JP2010024165A - Krill protein-derived angiotensin converting enzyme inhibitor - Google Patents
Krill protein-derived angiotensin converting enzyme inhibitor Download PDFInfo
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- JP2010024165A JP2010024165A JP2008185773A JP2008185773A JP2010024165A JP 2010024165 A JP2010024165 A JP 2010024165A JP 2008185773 A JP2008185773 A JP 2008185773A JP 2008185773 A JP2008185773 A JP 2008185773A JP 2010024165 A JP2010024165 A JP 2010024165A
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- Coloring Foods And Improving Nutritive Qualities (AREA)
- Medicines That Contain Protein Lipid Enzymes And Other Medicines (AREA)
- Medicines Containing Material From Animals Or Micro-Organisms (AREA)
- Peptides Or Proteins (AREA)
Abstract
Description
本発明はアンジオテンシン変換酵素阻害活性を有し、血圧低下作用を有するペプチドを含有する組成物、その組成物を有効成分とするアンジオテンシン変換酵素阻害剤、およびその組成物を有効成分とする血圧低下剤および高血圧症の予防・改善に用いることのできる機能性食品に関する。 The present invention relates to a composition comprising a peptide having angiotensin converting enzyme inhibitory activity and having a blood pressure lowering action, an angiotensin converting enzyme inhibitor comprising the composition as an active ingredient, and a blood pressure reducing agent comprising the composition as an active ingredient. And a functional food that can be used for prevention and improvement of hypertension.
生体内の血圧調節はレニンーアンギオテンシン−アルドステロン(RAA)系、カリクレイン−キニン系、及びプロスタグランジン合成系等が相補的に関与していることが知られている。中でもRAA系は体液系での昇圧調節の中心的役割を担っているとされている。すなわち、肝臓で産生されたアンギオテンシノーゲンは腎由来の酵素レニンによって血中内で10アミノ酸残基のアンギオテンシン−Iに分解され、次いで主に肺に存在するアンギオテンシン−II変換酵素(ACE)の作用により8アミノ酸残基のアンギオテンシン−IIに変換される。アンギオテンシン−IIは生体内において最も強力な昇圧物質であり、血管平滑筋を収縮させる直接的昇圧作用を有しているだけでなく、副腎でのアルドステロン分泌を刺激し、ナトリウムや水の貯留量増大を引き起こし間接的な血圧上昇にも関与する。従って、RAA系の亢進阻害が血圧上昇抑制に有効であることが臨床的に知られており、薬物療法的にはカプトプリル等のACE阻害剤、あるいはロサルタン等のアンギオテンシン−IIレセプターアンタゴニストの使用が有効である。
近年、食品成分をターゲットとしたACE阻害性物質の研究が進み、種々のタンパク質由来ペプチドが有効なACE阻害活性、更には血圧降下作用を示すことが知られている(特許文献1−5等)。
It is known that renin-angiotensin-aldosterone (RAA) system, kallikrein-kinin system, prostaglandin synthesis system and the like are complementarily involved in blood pressure regulation in vivo. Above all, the RAA system is said to play a central role in regulating pressure in body fluid systems. That is, angiotensinogen produced in the liver is broken down into 10 amino acid residues of angiotensin-I in the blood by the kidney-derived enzyme renin, and then the action of angiotensin-II converting enzyme (ACE) mainly present in the lung Converts to 8 amino acid residues of angiotensin-II. Angiotensin-II is the most potent vasopressor in the body, not only has a direct vasopressor action to contract vascular smooth muscle, but also stimulates aldosterone secretion in the adrenal gland and increases sodium and water storage. Involved in indirect blood pressure increase. Therefore, it is clinically known that the inhibition of RAA system enhancement is effective in suppressing blood pressure elevation, and the use of ACE inhibitors such as captopril or angiotensin-II receptor antagonists such as losartan is effective for pharmacotherapy. It is.
In recent years, research on ACE-inhibiting substances targeting food ingredients has progressed, and it is known that various protein-derived peptides exhibit effective ACE-inhibiting activity and further blood pressure lowering action (Patent Documents 1-5, etc.) .
