Western University of Health Sciences, Pomona, California, United States of America.
PLoS Pathog. 2024 Jan 8;20(1):e1011925. doi: 10.1371/journal.ppat.1011925. eCollection 2024 Jan.
Hantaviruses have evolved a unique translation strategy to boost the translation of viral mRNA in infected cells. Hantavirus nucleocapsid protein (NP) binds to the viral mRNA 5' UTR and the 40S ribosomal subunit via the ribosomal protein S19. NP associated ribosomes are selectively loaded on viral transcripts to boost their translation. Here we demonstrate that NP expression upregulated the steady-state levels of a subset of host cell factors primarily involved in protein processing in the endoplasmic reticulum. Detailed investigation of Valosin-containing protein (VCP/p97), one of the upregulated host factors, in both transfected and virus infected cells revealed that NP with the assistance of VCP mRNA 5' UTR facilitates the translation of downstream VCP ORF. The VCP mRNA contains a 5' UTR of 987 nucleotides harboring six unusual start codons upstream of the correct start codon for VCP which is located at 988th position from the 5' cap. In vitro translation of a GFP reporter transcript harboring the VCP mRNA 5' UTR generated both GFP and a short polypeptide of ~14 KDa by translation initiation from start codon located in the 5' UTR at 542nd position from the 5' cap. The translation initiation from 542nd AUG in the UTR sequence was confirmed in cells using a dual reporter construct expressing mCherry and GFP. The synthesis of 14KDa polypeptide dramatically inhibited the translation of the ORF from the downstream correct start codon at 988th position from the 5' cap. We report that purified NP binds to the VCP mRNA 5' UTR with high affinity and NP binding site is located close to the 542ndAUG. NP binding shuts down the translation of 14KDa polypeptide which then facilitates the translation initiation at the correct AUG codon. Knockdown of VCP generated lower levels of poorly infectious hantavirus particle in the cellular cytoplasm whose egress was dramatically inhibited in human umbilical vein endothelial cells. We demonstrated that VCP binds to the hantavirus glycoprotein Gn before its incorporation into assembled virions and facilitates viral spread to neighboring cells during infection. Our results suggest that ribosome engagement at the 542nd AUG codon in the 5' UTR likely regulates the endogenous steady state levels of VCP in cells. Hantaviruses interrupt this regulatory mechanism to enhance the steady state levels of VCP in virus infected cells. This augmentation facilitates virus replication, supports the transmission of the virus to adjacent cells, and promotes the release of infectious virus particles from the host cell.
汉坦病毒进化出了一种独特的翻译策略,以提高感染细胞中病毒 mRNA 的翻译效率。汉坦病毒核衣壳蛋白(NP)通过核糖体蛋白 S19 与病毒 mRNA 的 5'UTR 和 40S 核糖体亚基结合。NP 相关的核糖体被选择性地上调到病毒转录本上,以提高它们的翻译效率。在这里,我们证明 NP 表达上调了一组主要涉及内质网中蛋白质加工的宿主细胞因子的稳态水平。在转染和病毒感染的细胞中,对上调的宿主因子之一——含缬氨酸蛋白(VCP/p97)进行详细研究表明,NP 在 VCP mRNA 5'UTR 的协助下,促进下游 VCP ORF 的翻译。VCP mRNA 包含一个 987 个核苷酸的 5'UTR,在前正确起始密码子上游有六个不寻常的起始密码子,该起始密码子位于从 5'帽算起的第 988 位。携带 VCP mRNA 5'UTR 的 GFP 报告转录本的体外翻译从位于 5'帽起第 542 位的 5'UTR 中的起始密码子开始,生成 GFP 和大约 14 kDa 的短多肽。使用表达 mCherry 和 GFP 的双报告构建体在细胞中证实了从 UTR 序列中第 542 位 AUG 的翻译起始。NP 结合以高亲和力结合到 VCP mRNA 5'UTR,NP 结合位点靠近 542 位 AUG。NP 结合阻止了 14 kDa 多肽的翻译,从而促进了正确 AUG 密码子处的翻译起始。VCP 的敲低导致细胞质中传染性差的汉坦病毒颗粒水平降低,其在人脐静脉内皮细胞中的出芽明显受到抑制。我们证明 VCP 在其掺入组装的病毒粒子之前与汉坦病毒糖蛋白 Gn 结合,并在感染过程中促进病毒向邻近细胞的传播。我们的结果表明,核糖体在 5'UTR 中第 542 位 AUG 密码子的结合可能调节细胞中 VCP 的内源性稳态水平。汉坦病毒中断了这种调节机制,以提高病毒感染细胞中 VCP 的稳态水平。这种增加促进了病毒复制,支持病毒向相邻细胞的传播,并促进了感染性病毒颗粒从宿主细胞中的释放。
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