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The vaccinia virus A14.5L gene encodes a hydrophobic 53-amino-acid virion membrane protein that enhances virulence in mice and is conserved among vertebrate poxviruses.痘苗病毒A14.5L基因编码一种由53个氨基酸组成的疏水性病毒粒子膜蛋白,该蛋白可增强小鼠的毒力,并且在脊椎动物痘病毒中具有保守性。
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Complete genomic sequence of the Amsacta moorei entomopoxvirus: analysis and comparison with other poxviruses.摩尔夜蛾昆虫痘病毒的全基因组序列:与其他痘病毒的分析和比较
Virology. 2000 Aug 15;274(1):120-39. doi: 10.1006/viro.2000.0449.
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Genome-wide analysis of vaccinia virus protein-protein interactions.痘苗病毒蛋白质-蛋白质相互作用的全基因组分析。
Proc Natl Acad Sci U S A. 2000 Apr 25;97(9):4879-84. doi: 10.1073/pnas.080078197.
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Alastrim smallpox variola minor virus genome DNA sequences.类天花病毒(天花轻症病毒)基因组DNA序列。
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A model for vaccinia virus pathogenesis and immunity based on intradermal injection of mouse ear pinnae.基于小鼠耳廓皮内注射的痘苗病毒发病机制和免疫模型。
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The complete genome sequence of shope (rabbit) fibroma virus.肖普(兔)纤维瘤病毒的全基因组序列
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The complete DNA sequence of myxoma virus.黏液瘤病毒的完整DNA序列。
Virology. 1999 Nov 25;264(2):298-318. doi: 10.1006/viro.1999.0001.
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Vaccinia virus strains Lister, USSR and Evans express soluble and cell-surface tumour necrosis factor receptors.痘苗病毒株李斯特、苏联株和埃文斯株表达可溶性和细胞表面肿瘤坏死因子受体。
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9
The complete genomic sequence of the modified vaccinia Ankara strain: comparison with other orthopoxviruses.改良安卡拉痘苗病毒株的全基因组序列:与其他正痘病毒的比较。
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10
Blockade of chemokine activity by a soluble chemokine binding protein from vaccinia virus.痘苗病毒来源的可溶性趋化因子结合蛋白对趋化因子活性的阻断作用
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痘苗病毒超氧化物歧化酶样蛋白(A45R)是一种病毒粒子成分,对病毒复制并非必需。

The vaccinia virus superoxide dismutase-like protein (A45R) is a virion component that is nonessential for virus replication.

作者信息

Almazán F, Tscharke D C, Smith G L

机构信息

Sir William Dunn School of Pathology, University of Oxford, Oxford OX1 3RE, United Kingdom.

出版信息

J Virol. 2001 Aug;75(15):7018-29. doi: 10.1128/JVI.75.15.7018-7029.2001.

DOI:10.1128/JVI.75.15.7018-7029.2001
PMID:11435582
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC114430/
Abstract

A characterization of the A45R gene from vaccinia virus (VV) strain Western Reserve is presented. The open reading frame is predicted to encode a 125-amino-acid protein (M(r), of 13,600) with 39% amino acid identity to copper-zinc superoxide dismutase (Cu-Zn SOD). Sequencing of the A45R gene from other orthopoxviruses, here and by others, showed that the protein is highly conserved in all viruses sequenced, including 16 strains of VV, 2 strains of cowpox virus, camelpox virus, and 4 strains of variola virus. In all cases the protein lacks key residues involved in metal ion binding that are important for the catalytic activity. The A45R protein was expressed in Escherichia coli, purified, and tested for SOD activity, but neither enzymatic nor inhibitory SOD activity was detected. Additionally, no virus-encoded SOD activity was detected in infected cells or purified virions. A monoclonal antibody raised against the A45R protein expressed in E. coli identified the A45R gene product as a 13.5-kDa protein that is expressed late during VV infection. Confocal microscopy of VV-infected cells indicated that the A45R protein accumulated predominantly in cytoplasmic viral factories. Electron microscopy and biochemical analyses showed that the A45R protein is incorporated into the virion core. A deletion mutant lacking the majority of the A45R gene and a revertant virus in which the deleted gene was restored were constructed and characterized. The growth properties of the deletion mutant virus were indistinguishable from those of wild-type and revertant viruses in all cell lines tested, including macrophages. Additionally, the virulence and pathogenicity of the three viruses were also comparable in murine and rabbit models of infection. A45R is unusual in being the first VV core protein described that affects neither virus replication nor virulence.

摘要

本文介绍了来自痘苗病毒(VV)西储株的A45R基因的特征。该开放阅读框预计编码一个125个氨基酸的蛋白质(分子量为13,600),与铜锌超氧化物歧化酶(Cu-Zn SOD)具有39%的氨基酸同一性。对来自其他正痘病毒的A45R基因进行测序,包括这里以及其他人的研究,结果表明该蛋白在所有测序的病毒中高度保守,其中包括16株VV、2株牛痘病毒、骆驼痘病毒以及4株天花病毒。在所有情况下,该蛋白都缺乏对催化活性至关重要的金属离子结合关键残基。A45R蛋白在大肠杆菌中表达、纯化并检测其超氧化物歧化酶活性,但未检测到酶活性或抑制性超氧化物歧化酶活性。此外,在感染细胞或纯化的病毒粒子中也未检测到病毒编码的超氧化物歧化酶活性。针对在大肠杆菌中表达的A45R蛋白产生的单克隆抗体,将A45R基因产物鉴定为一种13.5 kDa的蛋白,该蛋白在VV感染后期表达。对VV感染细胞进行共聚焦显微镜检查表明,A45R蛋白主要聚集在细胞质病毒工厂中。电子显微镜和生化分析表明,A45R蛋白被整合到病毒粒子核心中。构建并鉴定了一个缺失大部分A45R基因的缺失突变体和一个恢复了缺失基因的回复病毒。在所有测试的细胞系中,包括巨噬细胞,缺失突变体病毒的生长特性与野生型和回复病毒没有区别。此外,这三种病毒在小鼠和兔感染模型中的毒力和致病性也相当。A45R不同寻常之处在于,它是第一个被描述的不影响病毒复制和毒力的VV核心蛋白。