本発明は、副作用がなく安全で、血圧低下作用を有し、医薬品や食品として摂取することができる血圧低下成分を提供することを目的とする。 An object of the present invention is to provide a blood pressure lowering component that is safe without side effects, has a blood pressure lowering action, and can be taken as a pharmaceutical or food.
各種タンパク質由来のペプチドにアンジオテンシン変換酵素阻害活性があることが知られている。本出願人は、先にオキアミから得たトリペプチド(Leu-Lys-Tyr)がアンジオテンシンI転換酵素(ACE)阻害活性を有することを見出している(特許文献1)。本発明はさらに有効なACE阻害剤を見出すため、オキアミを各種分解酵素で分解し、それらに含まれるペプチドを検討し、本願発明を完成させた。 It is known that peptides derived from various proteins have angiotensin converting enzyme inhibitory activity. The present applicant has previously found that a tripeptide (Leu-Lys-Tyr) obtained from krill has an angiotensin I converting enzyme (ACE) inhibitory activity (Patent Document 1). In order to find a more effective ACE inhibitor in the present invention, krill was decomposed with various degrading enzymes, and peptides contained therein were studied to complete the present invention.
本発明は、(1)〜(3)のアンジオテンシン変換酵素阻害剤、及び、(4)〜(6)の血圧降下剤、機能性食品を要旨とする。
(1)下記(i)ないし(xiii)のアミノ酸配列を有するペプチド又はその塩のいずれか1種以上を有効成分として含有するアンジオテンシン変換酵素阻害剤。
(i)Ile−Thr−Arg−Tyr
(ii)Val−Phe−Glu−Arg
(iii)Ile−Trp−Ala−Lys
(iv)Val−Asp−Tyr
(v)Ala−Leu−Pro−His
(vi)Phe−Glu−Gln
(vii)Ile−Thr−Ala
(viii)Leu−Gly−Asp−Tyr−Asn
(ix)Phe−Asn−Pro
(x)Val−Asp−Pro
(xi)Val−Tyr−Glu−Gly
(xii)Phe−Arg−Ala−Gly
(xiii)Ile−Ile−Gly−Glu−Tyr
The gist of the present invention is the angiotensin converting enzyme inhibitor (1) to (3), the antihypertensive agent (4) to (6), and a functional food.
(1) An angiotensin converting enzyme inhibitor comprising as an active ingredient any one or more of peptides having the amino acid sequences of (i) to (xiii) below or salts thereof:
(I) Ile-Thr-Arg-Tyr
(Ii) Val-Phe-Glu-Arg
(Iii) Ile-Trp-Ala-Lys
(Iv) Val-Asp-Tyr
(V) Ala-Leu-Pro-His
(Vi) Phe-Glu-Gln
(Vii) Ile-Thr-Ala
(Viii) Leu-Gly-Asp-Tyr-Asn
(Ix) Phe-Asn-Pro
(X) Val-Asp-Pro
(Xi) Val-Tyr-Glu-Gly
(Xii) Phe-Arg-Ala-Gly
(Xiii) Ile-Ile-Gly-Glu-Tyr
(2)オキアミタンパク質の蛋白質分解酵素による分解物からなる(1)のアンジオテンシン変換酵素阻害剤。
(3)蛋白質分解酵素がサーモライシンである(2)のアンジオテンシン変換酵素阻害剤。
(2) The angiotensin converting enzyme inhibitor according to (1), comprising a degradation product of a krill protein by a proteolytic enzyme.
(3) The angiotensin converting enzyme inhibitor according to (2), wherein the proteolytic enzyme is thermolysin.
(4)(1)ないし(3)いずれかのアンジオテンシン変換酵素阻害剤を有効成分とする血圧降下剤。
(5)(1)ないし(3)いずれかのアンジオテンシン変換酵素阻害剤を含有する機能性食品。
(6)高血圧症の予防・改善に有効であることを表示した食品である(5)の機能性食品。
(4) An antihypertensive agent comprising the angiotensin converting enzyme inhibitor according to any one of (1) to (3) as an active ingredient.
(5) A functional food containing any one of the angiotensin converting enzyme inhibitors (1) to (3).
(6) The functional food according to (5), which is a food indicating that it is effective in preventing and improving hypertension.
