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Structure of papain refined at 1.65 A resolution.木瓜蛋白酶结构在1.65埃分辨率下的精修。
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Sequence analysis of three Sindbis virus mutants temperature-sensitive in the capsid protein autoprotease.三种在衣壳蛋白自蛋白酶中对温度敏感的辛德毕斯病毒突变体的序列分析。
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辛德毕斯病毒nsP2蛋白酶活性位点残基的鉴定。

Identification of the active site residues in the nsP2 proteinase of Sindbis virus.

作者信息

Strauss E G, De Groot R J, Levinson R, Strauss J H

机构信息

Division of Biology, California Institute of Technology, Pasadena 91125.

出版信息

Virology. 1992 Dec;191(2):932-40. doi: 10.1016/0042-6822(92)90268-t.

DOI:10.1016/0042-6822(92)90268-t
PMID:1448929
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC7131396/
Abstract

The nonstructural polyproteins of Sindbis virus are processed by a virus-encoded proteinase which is located in the C-terminal domain of nsP2. Here we have performed a mutagenic analysis to identify the active site residues of this proteinase. Substitution of other amino acids for either Cys-481 or His-558 completely abolished proteolytic processing of Sindbis virus polyproteins in vitro. Substitutions within this domain for a second cysteine conserved among alphaviruses, for four other conserved histidines, or for a conserved serine did not affect the activity of the enzyme. These results suggest that nsP2 is a papain-like proteinase whose catalytic dyad is composed of Cys-481 and His-558. Since an asparagine residue has been implicated in the active site of papain, we changed the four conserved asparagine residues in the C-terminal half of nsP2 and found that all could be substituted without total loss of activity. Among papain-like proteinases, the residue following the catalytic histidine is alanine or glycine in the plant and animal enzymes, and the presence of Trp-559 in alphaviruses is unusual. A mutant enzyme containing Ala-559 was completely inactive, implying that Trp-559 is essential for a functional proteinase. All of these mutations were introduced into a full-length clone of Sindbis virus from which infectious RNA could be transcribed in vitro, and the effects of these changes on viability were tested. In all cases it was found that mutations which abolished proteolytic activity were lethal, whether or not these mutations were in the catalytic residues, indicating that proteolysis of the nonstructural polyprotein is essential for Sindbis replication.

摘要

辛德毕斯病毒的非结构多聚蛋白由一种病毒编码的蛋白酶进行加工处理,该蛋白酶位于nsP2的C末端结构域。在此,我们进行了诱变分析以确定这种蛋白酶的活性位点残基。用其他氨基酸取代Cys-481或His-558会完全消除辛德毕斯病毒多聚蛋白在体外的蛋白水解加工。在该结构域内,用其他氨基酸取代在甲病毒中保守的第二个半胱氨酸、另外四个保守的组氨酸或一个保守的丝氨酸,均不影响该酶的活性。这些结果表明,nsP2是一种木瓜蛋白酶样蛋白酶,其催化二元体由Cys-481和His-558组成。由于天冬酰胺残基与木瓜蛋白酶的活性位点有关,我们改变了nsP2 C末端一半中四个保守的天冬酰胺残基,发现所有这些残基都可以被取代而不会完全丧失活性。在木瓜蛋白酶样蛋白酶中,催化组氨酸之后的残基在植物和动物酶中是丙氨酸或甘氨酸,而甲病毒中Trp-559的存在是不寻常的。含有Ala-559的突变酶完全无活性,这意味着Trp-559对于功能性蛋白酶至关重要。所有这些突变都被引入到辛德毕斯病毒的全长克隆中,该克隆可在体外转录出感染性RNA,并测试了这些变化对病毒生存能力的影响。在所有情况下都发现,消除蛋白水解活性的突变是致死性的,无论这些突变是否位于催化残基中,这表明非结构多聚蛋白的蛋白水解对于辛德毕斯病毒的复制至关重要。