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黄热病病毒NS1蛋白的遗传分析:鉴定出一个阻断RNA积累的温度敏感突变。

Genetic analysis of the yellow fever virus NS1 protein: identification of a temperature-sensitive mutation which blocks RNA accumulation.

作者信息

Muylaert I R, Galler R, Rice C M

机构信息

Department of Molecular Microbiology, Washington University School of Medicine, St. Louis, Missouri 63110-1093, USA.

出版信息

J Virol. 1997 Jan;71(1):291-8. doi: 10.1128/JVI.71.1.291-298.1997.

DOI:10.1128/JVI.71.1.291-298.1997
PMID:8985349
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC191050/
Abstract

The flavivirus NS1 protein is a highly conserved nonstructural glycoprotein that is capable of eliciting protective immunity. NS1 homodimers are secreted from virus-infected mammalian cells, but the protein is also present at the plasma membrane and in the lumen of intracellular vesicles. Based on these properties, it has been speculated that NS1 may function in virus maturation or release. To gain further insight into NS1 function, we used clustered charged-amino-acid-to-alanine mutagenesis to create 28 clustered substitutions in the NS1 protein of yellow fever virus. To screen for conditional mutations, full-length RNAs containing each mutation were assayed for plaque formation at 32 and 39 degrees C after RNA transfection. We found that 9 mutations were lethal, 18 allowed plaque formation at both temperatures, and 1, ts25, was strongly heat sensitive and was unable to form plaques at 39 degrees C. Lethal mutations clustered in the amino-terminal half of NS1, whereas those leading to impaired replication relative to the parent were distributed throughout the protein. High-multiplicity infections at 39 degrees C demonstrated that ts25 was defective for RNA accumulation, leading to depressed viral protein synthesis and delayed virus production. Although ts25 secreted less NS1 than did the parent, temperature shift experiments failed to demonstrate any temperature-dependent differences in polyprotein processing, NS1 stability and secretion, or release of infectious virus. The ts lesion of ts25 was shown to be due to a single alanine substitution for Arg-299, a residue which is conserved among flaviviruses. These results argue that NS1 plays an essential but as yet undefined role in flavivirus RNA amplification.

摘要

黄病毒NS1蛋白是一种高度保守的非结构糖蛋白,能够引发保护性免疫。NS1同型二聚体从病毒感染的哺乳动物细胞中分泌出来,但该蛋白也存在于质膜和细胞内囊泡腔中。基于这些特性,推测NS1可能在病毒成熟或释放中发挥作用。为了进一步深入了解NS1的功能,我们使用簇状带电氨基酸到丙氨酸诱变技术,在黄热病毒的NS1蛋白中创建了28个簇状替换。为了筛选条件性突变,在RNA转染后,对含有每个突变的全长RNA在32℃和39℃下进行噬斑形成检测。我们发现9个突变是致死性的,18个在两个温度下都允许噬斑形成,还有1个,即ts25,对热高度敏感,在39℃下无法形成噬斑。致死性突变聚集在NS1的氨基末端一半,而相对于亲本导致复制受损的突变则分布在整个蛋白中。在39℃下进行的高倍感染表明,ts25在RNA积累方面存在缺陷,导致病毒蛋白合成减少和病毒产生延迟。尽管ts25分泌的NS1比亲本少,但温度转换实验未能证明在多聚蛋白加工、NS1稳定性和分泌或感染性病毒释放方面存在任何温度依赖性差异。ts25的温度敏感损伤被证明是由于单个丙氨酸取代了精氨酸-299,该残基在黄病毒中是保守的。这些结果表明,NS1在黄病毒RNA扩增中起着至关重要但尚未明确的作用。

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本文引用的文献

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Immunolocalization of the dengue virus nonstructural glycoprotein NS1 suggests a role in viral RNA replication.登革病毒非结构糖蛋白NS1的免疫定位表明其在病毒RNA复制中起作用。
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Cleavage at a novel site in the NS4A region by the yellow fever virus NS2B-3 proteinase is a prerequisite for processing at the downstream 4A/4B signalase site.黄热病毒NS2B-3蛋白酶在NS4A区域一个新位点的切割是下游4A/4B信号酶位点进行加工的先决条件。
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Mutagenesis of conserved residues at the yellow fever virus 3/4A and 4B/5 dibasic cleavage sites: effects on cleavage efficiency and polyprotein processing.黄热病毒3/4A和4B/5双碱性切割位点保守残基的诱变:对切割效率和多聚蛋白加工的影响。
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The effects of site-directed mutagenesis on the dimerization and secretion of the NS1 protein specified by dengue virus.定点诱变对登革病毒所编码的NS1蛋白二聚化及分泌的影响。
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Computer-assisted identification of a putative methyltransferase domain in NS5 protein of flaviviruses and lambda 2 protein of reovirus.计算机辅助鉴定黄病毒NS5蛋白和呼肠孤病毒λ2蛋白中的假定甲基转移酶结构域。
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