本発明のペプチドはアンジオテンシン変換酵素阻害活性を有し、経口投与により血圧低下作用を有するので、経口投与で高血圧の予防、治療に有効である。 Since the peptide of the present invention has an angiotensin converting enzyme inhibitory activity and has a blood pressure lowering effect by oral administration, it is effective for prevention and treatment of hypertension by oral administration.
本発明においてオキアミとは資源量が豊富な南極オキアミ(Euphausia pacifica)が好ましいが、その他のオキアミでも同様に使用できる。本発明の活性成分は、これらオキアミのタンパク質をタンパク質分解酵素で分解したペプチドである。
本発明のオキアミタンパク質の酵素分解物は、オキアミを酵素処理に適するように前処理したうえで、蛋白質分解酵素処理しペプチドを生成させ、これを必要に応じて、分離、濾過、濃縮、殺菌処理することによって得ることができる。
In the present invention, krill is preferably Antarctic krill (Euphausia pacifica), which has abundant resources, but other krill can be used as well. The active ingredient of the present invention is a peptide obtained by degrading these krill proteins with a proteolytic enzyme.
The enzyme degradation product of the krill protein of the present invention is pretreated so that the krill is suitable for enzyme treatment, and then proteolytic enzyme treatment is performed to produce a peptide, which is separated, filtered, concentrated and sterilized as necessary. Can be obtained.
本発明の組成物はオキアミを原料として製造するものであるが、頭や殻がついたままでも、頭や殻を除去したものでもどちらでもかまわない。処理しやすいのは頭や殻を除去した剥き身である。剥き身であればそのまま酵素処理にかけることができる。頭や殻付きの場合でも、そのままあるいは裁断して酵素処理することができる。好ましくはホモジナイザーなどで裁断すると効率よく酵素処理することができる。酵素処理後、分解しなかった殻などを濾過などにより除去する。 The composition of the present invention is produced from krill as a raw material, but it may be either with the head and shell attached or with the head and shell removed. Easy to handle is stripped skin with the head and shell removed. If it is stripped, it can be directly subjected to enzyme treatment. Even with a head or shell, the enzyme treatment can be performed as it is or after cutting. Preferably, the enzyme treatment can be efficiently performed by cutting with a homogenizer or the like. After the enzyme treatment, the shells that have not been decomposed are removed by filtration or the like.
酵素処理は、原料重量に対して1/2量〜20倍量、好ましくは等量〜10倍量の加水を行った後、アンモニア水、水酸化ナトリウム(カリウム)水溶液等アルカリ剤を加えて、使用する蛋白分解酵素の適値にpHを調整し、温度も酵素適温(使用酵素によって異なるが、20〜65℃、室温でも十分に反応する)に加温し、蛋白分解酵素を加えて30分〜30時間(好ましくは5〜20時間)処理する。 Enzyme treatment is carried out by adding 1/2 to 20 times, preferably 10 to 10 times the amount of the raw material, and then adding an alkaline agent such as aqueous ammonia or sodium hydroxide (potassium) solution, Adjust the pH to the appropriate value for the proteolytic enzyme to be used, warm the temperature to the appropriate enzyme temperature (depending on the enzyme used, 20-65 ° C, reacts well even at room temperature), add the proteolytic enzyme, and add 30 minutes Treat for ~ 30 hours (preferably 5-20 hours).
