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从金针菇菌丝体培养上清液中纯化和鉴定一种纤溶蛋白酶

Purification and characterization of a fibrinolytic protease from a culture supernatant of Flammulina velutipes mycelia.

作者信息

Park Se-Eun, Li Mei-Hong, Kim Jae-Sung, Sapkota Kumar, Kim Ji-Eun, Choi Bong-Suk, Yoon Yeon-Hee, Lee Jin-Cheol, Lee Hyun-Hwa, Kim Chun-Sung, Kim Sung-Jun

机构信息

Department of Biotechnology and BK21 Research Team for Protein Activity Control Chosun University, Gwangju 501-579, Republic of Korea.

出版信息

Biosci Biotechnol Biochem. 2007 Sep;71(9):2214-22. doi: 10.1271/bbb.70193. Epub 2007 Sep 7.

DOI:10.1271/bbb.70193
PMID:17827681
Abstract

In this study we purified a fibrinolytic enzyme from the culture supernatant of Flammulina velutipes mycelia by ion exchange and gel filtration chromatographies, it was designated as F. velutipes protease (FVP-I). This purification protocol resulted in 18.52-fold purification of the enzyme at a final yield of 0.69%. The molecular mass of the purified enzyme was estimated to be 37 kDa by SDS-PAGE, fibrin-zymography and size exclusion by FPLC. This protease effectively hydrolyzed fibrin, preferentially digesting alpha-chain over beta-and gamma-gamma chain. Optimal protease activity was found to occur at a pH of 6.0 and a temperature of 20 to 30 degrees C. The protease activity was inhibited by Cu2+, Fe2+ and Fe3+ ions, but was found to be enhanced by Mn2+ and Mg2+ ions. Furthermore, FVP-I activity was potently inhibited by EDTA and EGTA, and it was found to exhibit a higher specificity for chromogenic substrate S-2586 for chymotrypsin, indicating that the enzyme is a chymotrypsin-like metalloprotease. The first 20 amino acid residues of the N-terminal sequence of FVP-I were LTYRVIPITKQAVTEGTELL. They had a high degree of homology with hypothetical protein CC1G_11771, GeneBank Accession no. EAU86463.

摘要

在本研究中,我们通过离子交换和凝胶过滤色谱法从金针菇菌丝体的培养上清液中纯化出一种纤溶酶,将其命名为金针菇蛋白酶(FVP-I)。该纯化方案使该酶的纯化倍数达到18.52倍,最终产率为0.69%。通过SDS-PAGE、纤维蛋白酶谱法和FPLC尺寸排阻法估计纯化酶的分子量为37 kDa。这种蛋白酶能有效水解纤维蛋白,优先消化α链而非β链和γ链。发现蛋白酶的最佳活性出现在pH值为6.0、温度为20至30摄氏度时。蛋白酶活性受到Cu2+、Fe2+和Fe3+离子的抑制,但发现Mn2+和Mg2+离子可增强其活性。此外,FVP-I的活性受到EDTA和EGTA的强烈抑制,并且发现它对胰凝乳蛋白酶的生色底物S-2586具有更高的特异性,表明该酶是一种类胰凝乳蛋白酶金属蛋白酶。FVP-I N端序列的前20个氨基酸残基为LTYRVIPITKQAVTEGTELL。它们与假定蛋白CC1G_11771(基因库登录号EAU86463)具有高度同源性。

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