the lipase used can act. For example, the temperature range is 15 to 80 ° C. More preferably, it is 25-60 degreeC, More preferably, 25-50 degreeC is good. The amount of enzyme to be added is examined in advance, and may be any amount that can release the target fatty acid.
尿素包括法による飽和脂肪酸の除去
上記のようにして調製した脂肪酸組成物原料には、特定の目的とする高度不飽和脂肪酸を含めての不飽和脂肪酸のほかに、飽和脂肪酸も含まれているので、特定の目的とする高度不飽和脂肪酸を濃縮するに先立って、飽和脂肪酸を除去する。このための方法としては特に限定するものではないが、例えば、一般的に飽和脂肪酸の除去に用いられている尿素包括法(H.Traitler, et.al., J.Am. Oil Chem. Soc., 75, 755(1998))を用いてもよい。この場合、使う溶媒はアルコール(エチルアルコール、メチルアルコール、プロパノール等)が好ましい。
Removal of saturated fatty acids by the urea inclusion method The fatty acid composition raw material prepared as described above contains saturated fatty acids in addition to unsaturated fatty acids including specific unsaturated polyunsaturated fatty acids. Prior to concentrating the polyunsaturated fatty acid of interest for a particular purpose, the saturated fatty acid is removed. The method for this is not particularly limited. For example, the urea inclusion method (H. Traitler, et.al., J. Am. Oil Chem. Soc. 75, 755 (1998)). In this case, the solvent used is preferably an alcohol (ethyl alcohol, methyl alcohol, propanol, etc.).
目的とする特定の高度不飽和脂肪酸の濃縮
目的とする特定の高度不飽和脂肪酸を濃縮するため、本発明のおいては、上記のようにして調製した不飽和脂肪酸組成物原料に含まれる不飽和脂肪酸の内、目的とする特定の高度不飽和脂肪酸以外の不飽和脂肪酸を選択的にエステル化し、生成したエステルを除去することにより、目的とする特定の高度不飽和脂肪酸を遊離(非エステル化)脂肪酸として濃縮する。
Concentration of a specific highly unsaturated fatty acid of interest In order to concentrate a specific highly unsaturated fatty acid of interest, the unsaturated fatty acid composition raw material prepared as described above is used in the present invention. Of the fatty acids, unsaturated fatty acids other than the specific polyunsaturated fatty acid are selectively esterified, and the produced specific polyunsaturated fatty acids are liberated (unesterified) by removing the produced ester. Concentrate as fatty acid.
(a)エステル化基質
エステル化基質として、脂肪酸のほかにアルコールが必要である。このアルコールとして脂肪アルコールが使用され、好ましくは炭素原子数8〜16個の脂肪アルコールが使用される。炭素原子数12個のラウリルアルコールが好ましい。エステル化を脂肪酸に関して高収率で行うには、脂肪酸に対して1以上のモル量のアルコールを使用する必要があり、例えば全脂肪酸モル量に対して2倍モル量の脂肪アルコール、例えばラウリルアルコールを使用する。
(A) Esterification substrate In addition to the fatty acid, alcohol is required as the esterification substrate. A fatty alcohol is used as this alcohol, preferably a fatty alcohol having 8 to 16 carbon atoms. Lauryl alcohol having 12 carbon atoms is preferred. In order to carry out the esterification in high yields with respect to fatty acids, it is necessary to use one or more molar amounts of alcohol relative to the fatty acid, for example twice the amount of fatty alcohol relative to the total fatty acid molar amount, such as lauryl alcohol Is used.
(b)特異的リパーゼの選択
選択性が比較的高いとされるカンジダ(Candida)属微生物、特にカンジダ・ルゴサ(Candida rugosa)等、由来のリパーゼは炭素数が18以下で二重結合が2個以下の脂肪酸に特異的に作用するので、除去すべき脂肪酸の炭素原子数が20個以上の場合及び二重結合が3個以上の場合にはこのリパーゼを使用することができず、従って本願発明において使用することができない。
そこで本件発明者は、リパーゼの選択的エステル化を効率よくするため、選択的リパーゼのスクリーニングを行った。
(B) Selection of specific lipases Lipids derived from Candida genus microorganisms, especially Candida rugosa, which are considered to have relatively high selectivity, have 18 carbon atoms or less and two double bonds. Since it specifically acts on the following fatty acids, this lipase cannot be used when the number of carbon atoms of the fatty acid to be removed is 20 or more and when the number of double bonds is 3 or more. Cannot be used in
Therefore, the present inventor screened a selective lipase in order to efficiently perform selective esterification of the lipase.