蛋白分解酵素としては、中性又はアルカリ性条件下で蛋白質を分解し得る酵素であればすべての酵素が単独で又は混合して使用し得る。その起源は、動植物のほかに微生物に求めることができ、ペプシン、レニン、トリプシン、キモトリプシン、パパイン、ブロメレインのほか、細菌プロテアーゼ、糸状菌プロテアーゼ、放線菌プロテアーゼ等も広く利用できる。これらの酵素は、通常、市販されているものが使用されるが、未精製の酵素、酵素を含有した培養液、麹といった固体又は液体の酵素含有物も、目的により必要に応じて使用することができる。酵素の添加量としては0.1%〜5.0%程度でよい。
好ましい蛋白分解酵素としては、Aspergillus oryzae属菌株由来プロテアーゼ、Bacillus subtilis属菌株由来プロテアーゼ、Aspergillus oryzae属菌株由来プロテアーゼ、Aspergillus melleus属菌株由来プロテアーゼ、Bacillus stearothermophilus属菌株由来プロテアーゼ、Bacillus subtilis属菌株由来プロテアーゼ、Rhizopus oryzae属菌株由来ペプチダーゼ、Aspergillus oryzae属菌株由来ペプチダーゼなどが例示される。特に好ましいのは、Bacillus stearothermophilus属菌株由来プロテアーゼであるサーモライシンである。
As the proteolytic enzyme, all enzymes can be used alone or in combination as long as they are capable of degrading proteins under neutral or alkaline conditions. Its origin can be found in microorganisms in addition to animals and plants, and in addition to pepsin, renin, trypsin, chymotrypsin, papain, bromelain, bacterial protease, filamentous fungal protease, actinomycete protease, etc. can be widely used. These enzymes are usually commercially available. However, unpurified enzymes, enzyme-containing culture fluids, and solid or liquid enzyme-containing materials such as sputum should also be used as required. Can do. The amount of enzyme added may be about 0.1% to 5.0%.
Preferred proteases include Aspergillus oryzae genus protease, Bacillus subtilis genus protease, Aspergillus oryzae genus protease, Aspergillus melleus genus protease, Bacillus stearothermophilus genus protease, Bacillus subtilis genus protease, Rhizopus Examples include peptidases derived from oryzae strains, peptidases derived from Aspergillus oryzae strains, and the like. Particularly preferred is thermolysin, which is a protease derived from the genus Bacillus stearothermophilus.
酵素処理後、必要あれば中和処理を行った後、70℃(好適には80℃)以上の温度に2〜60分間(好適には5〜30分間)保持し、酵素を失活させるとともに後に行う分離を良好ならしめる。加熱失活処理後、ハイブロスクリーン等による濾過によって粗分離し、必要によりジェクター処理した後、遠心分離処理して、浮遊物、沈殿物を除去する。そのままでもアンジオテンシン転換酵素阻害活性を有するのでそのまま用いてもよいが、原料由来の独特の味や臭いがあるので、使用目的によってはさらに濾過、活性炭処理などにより、脱臭、脱色、精製する。殺菌、噴霧乾燥、凍結乾燥なども必要に応じて行う。 After the enzyme treatment, neutralization treatment is performed if necessary, and then kept at a temperature of 70 ° C. (preferably 80 ° C.) for 2 to 60 minutes (preferably 5 to 30 minutes) to deactivate the enzyme. Ensure good separation later. After heat deactivation treatment, it is roughly separated by filtration with a hybro screen or the like, and if necessary, subjected to a jet treatment and then centrifuged to remove suspended matters and precipitates. Since it has angiotensin converting enzyme inhibitory activity as it is, it may be used as it is, but since it has a unique taste and smell derived from the raw material, it is further deodorized, decolorized and purified by filtration, activated carbon treatment, etc. depending on the purpose of use. Sterilization, spray drying, freeze drying, etc. are performed as necessary.
本発明のオキアミタンパク質の蛋白質酵素分解物を有効成分とするアンジオテンシン変換酵素阻害剤は実施例に示すようにすぐれたACE阻害活性を有することが確認されたので、ACE阻害剤、あるいは、血圧降下を目的とした医薬品、健康食品、特に特定保健用食品としても使用することができる。食品として使用する場合には、酵素分解物をそのまま添加したり、他の食品ないしは食品成分と併用したりして適宜常法にしたがって使用できる。常法にしたがい、錠剤、顆粒剤、粉末剤、カプセル剤、散剤とすることができる。
本発明のアンジオテンシン転換酵素阻害剤であるオキアミタンパク質酵素分解物の使用のめやすは、約0.1〜6000mg/日であり、1日に1〜2回経口投与するのが好ましい。また必要ある場合には、他の薬剤との併用も可能である。本発明のオキアミタンパク質の蛋白質酵素分解物は食品として長い食経験のあるオキアミの酵素分解物であり、安全性が高く、安心して使用できる。
Since the angiotensin converting enzyme inhibitor comprising the protein enzyme degradation product of the krill protein of the present invention as an active ingredient was confirmed to have excellent ACE inhibitory activity as shown in the Examples, it was confirmed that the ACE inhibitor or blood pressure lowering was achieved. It can also be used as the intended medicine, health food, especially food for specified health use. When used as a food, the enzyme degradation product can be added as it is, or used in combination with other foods or food ingredients as appropriate according to conventional methods. According to a conventional method, tablets, granules, powders, capsules and powders can be prepared.
