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来自橄榄绿链霉菌的一种外切几丁质酶的特性、其相应基因、推定的蛋白质结构域以及与其他几丁质酶的关系。

Characteristics of an exochitinase from Streptomyces olivaceoviridis, its corresponding gene, putative protein domains and relationship to other chitinases.

作者信息

Blaak H, Schnellmann J, Walter S, Henrissat B, Schrempf H

机构信息

FB Biologie/Chemie, University of Osnabrück, Germany.

出版信息

Eur J Biochem. 1993 Jun 15;214(3):659-69. doi: 10.1111/j.1432-1033.1993.tb17966.x.

DOI:10.1111/j.1432-1033.1993.tb17966.x
PMID:8319677
Abstract

Streptomyces olivaceoviridis efficiently degrades chitin. Shotgun cloning of partially Sau3A-cleaved DNA using the multicopy vector pIJ702 and Streptomyces lividans 66 as host resulted in the identification of the plasmid pCHI O1 which harbours an insert of 4.6 kb. In the presence of chitin as sole carbon source, transformants of S. lividans 66 carrying pCHI O1 or its derivatives with smaller inserts overproduced an exochitinase which was purified to homogeneity. The chitin-inducible enzyme with an isoelectric point of 4.0 shows optimal activity at pH 7.3 and 55 degrees C, has an apparent molecular mass of 47 kDa and is competitively inhibited by the pseudosugar allosamidin. The enzyme was identified as an exochitinase since it generates exclusively chitobiose from chitotetraose, chitohexaose, and colloidal high-molecular mass chitin. Sequence analysis of a reading frame of 1794 base pairs and comparison of the deduced amino-acid sequence allowed the identification of the putative catalytic domain, one region with significant similarity to the type-III module of fibronectin and one domain of unknown function. Multiple sequence alignment and hydrophobic-cluster analysis of 25 chitinolytic enzymes from bacteria, fungi and plants allowed the identification of their characteristic domains. The exochitinase from S. olivaceoviridis shares highest similarity with the chitinase D from Bacillus circulans.

摘要

橄榄绿链霉菌能高效降解几丁质。使用多拷贝载体pIJ702以及以变铅青链霉菌66作为宿主,对经部分Sau3A酶切的DNA进行鸟枪法克隆,结果鉴定出携带4.6 kb插入片段的质粒pCHI O1。在以几丁质作为唯一碳源的情况下,携带pCHI O1或其带有较小插入片段的衍生物的变铅青链霉菌66转化子过量产生了一种外切几丁质酶,并将其纯化至同质。这种几丁质诱导型酶的等电点为4.0,在pH 7.3和55℃时表现出最佳活性,表观分子量为47 kDa,并且被假糖别洛沙米竞争性抑制。该酶被鉴定为外切几丁质酶,因为它仅从壳四糖、壳六糖和胶体状高分子量几丁质产生壳二糖。对一个1794个碱基对的阅读框进行序列分析,并比较推导的氨基酸序列,从而鉴定出推定的催化结构域、一个与纤连蛋白III型模块具有显著相似性的区域以及一个功能未知的结构域。对来自细菌、真菌和植物的25种几丁质分解酶进行多序列比对和疏水簇分析,从而鉴定出它们的特征结构域。橄榄绿链霉菌的外切几丁质酶与环状芽孢杆菌的几丁质酶D具有最高的相似性。

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