即ち、各種脂肪酸のいずれかと、脂肪酸に対して2倍モル量のラウリルアルコールとに、種々の入手可能な公知の食品加工用リパーゼの内の1種を作用させ、2時間の反応の後に残留脂肪酸組成を算出し、オレイン酸への酵素活性を100として、各脂肪酸に対する酵素活性の相対値を求めた。使用したリパーゼは、下記のとおりであった。 That is, one of various available known food processing lipases is allowed to act on any one of various fatty acids and 2-fold molar amount of lauryl alcohol with respect to the fatty acid, and the residual fatty acid after the reaction for 2 hours. The composition was calculated, and the enzyme activity for oleic acid was taken as 100, and the relative value of enzyme activity for each fatty acid was determined. The lipases used were as follows:
(1)アルカリゲネス・スペーシス(Alcaligenes sp.)由来のリパーゼ(GLM)(名糖産業社製)
(2)ブルクホルデリア・セパシア(Burkholderia cepacia)〔旧名称:シュードモナス・スペーシス(Pseudomonas sp.)〕由来のリパーゼ(PS)(アマノエンザイム社製)
(3)シュードモナス・アエルギノサ(Pseudomonas aeruginisa)由来リパーゼ(LPL)(TOYOBO社製)
(4)シュードモナス・スツチェリ(Pseudomonas stutzeri)由来のリパーゼ(TL)(名糖産業社製)
(5)バークホルデリア・セパシア(Burkholderia cepacia)由来のリパーゼ(SL)(名糖産業社製)
(6)リゾプス・オリゼー(Rhizopus oryzae)由来のリパーゼ(タリパーゼ)(アマノエンザイム社製)
(7)カンジダ・ルゴサ(Candida rugosa)由来のリパーゼ(OF)(名糖産業社製)
(1) Lipase (GLM) derived from Alcaligenes sp.
(2) Lipase (PS) derived from Burkholderia cepacia (formerly Pseudomonas sp.) (Manufactured by Amano Enzyme)
(3) Pseudomonas aeruginisa derived lipase (LPL) (manufactured by TOYOBO)
(4) Lipase (TL) derived from Pseudomonas stutzeri (manufactured by Meito Sangyo Co., Ltd.)
(5) Lipase (SL) derived from Burkholderia cepacia (manufactured by Meito Sangyo Co., Ltd.)
(6) Lipase derived from Rhizopus oryzae (Talipase) (manufactured by Amano Enzyme)
(7) Candida rugosa-derived lipase (OF) (manufactured by Meito Sangyo Co., Ltd.)
結果を、下記表1に示す。
原料の微生物が生産した油脂の脂肪酸組成を前もって測定し、どの脂肪酸を除去したいかを明確にしたとき、上の表で示したリパーゼの内どの種類のリパーゼを使用すべきかが決まってくる。例えば、アラキドン酸を高含有する微生物油脂にはアラキドン酸の他に、DGLAやGLAが含まれている。先に述べたカンジダ・ルゴサ(Candida rugosa)のリパーゼはアラキドン酸とDGLA及びGLAに対する反応性はほぼ同等であり、この反応でアラキドン酸からDGLAやGLAを分別することは出来ない。 When the fatty acid composition of the fats and oils produced by the raw material microorganisms is measured in advance and it is clarified which fatty acid is desired to be removed, it is decided which kind of lipase from the lipases shown in the above table should be used. For example, microbial fats and oils containing a high amount of arachidonic acid contain DGLA and GLA in addition to arachidonic acid. The Candida rugosa lipase mentioned above has almost the same reactivity with arachidonic acid and DGLA and GLA, and DGLA and GLA cannot be separated from arachidonic acid by this reaction.
一方、ブルクホルデリア・セパシア(Burkholderia cepacia)〔旧名称:シュードモナス・スペーシス(Pseudomonas sp.)〕由来のリパーゼの反応性は、アラキドン酸とDGLA及びGLAとの間で大きく異なり、アラキドン酸に対する反応性はほぼ1/10である。この差を利用することで選択性が生まれ、高純度のアラキドン酸が得られることになる。従って、アラキドン酸の濃縮のためには、シュードモナスPseudomonas)属に由来し、アラキドン酸に対してよりもDGLA及びGLAに対して高い特異性を示すリパーゼが好ましい。 On the other hand, the reactivity of lipase derived from Burkholderia cepacia (former name: Pseudomonas sp.) Is significantly different between arachidonic acid and DGLA and GLA. Is almost 1/10. By utilizing this difference, selectivity is born and high purity arachidonic acid can be obtained. Therefore, for the concentration of arachidonic acid, lipases derived from the genus Pseudomonas) and exhibiting higher specificity for DGLA and GLA than for arachidonic acid are preferred.