The standard for using the krill protein enzyme degradation product, which is an angiotensin converting enzyme inhibitor of the present invention, is about 0.1 to 6000 mg / day, and is preferably orally administered once or twice a day. If necessary, it can be used in combination with other drugs. The enzyme-decomposed product of krill protein of the present invention is an enzyme-decomposed product of krill that has a long dietary experience as food, and is highly safe and can be used with confidence.
以下に本発明の実施例を記載するが、本発明はこれらに何ら限定されるものではない。 Examples of the present invention will be described below, but the present invention is not limited thereto.
オキアミタンパク質由来ペプチド粉末の製造
オキアミ剥き身1kg(日本水産株式会社製)に等量の水を加え、70℃になるまで加温した後に、オキアミ剥き身に対して重量比0.15%となるようにサモアーゼPC-10F(天野エンザイム社製)を加え、攪拌しながら70℃で20時間の酵素反応を行った。酵素反応の後に100℃で30分間保温し酵素を失活させた。遠心分離及び濾過による残渣の除去後、エバポレーターを用いた濃縮を行い、スプレードライを用いてペプチド乾燥粉末体を得た(75g)(本発明品)。ペプチド粉末は使用するまで-20℃で保存した。
Manufacture of Krill Protein-Derived Peptide Powder After adding an equal amount of water to 1 kg of krill flakes ( manufactured by Nihon Suisan Co., Ltd.) and heating to 70 ° C, Samoaase PC is 0.15% by weight with respect to the krill flakes -10F (manufactured by Amano Enzyme) was added, and the enzyme reaction was performed at 70 ° C. for 20 hours with stirring. After the enzyme reaction, the enzyme was inactivated by incubating at 100 ° C. for 30 minutes. After removal of the residue by centrifugation and filtration, concentration using an evaporator was performed, and a peptide dry powder was obtained using spray drying (75 g) (product of the present invention). The peptide powder was stored at -20 ° C until use.
ゲル電気泳動分析
得られたオキアミタンパク質由来ペプチドの分子量分布を調べるために、SMART system(GE healthcare bioscience)上で、Superdex Peptide PC 3.2/30ゲル濾過カラム(GE
healthcare bioscience)を用いたゲル濾過クロマトグラフィーを行った。溶媒には、150 mM NaCl、6 Mグアニジン塩酸塩を含む50 mMリン酸緩衝液(pH 7.4)を用いて行い、サイズスタンダードとして、cytochrome C, aprotinin, gastrin I, bradykinin, varyl-tyrosine及びグリシンを用いて行った。
ゲル濾過クロマトグラフィーの結果、オキアミタンパク質由来ペプチドは、分子量10,000以下に分布していることが確認された(図1)。これはタンパク質が十分に分解されている状態である。
Gel electrophoresis analysis In order to examine the molecular weight distribution of the peptide derived from krill protein, a Superdex Peptide PC 3.2 / 30 gel filtration column (GE) was used on the SMART system (GE healthcare bioscience).
gel filtration chromatography using healthcare bioscience). As a solvent, 50 mM phosphate buffer (pH 7.4) containing 150 mM NaCl and 6 M guanidine hydrochloride is used. Used.
As a result of gel filtration chromatography, it was confirmed that the krill protein-derived peptide was distributed with a molecular weight of 10,000 or less (FIG. 1). This is a state where the protein is sufficiently degraded.
