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痘苗病毒病毒粒子蛋白的蛋白水解切割。特异性决定因素的突变分析。

Proteolytic cleavage of vaccinia virus virion proteins. Mutational analysis of the specificity determinants.

作者信息

Lee P, Hruby D E

机构信息

Department of Microbiology, Oregon State University, Corvallis 97331-3804.

出版信息

J Biol Chem. 1994 Mar 18;269(11):8616-22.

PMID:8132587
Abstract

Previous studies have suggested that cleavage of vaccinia virus core protein precursors occurs within the consensus tripeptide motif -A-G decreases X-. As an approach to delineate the sequence and structural features of the precursor polypeptides that are responsible for directing site-specific scission within this element, site-directed mutagenesis procedures were employed in concert with an in vivo trans-processing assay of the P25K: FLAG reporter plasmid. The results obtained suggest that residue occupancy at the P1' site (following the nomenclature of Schechter and Berger (Schechter, I., and Berger, A. (1976) Biochem. Biophys. Res. Commun. 27, 157-162), the positions at the amino- and carboxyl-proximal residues are indicated as P1, P2, etc., and P1', P2', etc., respectively) was extremely permissive, with only a proline substitution blocking cleavage. In contrast, the permissible occupancy of the P1 (serine or alanine) and P2 (cysteine, serine, or asparagine) sites was extremely restricted. Analysis of P1/P2 double mutants supported this conclusion and suggested additional levels of combinatorial stringency. Insertion or deletion of sequences immediately adjacent (amino- or carboxyl-terminal) to the -A-G-X- motif completely abrogated cleavage, suggesting the presence of additional important structural determinants. Mutation of the conserved proline or basic amino acid residues in these regions had no effect on cleavage, whereas it appeared that the presence of a hydrophobic residue in the P4 site was required.

摘要

先前的研究表明,痘苗病毒核心蛋白前体的切割发生在共有三肽基序-A-G-X-内。作为一种描绘负责在该元件内指导位点特异性切割的前体多肽的序列和结构特征的方法,定点诱变程序与P25K:FLAG报告质粒的体内转加工分析协同使用。获得的结果表明,P1'位点(遵循Schechter和Berger的命名法(Schechter, I., and Berger, A. (1976) Biochem. Biophys. Res. Commun. 27, 157 - 162),氨基和羧基近端残基的位置分别表示为P1、P2等和P1'、P2'等)的残基占据非常宽松,只有脯氨酸取代会阻止切割。相比之下,P1(丝氨酸或丙氨酸)和P2(半胱氨酸、丝氨酸或天冬酰胺)位点的允许占据非常受限。对P1/P2双突变体的分析支持了这一结论,并表明存在额外水平的组合严格性。紧邻-A-G-X-基序(氨基或羧基末端)的序列插入或缺失完全消除了切割,表明存在其他重要的结构决定因素。这些区域中保守脯氨酸或碱性氨基酸残基的突变对切割没有影响,而似乎P4位点需要存在一个疏水残基。

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