また、微生物が作るDGLA含有油脂からDGLAを高純度化する場合には、別のリパーゼを使えばよい。DGLA含有油脂にはアラキドン酸がほとんど含まれず、除去する脂肪酸はGLAやリノール酸であり、DGLAとこれら脂肪酸との反応性が違うものはシュードモナス・アエルギノサ(Pseudomonas aeruginosa)由来のリパーゼであり、この酵素を選択的エステル化に用いることにより、DGLAの高純度化することが出来る。更に、DGLAの濃縮には、カンジダ・ルゴサ(Candida rugosa)由来のリパーゼも好ましい。従って、DGLAの濃縮には、シュードモナス・アエルギノサ(Pseudomonas aeruginosa)由来のリパーゼであって、DGLAに対してよりもGLAやリノール酸に高い特異性を有するリパーゼが好ましい。更に、カンジダ・ルゴサ(Candida rugosa)属由来のリパーゼも好ましい。これらのリパーゼは組み合わせて使用するのが好ましい。 Moreover, when DGLA is highly purified from DGLA-containing fats and oils produced by microorganisms, another lipase may be used. DGLA-containing fats and oils contain almost no arachidonic acid, and the fatty acids to be removed are GLA and linoleic acid. The lipase derived from Pseudomonas aeruginosa is different in the reactivity of DGLA and these fatty acids. Can be used for selective esterification to increase the purity of DGLA. Furthermore, lipase derived from Candida rugosa is also preferred for concentrating DGLA. Therefore, for enrichment of DGLA, a lipase derived from Pseudomonas aeruginosa and having a higher specificity for GLA and linoleic acid than for DGLA is preferred. Furthermore, lipases derived from the genus Candida rugosa are also preferred. These lipases are preferably used in combination.
ミード酸の濃縮に当っては、ブルクホルデリア・セパシア(旧名称:シュードモナス・スペーシス)由来のリパーゼを用いるのが好ましい。 In concentrating mead acid, it is preferable to use a lipase derived from Burkholderia cepacia (formerly Pseudomonas space).
エステル化された脂肪酸の除去
エステル化された脂肪酸は、当該エステル化された脂肪酸と目的とする特定の高度不飽和脂肪酸との理化学的性質の相違を利用して、エステルと遊離脂肪酸との間の分離に用いる常法を用いることができる。具体的には蒸留、溶剤抽出などを用いることができる。
例えば、蒸留によりエステル化された脂肪酸を蒸発除去することができる。また、ヘキサンなどの抽出溶剤を用いて、エステル化反応性生物から選択的にエステルを抽出除去すすることができる。
Removal of Esterified Fatty Acids Esterified fatty acids are used between esters and free fatty acids by taking advantage of the difference in physicochemical properties between the esterified fatty acids and the specific polyunsaturated fatty acids of interest. Conventional methods used for separation can be used. Specifically, distillation, solvent extraction, or the like can be used.
For example, fatty acids esterified by distillation can be removed by evaporation. Further, the ester can be selectively extracted from the esterification-reactive organism using an extraction solvent such as hexane.
濃縮された特定の高度不飽和脂肪酸の使用
上記の如く濃縮された高度不飽和脂肪酸は遊離型であり、用途に応じて分子形態を変えて使うことができる。例えば、香料のような使い方をする場合は、エチルエステル化して使ってもよいし、食用油脂に添加する場合はトリグリセライドの形にして添加しても問題ない。さらに、最近機能的に注目されているリン脂質の原料として使うことも可能である。
上記本発明の油脂、例えば、高純度のアラキドン酸、DGLA、ミード酸を含む油脂等の用途に関しては無限の可能性があり、食品、飲料、化粧品、医薬品の原料並びに添加物として使用することができる。そして、その使用目的、使用量に関して何ら制限を受けるものではない。
Use of Concentrated Specific Polyunsaturated Fatty Acids Polyunsaturated fatty acids concentrated as described above are free and can be used in various molecular forms depending on the application. For example, when used as a perfume, it may be used after ethyl esterification, or when added to edible fats and oils, there is no problem even if it is added in the form of triglyceride. Furthermore, it can also be used as a raw material for phospholipids that have recently attracted functional attention.
The oils and fats of the present invention, for example, fats and oils containing high-purity arachidonic acid, DGLA, mead acid, etc., have unlimited possibilities, and can be used as raw materials and additives for foods, beverages, cosmetics and pharmaceuticals. it can. And there is no restriction on the purpose and amount of use.
次に、例により、本発明をさらに具体的に説明する。しかし、本発明は、例に限定されない。
実施例1. アラキドン酸濃縮物の調製
(1)リパーゼによる分解
モルティエレラ・アルピナ(Mortierella alpina)から得られたアラキドン酸含有油(SUNTGA40S, トリアシルグリセロール)100gに200 gの水を加え、1800Uのリパーゼ(QLM:名糖産業)で40℃、72時間加水分解した。加水分解後、ヘキサンで遊離の脂肪酸を抽出し、ヘキサンをエバポレーターで除去した。
Next, the present invention will be described more specifically with reference to examples. However, the present invention is not limited to examples.
