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嗜热嗜酸古菌嗜热栖热菌β-糖苷酶中催化作用所必需的两个谷氨酸残基的鉴定。

Identification of two glutamic acid residues essential for catalysis in the beta-glycosidase from the thermoacidophilic archaeon Sulfolobus solfataricus.

作者信息

Moracci M, Capalbo L, Ciaramella M, Rossi M

机构信息

Institute of Protein Biochemistry and Enzymology-CNR, Naples, Italy.

出版信息

Protein Eng. 1996 Dec;9(12):1191-5. doi: 10.1093/protein/9.12.1191.

DOI:10.1093/protein/9.12.1191
PMID:9010932
Abstract

The Sulfolobus solfataricus, strain MT4, beta-glycosidase (Ss beta-gly) is a thermophilic member of glycohydrolase family 1. To identify active-site residues, glutamic acids 206 and 387 have been changed to isosteric glutamine by site-directed mutagenesis. Mutant proteins have been purified to homogeneity using the Schistosoma japonicum glutathione S-transferase (GST) fusion system. The proteolytic cleavage of the chimeric protein with thrombin was only obtainable after the introduction of a molecular spacer between the GST and the Ss beta-gly domains. The Glu387-->Gln mutant showed no detectable activity, as expected for the residue acting as the nucleophile of the reaction. The Glu206-->Gln mutant showed 10- and 60-fold reduced activities on aryl-galacto and aryl-glucosides, respectively, when compared with the wild type. Moreover, a significant Km decrease with p/o-nitrophenyl-beta-D-glucoside was observed. The residual activity of the Glu206-->Gln mutant lost the typical pH dependence shown by the wild type. These data suggest that Glu206 acts as the general acid/base catalyst in the hydrolysis reaction.

摘要

嗜热栖热菌MT4菌株的β-糖苷酶(Ssβ-gly)是糖水解酶家族1的嗜热成员。为了鉴定活性位点残基,通过定点诱变将谷氨酸206和387替换为等电子的谷氨酰胺。使用日本血吸虫谷胱甘肽S-转移酶(GST)融合系统将突变蛋白纯化至同质。只有在GST和Ssβ-gly结构域之间引入分子间隔后,才能用凝血酶对嵌合蛋白进行蛋白水解切割。正如预期的作为反应亲核试剂的残基那样,Glu387→Gln突变体没有可检测到的活性。与野生型相比,Glu206→Gln突变体对芳基半乳糖苷和芳基葡萄糖苷的活性分别降低了10倍和60倍。此外,观察到对p/o-硝基苯基-β-D-葡萄糖苷的Km显著降低。Glu206→Gln突变体的残余活性失去了野生型所具有的典型pH依赖性。这些数据表明,Glu206在水解反应中作为通用酸碱催化剂起作用。

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