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直观呈现病毒 RNA 包装信号的作用机制。

Visualizing Viral RNA Packaging Signals in Action.

机构信息

Astbury Centre for Structural Molecular Biology, University of Leeds, Leeds LS2 9JT, United Kingdom.

Astbury Centre for Structural Molecular Biology, University of Leeds, Leeds LS2 9JT, United Kingdom.

出版信息

J Mol Biol. 2024 Nov 15;436(22):168765. doi: 10.1016/j.jmb.2024.168765. Epub 2024 Aug 29.

DOI:10.1016/j.jmb.2024.168765
PMID:39214281
Abstract

Here we confirm, using genome-scale RNA fragments in assembly competition assays, that multiple sub-sites (Packaging Signals, PSs) across the 5' two-thirds of the gRNA of Satellite Tobacco Necrosis Virus-1 make sequence-specific contacts to the viral CPs helping to nucleate formation of its T = 1 virus-like particle (VLP). These contacts explain why natural virions only package their positive-sense genomes. Asymmetric cryo-EM reconstructions of these VLPs suggest that interactions occur between amino acid residues in the N-terminal ends of the CP subunits and the gRNA PS loop sequences. The base-paired stems of PSs also act non-sequence-specifically by electrostatically promoting the assembly of CP trimers. Importantly, alterations in PS-CP affinity result in an asymmetric distribution of bound PSs inside VLPs, with fuller occupation of the higher affinity 5' PS RNAs around one vertex, decreasing to an RNA-free opposite vertex within the VLP shell. This distribution suggests that gRNA folding regulates cytoplasmic genome extrusion so that the weakly bound 3' end of the gRNA, containing the RNA polymerase binding site, extrudes first. This probably occurs after cation-loss induced swelling of the CP-shell, weakening contacts between CP subunits. These data reveal for the first time in any virus how differential PS folding propensity and CP affinities support the multiple roles genomes play in virion assembly and infection. The high degree of conservation between the CP fold of STNV-1 and those of the CPs of many other viruses suggests that these aspects of genome function will be widely shared.

摘要

在这里,我们通过组装竞争实验中的基因组规模 RNA 片段证实,Satellite Tobacco Necrosis Virus-1(STNV-1)gRNA 的 5' 三分之二区域的多个亚位点(包装信号,PS)与病毒 CP 进行序列特异性接触,有助于形成其 T=1 病毒样颗粒(VLP)。这些接触解释了为什么天然病毒粒子仅包装其正链基因组。这些 VLPs 的非对称 cryo-EM 重建表明,CP 亚基的 N 端氨基酸残基与 gRNA PS 环序列之间发生相互作用。PS 的碱基配对茎也通过静电作用非特异性地促进 CP 三聚体的组装。重要的是,PS-CP 亲和力的改变导致结合 PS 在内的 VLPs 中呈不对称分布,具有更高亲和力的 5' PS RNA 在一个顶点周围更充分地占据,在 VLP 壳内的相反顶点处减少到无 RNA。这种分布表明,gRNA 折叠调节细胞质基因组外推,使得 gRNA 的弱结合 3' 端,包含 RNA 聚合酶结合位点,首先外推。这可能发生在 CP-壳阳离子损失诱导的肿胀之后,削弱了 CP 亚基之间的接触。这些数据首次揭示了在任何病毒中,差异 PS 折叠倾向和 CP 亲和力如何支持基因组在病毒粒子组装和感染中发挥多种作用。STNV-1 的 CP 折叠与许多其他病毒的 CP 之间高度保守,表明这些基因组功能的各个方面将得到广泛共享。

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