Example 1. Preparation of arachidonic acid concentrate (1) Degradation by lipase 200 g of water was added to 100 g of arachidonic acid-containing oil (SUNTGA40S, triacylglycerol) obtained from Mortierella alpina, and 1800 U of water was added. It was hydrolyzed with lipase (QLM: Meisho Sangyo) at 40 ° C for 72 hours. After hydrolysis, free fatty acids were extracted with hexane, and hexane was removed with an evaporator.
(2)尿素包括法による飽和脂肪酸の除去
前記(1)で調製した遊離脂肪酸組成物中に含まれる長鎖の飽和脂肪酸を尿素包括法により除去した。尿素包括に用いたアルコールを除去後、次のステップの選択的エステル化反応に供した。
(3)選択的エステル化(一回目)
選択的エステル化は同じリパーゼを用い、酵素力価を変えて2段階反応で行った。1回目の選択的酵素反応は、先の尿素包括で得た遊離脂肪酸に、その2倍量(モル比)のラウリルアルコールを加え、20U の選択的リパーゼ(Lipase PS)を添加して、30℃、16時間反応を行い、不要な脂肪酸をエステル化した。
(2) Removal of saturated fatty acid by urea inclusion method The long-chain saturated fatty acid contained in the free fatty acid composition prepared in the above (1) was removed by the urea inclusion method. After removing the alcohol used for urea inclusion, it was subjected to a selective esterification reaction in the next step.
(3) Selective esterification (first time)
Selective esterification was performed in a two-step reaction using the same lipase and varying the enzyme titer. In the first selective enzyme reaction, double the amount (molar ratio) of lauryl alcohol and 20 U of selective lipase (Lipase PS) were added to the free fatty acid obtained in the previous urea inclusion, and then 30 ° C. The reaction was carried out for 16 hours to esterify unnecessary fatty acids.
(4)エステル化脂肪酸の除去
この脂肪酸エステルをヘキサン抽出で除去した。残った水層を塩酸で酸性にして、もう一度ヘキサンで抽出して、さらに高純度化した遊離型アラキドン酸を得た。このときのアラキドン酸の純度は表2に示すように、85.7%に達した。
(4) Removal of esterified fatty acid This fatty acid ester was removed by hexane extraction. The remaining aqueous layer was acidified with hydrochloric acid and extracted once more with hexane to obtain further purified free arachidonic acid. The purity of arachidonic acid at this time reached 85.7% as shown in Table 2.
(5)選択的エステル化(2回目)
上記(4)で得た高純度のアラキドン酸を含む脂肪酸に1回目と同様の2倍量(モル比)のラウリルアルコールを加え、今回は高力価1回目より高力価である60U の選択的リパーゼ(Lipase PS)を添加して、30℃にて、16時間反応した。先の反応と同様にエステル化された脂肪酸をヘキサン抽出で除去して、残った水層から酸性条件下のヘキサン抽出で精製アラキドン酸を得た。48.9%の回収率で、96.6%の高純度の遊離型アラキドン酸を得た。実施例1で精製したアラキドン酸含有油脂の脂肪酸組成は表2に示す。
(1)DGLA含有脂肪酸組成物原料の調製
モルティエレラ(Mortierella)の変異株から得られたDGLA含有油(SUNTGD, トリアシルグリセロール)100gを、40 gの水酸化ナトリウム、80 gの水、および800 mlのエタノール混液を60℃まで加温した後に加え、窒素気流下で、時々攪拌しながら60℃で20分間保温した。800 mlの水を添加した後、pHが2以下になるまで濃塩酸を加え、室温まで冷却した。ここに存在する遊離脂肪酸を3000 mlのヘキサンで抽出した後、ヘキサン層を回収し、エバポレーターで脱溶媒した結果、92.1 gの遊離脂肪酸が得られた。
(5) Selective esterification (second time)
Add lauryl alcohol twice as much (molar ratio) to the fatty acid containing the high purity arachidonic acid obtained in (4) above, this time selecting 60U, which has a higher titer than the first. Lipase (Lipase PS) was added and reacted at 30 ° C. for 16 hours. The esterified fatty acid was removed by hexane extraction as in the previous reaction, and purified arachidonic acid was obtained from the remaining aqueous layer by hexane extraction under acidic conditions. With a recovery rate of 48.9%, 96.6% high purity free arachidonic acid was obtained. Table 2 shows the fatty acid composition of the oil containing arachidonic acid purified in Example 1.