アンギオテンシン変換酵素(ACE)阻害活性の測定
ウサギ肺由来ACE、ACEの基質であるN-[3-(Furyl)acryloyl]-Phe-Gly-Gly(FAPGG)、及び陽性対照として用いたバリルチロシンはSigma社製を用いた。ACE阻害活性の測定はPetersonらの方法(Anal. Biochem. 125; 420-426 (1982))を改変して行った。すなわち、18 μLの250 mM HEPES pH 8.3、1.5 M NaCl、10 μLの90 μg/mLに調製したACE、及び適宜希釈した被験物質を混合し90 μLとし室温で15分間、室温でプレインキュベーションを行った。次いで、上記反応液に10 μLの50 mM HEPES pH 8.3、300 mM NaCl及び1.5 mM FAPGGを加え室温で2-3時間、インキュベーションを行った。阻害活性の測定は320 nmの吸光度を測定することで行い、ACEを50%阻害する被験物質量をIC50として阻害活性を表した。
実施例1において製造した本発明品のオキアミタンパク質由来ペプチドのACE阻害活性は、IC50で約1.9 mg/mLであった。
Measurement of angiotensin converting enzyme (ACE) inhibitory activity Rabbit lung ACE, ACE substrate N- [3- (Furyl) acryloyl] -Phe-Gly-Gly (FAPGG), and valyltyrosine used as a positive control is Sigma The product made by company was used. The ACE inhibitory activity was measured by modifying the method of Peterson et al. (Anal. Biochem. 125; 420-426 (1982)). That is, 18 μL of 250 mM HEPES pH 8.3, 1.5 M NaCl, 10 μL of ACE prepared at 90 μg / mL, and an appropriately diluted test substance were mixed to make 90 μL and preincubated at room temperature for 15 minutes at room temperature. It was. Next, 10 μL of 50 mM HEPES pH 8.3, 300 mM NaCl, and 1.5 mM FAPGG were added to the reaction solution, followed by incubation at room temperature for 2-3 hours. The inhibitory activity was measured by measuring the absorbance at 320 nm, and the inhibitory activity was expressed with IC 50 as the amount of the test substance that inhibits ACE by 50%.
The ACE inhibitory activity of the peptide derived from the krill protein of the present invention produced in Example 1 was about 1.9 mg / mL with an IC 50 .
単回経口投与によるオキアミ由来ペプチドの降圧作用
本試験には7週齢雌性ラット(SHR/Izm、SPF)(日本エスエルシー)を用いた。ラットは室温22±3℃、相対湿度50±20%、照明時間12時間/日、換気回数13-17回/時間の条件下で固型飼料(ラボMRストック(日本農産工業製))を与えて飼育し飲料水は自由に接種させた。
7週齢のラットを上記の環境で1週間予備飼育し馴化して収縮期血圧がほぼ同一になるように群分けを行った(各群6尾)。群分けの後に一晩絶食させたラットに被験物質を強制的に単回経口投与し、投与2、4、6、8及び24時間後に小動物無加温型非観血圧計MK-2000(室町機械製)で血圧及び心拍数の測定を行った。被験物質としては、実施例1において製造したオキアミタンパク質由来ペプチド粉末を水溶液とし、1 mg/kg、10 mg/kg及び100 mg/kg投与群で行った。コントロール群には同量の水を投与した。)
Antihypertensive effect of krill-derived peptide after single oral administration In this study, 7-week-old female rats (SHR / Izm, SPF) (Japan SLC) were used. Rats were given solid feed (Lab MR Stock (Nippon Agricultural Industries)) under conditions of room temperature 22 ± 3 ° C, relative humidity 50 ± 20%, lighting time 12 hours / day, ventilation rate 13-17 times / hour. Breeding and drinking water was inoculated freely.
