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人冠状病毒229E复制酶多聚蛋白由病毒编码的3C样蛋白酶进行加工:鉴定pp1a和pp1ab共有的蛋白水解产物和切割位点。

Processing of the human coronavirus 229E replicase polyproteins by the virus-encoded 3C-like proteinase: identification of proteolytic products and cleavage sites common to pp1a and pp1ab.

作者信息

Ziebuhr J, Siddell S G

机构信息

Institute of Virology, University of Würzburg, 97078 Würzburg, Germany.

出版信息

J Virol. 1999 Jan;73(1):177-85. doi: 10.1128/JVI.73.1.177-185.1999.

Abstract

Replicase gene expression by the human coronavirus 229E involves the synthesis of two large polyproteins, pp1a and pp1ab. Experimental evidence suggests that these precursor molecules are subject to extensive proteolytic processing. In this study, we show that a chymotrypsin-like enzyme, the virus-encoded 3C-like proteinase (3CLpro), cleaves within a common region of pp1a and pp1ab (amino acids 3490 to 4068) at four sites. trans-cleavage assays revealed that polypeptides of 5, 23, 12, and 16 kDa are processed from pp1a/pp1ab by proteolysis of the peptide bonds Q3546/S3547, Q3629/S3630, Q3824/N3825, and Q3933/A3934. Relative rate constants for the 3CLpro-mediated cleavages Q2965/A2966, Q3267/S3268, Q3824/N3825, and Q3933/A3934 were derived by competition experiments using synthetic peptides and recombinant 3CLpro. The results indicate that coronavirus cleavage sites differ significantly with regard to their susceptibilities to proteolysis by 3CLpro. Finally, immunoprecipitation with specific rabbit antisera was used to detect the pp1a/pp1ab processing end products in virus-infected cells, and immunofluorescence data that suggest an association of these polypeptides with intracellular membranes were obtained.

摘要

人冠状病毒229E的复制酶基因表达涉及两种大的多聚蛋白pp1a和pp1ab的合成。实验证据表明,这些前体分子会经历广泛的蛋白水解加工。在本研究中,我们发现一种类胰凝乳蛋白酶样酶,即病毒编码的3C样蛋白酶(3CLpro),在pp1a和pp1ab的一个共同区域(氨基酸3490至4068)内的四个位点进行切割。反式切割试验表明,通过切割肽键Q3546/S3547、Q3629/S3630、Q3824/N3825和Q3933/A3934,可从pp1a/pp1ab加工出5 kDa、23 kDa、12 kDa和16 kDa的多肽。使用合成肽和重组3CLpro通过竞争实验得出3CLpro介导的切割Q2965/A2966、Q3267/S3268、Q3824/N3825和Q3933/A3934的相对速率常数。结果表明,冠状病毒切割位点对3CLpro蛋白水解的敏感性存在显著差异。最后,使用特异性兔抗血清进行免疫沉淀,以检测病毒感染细胞中pp1a/pp1ab加工的终产物,并获得了表明这些多肽与细胞内膜相关的免疫荧光数据。

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