(2)尿素付加による飽和脂肪酸の除去
100 gの尿素、14 mlの水、500 mlのメタノール、および92 gの上記遊離脂肪酸を混合し、尿素と遊離脂肪酸が完全溶解するまで60℃で攪拌した。引き続き攪拌しながら、6時間かけて4℃まで徐冷した。濾過により沈殿を除去後、得られた上清画分に0.1Mの塩酸水を500 ml添加した。さらに2000 mlのヘキサンで遊離脂肪酸を抽出した後、ヘキサン層を回収し、エバポレーターで脱溶媒した。その結果、53.0 gの遊離脂肪酸が得られた。この時の酸価は187.4 mg KOH/gであった。原料油、ケン化分解後、および尿素付加後の油の脂肪酸組成を表3に記載する。
(2) Removal of saturated fatty acids by urea addition
100 g of urea, 14 ml of water, 500 ml of methanol, and 92 g of the free fatty acid were mixed and stirred at 60 ° C. until the urea and free fatty acid were completely dissolved. The mixture was gradually cooled to 4 ° C. over 6 hours while stirring. After removing the precipitate by filtration, 500 ml of 0.1M aqueous hydrochloric acid was added to the resulting supernatant fraction. Furthermore, after extracting a free fatty acid with 2000 ml of hexane, the hexane layer was collect | recovered and the solvent was removed with the evaporator. As a result, 53.0 g of free fatty acid was obtained. The acid value at this time was 187.4 mg KOH / g. Table 3 shows the fatty acid composition of the raw oil, the oil after saponification decomposition, and the oil after urea addition.
尿素付加により飽和脂肪酸含量を減少させることができ、DGLA含量が59.9%にまで高められた。今後はこの尿素付加後の遊離脂肪酸をFFA-DGLA60と呼ぶことにする。 Saturated fatty acid content could be reduced by urea addition and DGLA content was increased to 59.9%. In the future, this free fatty acid after urea addition will be called FFA-DGLA60.
(3)リパーゼLPLによる不要脂肪酸の選択的エステル化(1回目)
0.71 gのFFA-DGLA60、0.89 gのラウリルアルコール(LauOH、脂肪酸に対して2倍モル)、0.4 gの水、および400 UのPseudomonas aeruginosa由来リパーゼ(TOYOBO社製、リパーゼLPL)からなる混液を、30℃で攪拌しながら反応させた。同じ反応液を7本作った。2, 4, 6, 8, 10, 14, 17時間後、反応液の遠心分離により油層を回収した。この油層中の酸価の減少量からエステル化率を算出した。またヘキサン抽出により油層から未反応の遊離脂肪酸を回収し、その脂肪酸組成をガスクロマトグラフィーで分析した。結果を表4に記載する。
(3) Selective esterification of unwanted fatty acids with lipase LPL (first time)
A mixed solution consisting of 0.71 g of FFA-DGLA60, 0.89 g of lauryl alcohol (LauOH, 2 times mol to fatty acid), 0.4 g of water, and 400 U of lipase derived from Pseudomonas aeruginosa (manufactured by TOYOBO, lipase LPL) The reaction was allowed to stir at 30 ° C. Seven identical reaction solutions were made. After 2, 4, 6, 8, 10, 14, 17 hours, the oil layer was recovered by centrifugation of the reaction solution. The esterification rate was calculated from the decrease in acid value in the oil layer. Unreacted free fatty acids were recovered from the oil layer by hexane extraction, and the fatty acid composition was analyzed by gas chromatography. The results are listed in Table 4.
エステル化率の上昇と共にC16:0, C18:0, C18:1, C18:2, GLA含量が減少し、DGLA含量が上昇した。これは、リパーゼLPLがC16:0, C18:0, C18:1, C18:2, GLAに作用しやすく、DGLAに作用しにくいため、未反応の遊離脂肪酸画分にDGLAが濃縮されるためである。エステル化率約60%の時、DGLA含量は最大の約82%に達した。 As the esterification rate increased, C16: 0, C18: 0, C18: 1, C18: 2, GLA content decreased and DGLA content increased. This is because lipase LPL is easy to act on C16: 0, C18: 0, C18: 1, C18: 2, GLA and is difficult to act on DGLA, so DGLA is concentrated in the unreacted free fatty acid fraction. is there. When the esterification rate was about 60%, the DGLA content reached a maximum of about 82%.
