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人星状病毒非结构蛋白的蛋白水解加工

Proteolytic processing of a human astrovirus nonstructural protein.

作者信息

Kiang David, Matsui Suzanne M

机构信息

Division of Gastroenterology, Center for Clinical Sciences Research, Room 3115, Stanford University School of Medicine, 300 Pasteur Drive, Stanford, CA 94305-5187, USA, and VA Palo Alto Health Care System, Palo Alto, CA 94304, USA1.

出版信息

J Gen Virol. 2002 Jan;83(Pt 1):25-34. doi: 10.1099/0022-1317-83-1-25.

DOI:10.1099/0022-1317-83-1-25
PMID:11752697
Abstract

To analyse the activity of the putative 3C-like serine protease encoded in open reading frame (ORF)-1a of human astrovirus serotype 1 (HAstV-1), ORF-1a was transcribed and translated in vitro. Translation products, identified by immunoprecipitation with specific antibodies against recombinant C-terminal ORF-1a fragments, include the full-length 101 kDa (p101) protein and a 38 kDa band (p38). In addition, a 64 kDa protein (p64) was immunoprecipitated by an anti-FLAG antibody when a FLAG epitope was inserted at the N terminus of the ORF-1a product. Mutation of the amino acids predicted to form the catalytic triad of the HAstV-1 3C-like serine protease (Ser-551, Asp-489, His-461) resulted in undetectable levels of p38, supporting the involvement of the HAstV-1 3C-like serine protease and the importance of these amino acids in the processing of p101 into p38 and p64. N-terminal deletions of up to 420 aa of p101 that did not involve the predicted 3C-like serine protease motif did not alter levels of p38 compared to wild-type. C-terminal deletion analysis localized p38 to the C terminus of ORF-1a. Mutation of the P1 residue of the predicted cleavage site, which is conserved among known human and sheep astrovirus sequences, resulted in no detectable p38, supporting cleavage at the Gln-567/Thr-568 dipeptide. These results suggest that p101 is cleaved into an N-terminal p64 fragment and a C-terminal p38 product at Gln-567/Thr-568 in a process that is dependent on the viral 3C-like serine protease.

摘要

为分析人1型星状病毒(HAstV-1)开放阅读框(ORF)-1a中编码的假定3C样丝氨酸蛋白酶的活性,在体外对ORF-1a进行转录和翻译。通过用针对重组C末端ORF-1a片段的特异性抗体进行免疫沉淀鉴定的翻译产物包括全长101 kDa(p101)蛋白和一条38 kDa条带(p38)。此外,当在ORF-1a产物的N末端插入FLAG表位时,一种64 kDa蛋白(p64)被抗FLAG抗体免疫沉淀。预测形成HAstV-1 3C样丝氨酸蛋白酶催化三联体的氨基酸(Ser-551、Asp-489、His-461)发生突变,导致p38水平检测不到,这支持了HAstV-1 3C样丝氨酸蛋白酶的参与以及这些氨基酸在将p101加工成p38和p64过程中的重要性。与野生型相比,p101的N末端缺失多达420个氨基酸且不涉及预测的3C样丝氨酸蛋白酶基序,并未改变p38的水平。C末端缺失分析将p38定位到ORF-1a的C末端。预测的切割位点的P1残基发生突变,该残基在已知的人和羊星状病毒序列中保守,导致检测不到p38,支持在Gln-567/Thr-568二肽处进行切割。这些结果表明,在一个依赖病毒3C样丝氨酸蛋白酶的过程中,p101在Gln-567/Thr-568处被切割成N末端的p64片段和C末端的p38产物。

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