Key Laboratory of Animal Epidemiology of the Ministry of Agriculture and Rural Affairs, College of Veterinary Medicine, China Agricultural Universitygrid.22935.3f, Beijing, People's Republic of China.
J Virol. 2021 Aug 10;95(17):e0051821. doi: 10.1128/JVI.00518-21.
A critical step in replication of positive-stranded RNA viruses is the assembly of replication and transcription complexes (RTC). We have recently mapped the nonstructural protein (nsp) interaction network of porcine reproductive and respiratory syndrome virus (PRRSV) and provided evidence by truncation mutagenesis that the recruitment of viral core replicase enzymes (nsp9 and nsp10) to membrane proteins (nsp2, nsp3, nsp5, and nsp12) is subject to regulation. Here, we went further to discover an intramolecular switch within the helicase nsp10 that controls its interaction with the membrane-associated protein nsp12. Deletion of nsp10 linker region amino acids 124 to 133, connecting domain 1B to 1A, led to complete relocalization and colocalization in the cells coexpressing nsp12. Moreover, single-amino-acid substitutions (e.g., nsp10 E131A and I132A) were sufficient to enable the nsp10-nsp12 interaction. Further proof came from membrane floatation assays that revealed a clear movement of nsp10 mutants, but not wild-type nsp10, toward the top of sucrose gradients in the presence of nsp12. Interestingly, the same mutations were not able to activate the nsp10-nsp2/3 interaction, suggesting a differential requirement for conformation. Reverse genetics analysis showed that PRRSV mutants carrying the single substitutions were not viable and were defective in subgenomic RNA (sgRNA) accumulation. Together, our results provide strong evidence for a regulated interaction between nsp10 and nsp12 and suggest an essential role for an orchestrated RTC assembly in sgRNA synthesis. Assembly of replication and transcription complexes (RTC) is a limiting step for viral RNA synthesis. The PRRSV RTC macromolecular complexes are comprised of mainly viral nonstructural replicase proteins (nsps), but how they come together remains elusive. We previously showed that viral helicase nsp10 interacts nsp12 in a regulated manner by truncation mutagenesis. Here, we revealed that the interaction is controlled by single residues within the domain linker region of nsp10. Moreover, the activation mutations lead to defects in viral sgRNA synthesis. Our results provide important insight into the mechanisms of PRRSV RTC assembly and regulation of viral sgRNA synthesis.
正链 RNA 病毒复制的一个关键步骤是复制和转录复合物(RTC)的组装。我们最近绘制了猪繁殖与呼吸综合征病毒(PRRSV)的非结构蛋白(nsp)相互作用网络,并通过截短突变提供了证据,证明病毒核心复制酶(nsp9 和 nsp10)被招募到膜蛋白(nsp2、nsp3、nsp5 和 nsp12)受到调节。在这里,我们更进一步发现 nsp10 解旋酶内的分子内开关控制其与膜相关蛋白 nsp12 的相互作用。删除连接域 1B 和 1A 的 nsp10 连接区氨基酸 124 至 133,导致共表达 nsp12 的细胞中完全重新定位和共定位。此外,单个氨基酸取代(例如,nsp10 E131A 和 I132A)足以使 nsp10-nsp12 相互作用。进一步的证据来自膜漂浮实验,该实验表明在存在 nsp12 的情况下,nsp10 突变体而不是野生型 nsp10 明显向蔗糖梯度的顶部移动。有趣的是,相同的突变不能激活 nsp10-nsp2/3 相互作用,表明构象存在差异要求。反向遗传学分析表明,携带单取代的 PRRSV 突变体不能存活并且在亚基因组 RNA(sgRNA)积累中存在缺陷。总之,我们的结果为 nsp10 和 nsp12 之间受调控的相互作用提供了有力证据,并表明协调的 RTC 组装在 sgRNA 合成中起重要作用。复制和转录复合物(RTC)的组装是病毒 RNA 合成的限速步骤。PRRSV RTC 大分子复合物主要由病毒非结构复制酶蛋白(nsps)组成,但它们如何聚集在一起仍不清楚。我们之前通过截断突变显示病毒解旋酶 nsp10 以受调控的方式与 nsp12 相互作用。在这里,我们揭示了这种相互作用受 nsp10 结构域连接区的单个残基控制。此外,激活突变导致病毒 sgRNA 合成缺陷。我们的结果为 PRRSV RTC 组装和病毒 sgRNA 合成的调控机制提供了重要的见解。