前報告(島田ら、科学と工業, Vol.73, p.125-130, 1999)では、アラキドン酸(AA)含有油から、Candida rugosa由来リパーゼ (名糖産業社製、リパーゼOF)による選択的エステル化によりAAを精製している。しかし、リパーゼOFのAA、GLA、DGLAに対する作用性がほぼ同等であるため、AA、GLA、DGLAが同じ未反応遊離脂肪酸画分に濃縮された。したがって、リパーゼOFをFFA-DGLA60に作用させたとすれば、GLAとDGLAが同じ未反応遊離脂肪酸画分に濃縮されると推定される。しかし、本実施例で用いたリパーゼLPLはGLAとDGLAを区別する(GLAには良く作用するがDGLAには作用しにくい)ため、GLAの除去を行うことができた。 In a previous report (Shimada et al., Science and Industry, Vol.73, p.125-130, 1999), selective use of arachidonic acid (AA) -containing oil by Candida rugosa-derived lipase (manufactured by Meito Sangyo Co., Ltd., lipase OF) AA is purified by esterification. However, since the activity of lipase OF on AA, GLA and DGLA is almost the same, AA, GLA and DGLA were concentrated in the same unreacted free fatty acid fraction. Therefore, if lipase OF is allowed to act on FFA-DGLA60, it is presumed that GLA and DGLA are concentrated in the same unreacted free fatty acid fraction. However, since the lipase LPL used in this example distinguishes GLA and DGLA (works well for GLA but hardly acts on DGLA), it was possible to remove GLA.
リパーゼLPLを用いた選択的エステル化によりGLAを除くことはできたが、C16:0, C18:0, C18:1の除去効率はあまり良くなかった。これらの脂肪酸の除去にはリパーゼLPLよりもリパーゼOFの方の効率が良いと予測した。そこで、リパーゼLPLを用いた選択的エステル化により未反応遊離脂肪酸画分を集めた後、リパーゼOFを用いた選択的エステル化を行うことにした。 GLA could be removed by selective esterification using lipase LPL, but the removal efficiency of C16: 0, C18: 0, C18: 1 was not very good. The removal of these fatty acids was predicted to be more efficient with lipase OF than with lipase LPL. Therefore, after the unreacted free fatty acid fraction was collected by selective esterification using lipase LPL, it was decided to perform selective esterification using lipase OF.
(4)リパーゼOFによる選択的エステル化(2回目)
試料の調製:20 gのFFA-DGLA60、25 gのLauOH、11.3 gの水、および11250 UのリパーゼLPLからなる混液を、30℃で攪拌しながら7時間反応させた。この時のエステル化率は45.8%であった。反応混液から未反応遊離脂肪酸をヘキサンにより抽出し、減圧下での脱溶媒により遊離脂肪酸11.6 gを得た。この標品のDGLA含量は77.6 wt%であったので、これをFFA-DGLA78と呼ぶことにする。
(4) Selective esterification with lipase OF (second time)
Sample preparation: A mixture of 20 g FFA-DGLA60, 25 g LauOH, 11.3 g water, and 11250 U lipase LPL was reacted at 30 ° C. with stirring for 7 hours. The esterification rate at this time was 45.8%. Unreacted free fatty acid was extracted from the reaction mixture with hexane, and 11.6 g of free fatty acid was obtained by desolvation under reduced pressure. Since this sample had a DGLA content of 77.6 wt%, it will be referred to as FFA-DGLA78.
0.71 gのFFA-DGLA78、0.89 gのLauOH、0.4 gの水、および400 UのリパーゼOFからなる混液を、30℃で攪拌しながら反応させた。同じ反応液を5本作った。4, 12, 24, 48, 72時間後、反応液の遠心分離により油層を回収した。この油層中の酸価の減少量からエステル化率を算出した。またヘキサン抽出により油層から未反応の遊離脂肪酸画分を回収し、脂肪酸組成をガスクロマトグラフィーで分析した。結果を表5に記載する。 A mixture consisting of 0.71 g of FFA-DGLA78, 0.89 g of LauOH, 0.4 g of water, and 400 U of lipase OF was reacted at 30 ° C. with stirring. Five identical reaction solutions were made. After 4, 12, 24, 48, and 72 hours, the oil layer was recovered by centrifugation of the reaction solution. The esterification rate was calculated from the decrease in acid value in the oil layer. Further, an unreacted free fatty acid fraction was recovered from the oil layer by hexane extraction, and the fatty acid composition was analyzed by gas chromatography. The results are listed in Table 5.
リパーゼOFを用いた選択的エステル化により、C16:0, C18:0, C18:1, C18:2が除去され、DGLA含量を約90%(89.8%)にまで高めることができた。 Selective esterification with lipase OF removed C16: 0, C18: 0, C18: 1, C18: 2 and increased the DGLA content to about 90% (89.8%).
