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一株新分离中度嗜盐菌LY6 产生和性质的新型胞外金属蛋白酶。

Production and characterization of a novel extracellular metalloproteinase by a newly isolated moderate halophile, Halobacillus sp. LY6.

机构信息

Life Science College, Yuncheng University, Yuncheng, China.

出版信息

Folia Microbiol (Praha). 2011 Jul;56(4):329-34. doi: 10.1007/s12223-011-0046-9. Epub 2011 May 31.

DOI:10.1007/s12223-011-0046-9
PMID:21625873
Abstract

A moderately halophilic bacterium LY6 with high proteolytic activity was isolated. Biochemical and physiological characterization, along with 16S rDNA sequence analysis placed the isolate in the genus Halobacillus. The salinity of the culture medium strongly influenced the proteinase production of LY6. Maximum enzyme production was observed in the medium containing 5% Na(2)SO(4) or 10% NaCl. Proteinase production was synchronized with bacterial growth and reached a maximum level during the mid-stationary phase. Enzyme purification was carried out by a simple approach including a combination of ammonium sulfate precipitation and Sephacryl S-100 gel filtration chromatography. SDS-PAGE and gelatin zymography analysis revealed it was a monomer with high molecular weight of 69 kDa. Optimal proteinase activity was obtained at pH 10.0, 40°C, and 10% NaCl. It was high active over broad temperature (30-80°C), pH (6.0-12.0), and NaCl concentration (0-25%) ranges, indicating its thermostable, alkali-stable, and halotolerant nature. Moreover, the enzyme activity was markedly enhanced by Ca(2+) and Cu(2+), but strongly inhibited by EDTA, PAO, and DEPC, indicating that it probably was a metalloproteinase with cysteine and histidine residues located in its active site.

摘要

一种具有高蛋白水解活性的中度嗜盐细菌 LY6 被分离出来。通过生化和生理特性分析以及 16S rDNA 序列分析,该分离株被归入 Halobacillus 属。培养基的盐度强烈影响 LY6 的蛋白酶产量。在含有 5%Na2SO4 或 10%NaCl 的培养基中观察到最大酶产量。蛋白酶的产生与细菌生长同步,在中期达到最高水平。通过简单的方法进行酶纯化,包括硫酸铵沉淀和 Sephacryl S-100 凝胶过滤层析的组合。SDS-PAGE 和明胶酶谱分析表明,它是一种具有高分子量(69 kDa)的单体。在 pH 值为 10.0、40°C 和 10%NaCl 的条件下,蛋白酶活性最佳。它在较宽的温度(30-80°C)、pH 值(6.0-12.0)和 NaCl 浓度(0-25%)范围内具有高活性,表明其具有热稳定性、耐碱性和耐盐性。此外,该酶的活性明显受 Ca2+和 Cu2+的增强,但受 EDTA、PAO 和 DEPC 的强烈抑制,表明它可能是一种含有半胱氨酸和组氨酸残基的金属蛋白酶,位于其活性部位。

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