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寨卡病毒 NS2A 蛋白的遗传和生化特性。

Genetic and biochemical characterizations of Zika virus NS2A protein.

机构信息

a State Key Laboratory of Virology , Wuhan Institute of Virology, Chinese Academy of Sciences , Wuhan , People's Republic of China.

b University of Chinese Academy of Sciences , Beijing , People's Republic of China.

出版信息

Emerg Microbes Infect. 2019;8(1):585-602. doi: 10.1080/22221751.2019.1598291.

Abstract

Zika virus (ZIKV) can cause devastating congenital Zika syndromes in pregnant women and Guillain-Barre syndrome in adults. Understanding the molecular mechanism of ZIKV replication is essential for antiviral and vaccine development. Here we report the structural and functional characterization of ZIKV NS2A protein. Biochemical structural probing suggests that ZIKV NS2A has a single segment that traverses the ER membrane and six segments that peripherally associate with the ER membrane. Functional analysis has defined distinct NS2A residues essential for viral RNA synthesis or virion assembly. Only the virion assembly-defective mutants, but not the RNA synthesis-defective mutants, could be rescued through trans complementation with a wide-type NS2A protein. These results suggest that the NS2A molecules in virion assembly complex could be recruited in trans, whereas the NS2A molecules in viral replication complex must be recruited in cis. Together with previous results, we propose a flavivirus assembly model where NS2A plays a central role in modulating viral structural and nonstructural proteins as well as genomic RNA during virion assembly.

摘要

寨卡病毒(ZIKV)可导致孕妇发生严重的先天性寨卡综合征,并可导致成年人发生格林-巴利综合征。了解寨卡病毒复制的分子机制对于抗病毒和疫苗的研发至关重要。在此,我们报告了寨卡病毒 NS2A 蛋白的结构和功能特征。生化结构探测表明,寨卡病毒 NS2A 具有一个贯穿内质网膜的片段和六个与内质网膜外周结合的片段。功能分析定义了 NS2A 中对病毒 RNA 合成或病毒粒子组装至关重要的不同残基。只有病毒粒子组装缺陷型突变体,而不是 RNA 合成缺陷型突变体,可以通过与野生型 NS2A 蛋白的转互补得到拯救。这些结果表明,在病毒粒子组装复合物中的 NS2A 分子可以在转位中被募集,而在病毒复制复合物中的 NS2A 分子必须在顺式中被募集。结合以前的结果,我们提出了一个黄病毒组装模型,其中 NS2A 在病毒粒子组装过程中调节病毒结构蛋白和非结构蛋白以及基因组 RNA 方面发挥核心作用。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2b81/6455252/7a998a82e9c7/TEMI_A_1598291_F0001_OC.jpg

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