実施例3. ミード酸濃縮物の調製
(1)MA含有脂肪酸組成物原料の調製
モルティエレラ(Mortierella)の変異株から得られたMA含有油(SUNTGM33, トリアシルグリセロール)100gを、40 gの水酸化ナトリウム、80 gの水、および800 mlのエタノール混液を60℃まで加温した後に添加し、窒素気流下で、時々攪拌しながら60℃で20分間保温した。800 mlの水を添加した後、pHが2以下になるまで濃塩酸を加え、室温まで冷却した。ここに存在する遊離脂肪酸を3000 mlのヘキサンで抽出した後、ヘキサン層を回収し、エバポレーターで脱溶媒した結果、93.0 gの遊離脂肪酸が得られた。
Example 3 Preparation of Mead Acid Concentrate (1) Preparation of MA-containing Fatty Acid Composition Raw Material 100 g of MA-containing oil (SUNTGM33, triacylglycerol) obtained from a mutant strain of Mortierella was added to 40 g of water. A mixture of sodium oxide, 80 g of water, and 800 ml of ethanol was added after heating to 60 ° C., and the mixture was kept at 60 ° C. for 20 minutes under nitrogen flow with occasional stirring. After adding 800 ml of water, concentrated hydrochloric acid was added until the pH was 2 or less, and the mixture was cooled to room temperature. The free fatty acid present therein was extracted with 3000 ml of hexane, and then the hexane layer was recovered and desolvated with an evaporator. As a result, 93.0 g of free fatty acid was obtained.
(2)尿素付加による飽和脂肪酸の除去
100 gの尿素、14 mlの水、500 mlのメタノール、および93 gの上記遊離脂肪酸を混合し、尿素と遊離脂肪酸が完全溶解するまで60℃で攪拌した。引き続き攪拌しながら、6時間かけて4℃まで徐冷した。濾過により沈殿を除去後、得られた上清画分に0.1Mの塩酸水を500 ml添加した。さらに2000 mlのヘキサンで遊離脂肪酸を抽出した後、ヘキサン層を回収し、エバポレーターで脱溶媒した。その結果、72.1 gの遊離脂肪酸が得られた。この時の酸価は187.9mg KOH/gであった。原料油、ケン化分解後、および尿素付加後の油の脂肪酸組成を表6に記載する。
(2) Removal of saturated fatty acids by urea addition
100 g of urea, 14 ml of water, 500 ml of methanol, and 93 g of the above free fatty acid were mixed and stirred at 60 ° C. until the urea and free fatty acid were completely dissolved. The mixture was gradually cooled to 4 ° C. over 6 hours while stirring. After removing the precipitate by filtration, 500 ml of 0.1M aqueous hydrochloric acid was added to the resulting supernatant fraction. Furthermore, after extracting a free fatty acid with 2000 ml of hexane, the hexane layer was collect | recovered and the solvent was removed with the evaporator. As a result, 72.1 g of free fatty acid was obtained. The acid value at this time was 187.9 mg KOH / g. Table 6 shows the fatty acid composition of the raw oil, the oil after saponification decomposition, and the oil after urea addition.
尿素付加によって飽和脂肪酸含量を減少させることができ、MA含量が41.2%にまで高められた。今後はこの尿素付加後の遊離脂肪酸をFFA-MA41と呼ぶことにする。 Saturated fatty acid content could be reduced by urea addition, increasing MA content to 41.2%. In the future, this free fatty acid after urea addition will be called FFA-MA41.
(3)リパーPSによる選択的エステル化(1回目)
0.71 gのFFA-MA41、0.89 gのLauOH(脂肪酸に対して2倍モル)、0.4 gの水、および400 Uのシュードモナス・スペーシス(Pseudomonas sp.)由来リパーゼ(アマノエンザイム製、リパーゼPS)からなる混液を、30℃で攪拌しながら反応させた。同じ反応液を7本作った。0.5, 1, 2, 3, 4, 6, 8時間後、反応液の遠心分離により油層を回収した。この油層中の酸価の減少量からエステル化率を算出した。またヘキサン抽出により油層から未反応の遊離脂肪酸を回収し、その脂肪酸組成をガスクロマトグラフィーで分析した。結果を表7に記載する。
(3) Selective esterification with Liper PS (first time)
Consists of 0.71 g of FFA-MA41, 0.89 g of LauOH (2-fold mol to fatty acid), 0.4 g of water, and 400 U of Pseudomonas sp. Lipase (manufactured by Amano Enzyme, Lipase PS) The mixed solution was reacted at 30 ° C. with stirring. Seven identical reaction solutions were made. After 0.5, 1, 2, 3, 4, 6, 8 hours, the oil layer was recovered by centrifugation of the reaction solution. The esterification rate was calculated from the decrease in acid value in the oil layer. Unreacted free fatty acids were recovered from the oil layer by hexane extraction, and the fatty acid composition was analyzed by gas chromatography. The results are listed in Table 7.
エステル化率の上昇と共にC16:0, C18:0, C18:1, C18:2, unknown 1, 2の含量が減少し、MA含量が上昇した。これは、リパーゼPSがC16:0, C18:0, C18:1, C18:2, unknown 1, 2に作用しやすく、MAに作用しにくいため、未反応の遊離脂肪酸画分にMAが濃縮されるためである。エステル化率約60%の時、MA含量は最大の約83%に達した。 As the esterification rate increased, the contents of C16: 0, C18: 0, C18: 1, C18: 2, unknown 1, 2 decreased, and the MA content increased. This is because lipase PS tends to act on C16: 0, C18: 0, C18: 1, C18: 2, unknown 1, 2 and hardly acts on MA, so MA is concentrated in the unreacted free fatty acid fraction. Because. When the esterification rate was about 60%, the MA content reached a maximum of about 83%.
