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风疹病毒非结构蛋白开放阅读框的表达及蛋白水解加工的证明

Expression of the rubella virus nonstructural protein ORF and demonstration of proteolytic processing.

作者信息

Marr L D, Wang C Y, Frey T K

机构信息

Department of Biology, Georgia State University, Atlanta 30302-4010.

出版信息

Virology. 1994 Feb;198(2):586-92. doi: 10.1006/viro.1994.1070.

Abstract

To analyze the proteins produced from the rubella virus (RUB) nonstructural protein open reading frame (NSP-ORF), a DNA containing the RUB NSP-ORF was introduced into the expression vector pTM3 in which the sequences to be expressed are downstream from a T7 RNA polymerase promoter. In cells infected with a vaccinia virus recombinant which expresses T7 RNA polymerase and transfected with this plasmid, three RUB-specific products with electrophoretic mobilities of 200, 150, and 97 kDa were clearly visible. By computer alignment, the presence of a cysteine protease was predicted within the NSP-ORF (A. E. Gorbalenya et al., FEBS Lett. 288, 201-205, 1991). When the Cys proposed as the catalytic residue of this protease (Cys1151) was mutated to a Gly, only the 200-kDa product was produced, demonstrating that the Cys is important in the activity of the protease responsible for the processing of the RUB NSPs and that the 150- and 97-kDa species are processing products. Transfections with deletion mutants revealed that the 150-kDa processing product is derived from the amino-terminal two-thirds of the ORF and that both the protease and the cleavage site on the COOH-terminal side of the 150-kDa product are between amino acids 1005 and 1507 of the ORF.

摘要

为了分析风疹病毒(RUB)非结构蛋白开放阅读框(NSP-ORF)产生的蛋白质,将含有RUB NSP-ORF的DNA导入表达载体pTM3中,其中待表达的序列位于T7 RNA聚合酶启动子的下游。在感染了表达T7 RNA聚合酶的痘苗病毒重组体并转染该质粒的细胞中,明显可见三种电泳迁移率分别为200、150和97 kDa的RUB特异性产物。通过计算机比对,预测在NSP-ORF内存在一种半胱氨酸蛋白酶(A.E.戈尔巴连亚等人,《欧洲生物化学学会联合会快报》288,201 - 205,1991)。当被提议作为该蛋白酶催化残基的半胱氨酸(Cys1151)突变为甘氨酸时,仅产生了200 kDa的产物,这表明半胱氨酸在负责RUB NSP加工的蛋白酶活性中很重要,并且150 kDa和97 kDa的产物是加工产物。用缺失突变体进行转染表明,150 kDa的加工产物源自ORF氨基末端的三分之二,并且蛋白酶和150 kDa产物COOH末端一侧的切割位点都在ORF的第1005至1507个氨基酸之间。

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