Seven-week-old rats were preliminarily bred for 1 week in the above environment and acclimated to perform grouping so that the systolic blood pressure was almost the same (6 mice in each group). Rats fasted overnight after grouping were forcibly administered a single oral dose of test substance, and 2, 4, 6, 8 and 24 hours after administration, small animal non-warming type non-invasive blood pressure monitor MK-2000 (Muromachi Kikai) Blood pressure and heart rate were measured. As a test substance, the krill protein-derived peptide powder produced in Example 1 was used as an aqueous solution in 1 mg / kg, 10 mg / kg and 100 mg / kg administration groups. The same amount of water was administered to the control group. )
1、10若しくは100 mg/kgのオキアミタンパク質由来ペプチドの投与群で、投与2時間後の収縮期血圧の低下量はそれぞれ、17 ± 1.59 mmHg、28 ± 4.97 mmHg及び24 ± 4.15 mmHgであり、有意な低下がみられた(図2)。その後、収縮期血圧は8時間後にほぼ元の値に戻った。また、オキアミタンパク質由来ペプチド投与群及び対照区において、オキアミタンパク質由来ペプチド投与後の心拍数に有意な差はみられなかった。
In the administration group of 1, 10, or 100 mg / kg krill protein-derived peptide, the decrease in
ACE阻害ペプチドの単離及び構造解析
ペプチド粉末を26.5 mMのギ酸に溶解させた後にAKTAexplorer 100システム(GE healthcare bioscience)上でSP10/16XL陽イオン交換カラム(GE healthcare bioscience)を用いたイオン交換クロマトグラフィーに供した。溶出は0-1 M NaClの直線グラジエントで行い、クロマトグラフィーの流速は2 mL/分で行った。また、溶出ペプチドのモニタリングは214 nmの吸光度を測定することで行った。ACE阻害活性の高かった画分を凍結乾燥し、ゲル濾過クロマトグラフィーに供した。ゲル濾過クロマトグラフィーは、凍結乾燥した画分を蒸留水に溶解させた後に、AKTAexplorer 100システム上でSuperdex Peptide 10/300 GLゲル濾過カラム(GE healthcare bioscience)を用いて行った。溶出には蒸留水を用いて行い、流速は0.9 mL/分で行った。溶出ペプチドのモニタリングは214 nmの吸光度を測定することで行った。最もACE阻害活性の高かった画分を凍結乾燥した後に26.5 mMのギ酸に溶解し、SMART system上でODS-80TM column (Tosoh corp.)カラムを用いた逆相クロマトグラフィーを行った。溶出は0-40%アセトニトリルの直線グラジエントで行い、流速は0.5 mL/分で行った。溶出ペプチドのモニタリングは214 nmの吸光度を測定することで行った。ACE阻害活性の高かった画分を凍結乾燥した後に0.1%トリフルオロ酢酸に溶解し、μRPC C2/C18 SC 2.1/10カラム(GE healthcare bioscience)を用いてペプチドの単離を行った。単離したペプチドはProcise 494 HTシークエンサー(Applied biosystems)を用いて、配列決定を行った。
Isolation and structural analysis of ACE inhibitory peptide Ion exchange chromatography using SP10 / 16XL cation exchange column (GE healthcare bioscience) on
結果
オキアミタンパク質由来ペプチドの陽イオン交換クロマトグラフィー及び各フラクションのACE阻害活性を図3に示した。ACE阻害活性の高かったフラクション24-25を次いでゲル濾過クロマトグラフィーに供した。フラクション24-25のゲル濾過クロマトグラフィー及び各フラクションのACE阻害活性を図4に示した。ACE阻害活性の高かったフラクション19を次いで逆相クロマトグラフィーに供した。溶出フラクションのACE阻害活性を図5に示した。得られたACE阻害活性ピークI-VIに含まれるペプチドを単離し、アミノ酸シークエンサーによる構造解析に供した。得られたペプチドシークエンスは、Ile−Thr−Arg−Tyr、Val−Trp、Val−Phe−Glu−Arg、Ile−Trp−Ala−Lys、Leu−Lys−Tyr、Val−Asp−Tyr、Ala−Leu−Pro−His、Phe−Glu−Gln、Ile−Thr−Ala、Leu−Gly−Asp−Tyr−Asn、Phe−Asn−Pro、Val−Asp−Pro、Val−Tyr−Glu−Gly、Phe−Arg−Ala−Gly、Ile−Ile−Gly−Glu−Tyrであった。
中でも、ピークII及びIIIに含まれていたVal−TrpおよびLeu−Lys−Tyrが高いACE阻害活性を示し(それぞれのIC50 = 2.75μg/mLおよび4.02μg/mL)、これらがオキアミタンパク質由来ペプチドの血圧降下作用に大きく寄与していることが考えられた。
Results Cation exchange chromatography of the krill protein-derived peptide and the ACE inhibitory activity of each fraction are shown in FIG. Fractions 24-25 with high ACE inhibitory activity were then subjected to gel filtration chromatography. The gel filtration chromatography of fractions 24-25 and the ACE inhibitory activity of each fraction are shown in FIG.