(4)リパーゼPSによる選択的エステル化(2回目)
25 gのFFA-MA41、31 gのLauOH、14 gの水、および14000 UのリパーゼPSからなる混液を、30℃で攪拌しながら3時間反応させた。この時のエステル化率は57.6%であった。反応混液から未反応遊離脂肪酸をヘキサンにより抽出し、減圧下での脱溶媒により遊離脂肪酸11.4 gを得た。この標品のMA含量は79.2 wt%であったので、これをFFA-MA79と呼ぶことにする。
(4) Selective esterification with lipase PS (second time)
A mixed solution composed of 25 g of FFA-MA41, 31 g of LauOH, 14 g of water, and 14000 U of lipase PS was reacted at 30 ° C. with stirring for 3 hours. The esterification rate at this time was 57.6%. Unreacted free fatty acid was extracted from the reaction mixture with hexane, and 11.4 g of free fatty acid was obtained by desolvation under reduced pressure. Since the MA content of this sample was 79.2 wt%, it will be referred to as FFA-MA79.
0.71 gのFFA-MA79、0.89 gのLauOH、0.4 gの水、および400 UのリパーゼPSからなる混液を、30℃で攪拌しながら反応させた。同じ反応液を6本作った1, 2, 4, 7, 14, 21時間後、反応液の遠心分離により油層を回収した。この油層中の酸価の減少量からエステル化率を算出した。またヘキサン抽出により油層から未反応の遊離脂肪酸画分を回収し、脂肪酸組成をガスクロマトグラフィーで分析した。結果を表8に記載する。 A mixed solution composed of 0.71 g of FFA-MA79, 0.89 g of LauOH, 0.4 g of water, and 400 U of lipase PS was reacted at 30 ° C. with stirring. After 1, 2, 4, 7, 14, 21 hours when 6 identical reaction solutions were prepared, the oil layer was recovered by centrifugation of the reaction solution. The esterification rate was calculated from the decrease in acid value in the oil layer. Further, an unreacted free fatty acid fraction was recovered from the oil layer by hexane extraction, and the fatty acid composition was analyzed by gas chromatography. The results are listed in Table 8.
リパーゼPSを用いた2回目の選択的エステル化により、C16:0, C18:0, C18:1, C18:2, unknown 1, 2が除去され、MA含量を92.1%にまで高めることができた。 The second selective esterification with lipase PS removed C16: 0, C18: 0, C18: 1, C18: 2, unknown 1, 2 and increased the MA content to 92.1%. .
Claims (27)
(1)前記特定の高度不飽和脂肪酸に対する特異性が、他の高度不飽和脂肪酸に対する特異性よりも低いリパーゼ(特異的リパーゼ)を、脂肪アルコールの存在下で、前記特定の高度不飽和脂肪酸を含んで成る脂肪酸組成物に作用させることにより、前記特定の高度不飽和脂肪酸以外の脂肪酸を選択的にエステル化し;
(2)前記工程(1)で生じたエステルを除去して、前記特定の高度不飽和脂肪酸が濃縮された脂肪酸組成物を得;そして
(3)前記工程(1)において使用したリパーゼと同じリパーゼ又は異なるリパーゼを用いて、前記工程(1)及び(2)を反復する;
ことを含んで成る方法。 In the method for producing a fatty acid composition in which the ratio of a specific highly unsaturated fatty acid is 50% or more,
(1) A lipase (specific lipase) having a specificity for the specific polyunsaturated fatty acid is lower than that for the other polyunsaturated fatty acid, and the specific polyunsaturated fatty acid in the presence of a fatty alcohol. Selectively esterifying fatty acids other than the specific polyunsaturated fatty acids by acting on the fatty acid composition comprising;
(2) removing the ester produced in the step (1) to obtain a fatty acid composition enriched with the specific polyunsaturated fatty acid; and (3) the same lipase as the lipase used in the step (1). Or repeat steps (1) and (2) using different lipases;
A method comprising that.
(a)前記特定の高度不飽和脂肪酸の含有する脂肪酸組成物を用意し;そして
(b)尿素包括法により飽和脂肪酸を除去して、高度不飽和脂肪酸が濃縮された脂肪酸組成物を得る;
により得る、請求項1に記載の方法。 The fatty acid composition used in the step (1) is the following step:
(A) preparing a fatty acid composition containing the specific highly unsaturated fatty acid; and (b) removing the saturated fatty acid by the urea inclusion method to obtain a fatty acid composition enriched in the highly unsaturated fatty acid;
The method of claim 1 obtained by:
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