Among them, Val-Trp and Leu-Lys-Tyr contained in Peaks II and III showed high ACE inhibitory activity (IC 50 = 2.75 μg / mL and 4.02 μg / mL, respectively), and these were peptides derived from krill protein. It was thought that this greatly contributed to the blood pressure lowering action of the blood.
本発明のオキアミタンパク質の酵素分解物はアンジオテンシン変換酵素阻害剤を有し、血圧降下作用を有するので高血圧症の治療・予防薬を提供することができる。 Since the enzyme degradation product of krill protein of the present invention has an angiotensin converting enzyme inhibitor and has a blood pressure lowering effect, it can provide a therapeutic / preventive agent for hypertension.
Claims (6)
(i)Ile−Thr−Arg−Tyr
(ii)Val−Phe−Glu−Arg
(iii)Ile−Trp−Ala−Lys
(iv)Val−Asp−Tyr
(v)Ala−Leu−Pro−His
(vi)Phe−Glu−Gln
(vii)Ile−Thr−Ala
(viii)Leu−Gly−Asp−Tyr−Asn
(ix)Phe−Asn−Pro
(x)Val−Asp−Pro
(xi)Val−Tyr−Glu−Gly
(xii)Phe−Arg−Ala−Gly
(xiii)Ile−Ile−Gly−Glu−Tyr An angiotensin converting enzyme inhibitor comprising as an active ingredient any one or more of peptides having the amino acid sequences of (i) to (xiii) below or salts thereof:
(I) Ile-Thr-Arg-Tyr
(Ii) Val-Phe-Glu-Arg
(Iii) Ile-Trp-Ala-Lys
(Iv) Val-Asp-Tyr
(V) Ala-Leu-Pro-His
(Vi) Phe-Glu-Gln
(Vii) Ile-Thr-Ala
(Viii) Leu-Gly-Asp-Tyr-Asn
(Ix) Phe-Asn-Pro
(X) Val-Asp-Pro
(Xi) Val-Tyr-Glu-Gly
(Xii) Phe-Arg-Ala-Gly
(Xiii) Ile-Ile-Gly-Glu-Tyr
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Cited By (5)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| JP2017043618A (en) * | 2015-08-26 | 2017-03-02 | 三井農林株式会社 | Dipeptidyl peptidase-IV inhibitor |
| KR101823045B1 (en) * | 2016-05-13 | 2018-01-31 | 전남대학교산학협력단 | A composition containing krill protein hydrolysate for treating and preventing hypertension, health functional food containg the same and manufacturing mehod thereof |
| CN114507702A (en) * | 2022-02-03 | 2022-05-17 | 中国海洋大学 | A kind of marine Antarctic krill peptide and its application |
| CN118388590A (en) * | 2023-11-24 | 2024-07-26 | 中国水产科学研究院黄海水产研究所 | Antarctic krill ACE (angiotensin converting enzyme) inhibitory peptide LFAGA, RDWPEGR, DWPEGR and application thereof |
| CN118955629A (en) * | 2024-10-18 | 2024-11-15 | 中国海洋大学 | Antarctic krill active peptide and its application |
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2008
- 2008-07-17 JP JP2008185773A patent/JP2010024165A/en active Pending
Cited By (6)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| JP2017043618A (en) * | 2015-08-26 | 2017-03-02 | 三井農林株式会社 | Dipeptidyl peptidase-IV inhibitor |
| KR101823045B1 (en) * | 2016-05-13 | 2018-01-31 | 전남대학교산학협력단 | A composition containing krill protein hydrolysate for treating and preventing hypertension, health functional food containg the same and manufacturing mehod thereof |
| CN114507702A (en) * | 2022-02-03 | 2022-05-17 | 中国海洋大学 | A kind of marine Antarctic krill peptide and its application |
| CN114507702B (en) * | 2022-02-03 | 2023-05-16 | 中国海洋大学 | Marine antarctic krill peptide and application thereof |
| CN118388590A (en) * | 2023-11-24 | 2024-07-26 | 中国水产科学研究院黄海水产研究所 | Antarctic krill ACE (angiotensin converting enzyme) inhibitory peptide LFAGA, RDWPEGR, DWPEGR and application thereof |
| CN118955629A (en) * | 2024-10-18 | 2024-11-15 | 中国海洋大学 | Antarctic krill active peptide and its application |
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