Institute of Molecular Biology, Academia Sinica, Taipei, Taiwan, Republic of China.
Genome and Systems Biology Degree Program, Academia Sinica and National Taiwan University, Taipei, Taiwan, Republic of China.
J Virol. 2020 May 4;94(10). doi: 10.1128/JVI.00093-20.
For cell entry, vaccinia virus requires fusion with the host membrane via a viral fusion complex of 11 proteins, but the mechanism remains unclear. It was shown previously that the viral proteins A56 and K2 are expressed on infected cells to prevent superinfection by extracellular vaccinia virus through binding to two components of the viral fusion complex (G9 and A16), thereby inhibiting membrane fusion. To investigate how the A56/K2 complex inhibits membrane fusion, we performed experimental evolutionary analyses by repeatedly passaging vaccinia virus in HeLa cells overexpressing the A56 and K2 proteins to isolate adaptive mutant viruses. Genome sequencing of adaptive mutants revealed that they had accumulated a unique G9R open reading frame (ORF) mutation, resulting in a single His44Tyr amino acid change. We engineered a recombinant vaccinia virus to express the G9 mutant protein, and it readily infected HeLa-A56/K2 cells. Moreover, similar to the ΔA56 virus, the G9 mutant virus on HeLa cells had a cell fusion phenotype, indicating that G9-mediated membrane fusion was less prone to inhibition by A56/K2. Coimmunoprecipitation experiments demonstrated that the G9 protein bound to A56/K2 at neutral pH, suggesting that the H44Y mutation did not eliminate the binding of G9 to A56/K2. Interestingly, upon acid treatment to inactivate A56/K2-mediated fusion inhibition, the G9 mutant virus induced robust cell-cell fusion at pH 6, unlike the pH 4.7 required for control and revertant vaccinia viruses. Thus, A56/K2 fusion suppression mainly targets the G9 protein. Moreover, the G9 mutant protein escapes A56/K2-mediated membrane fusion inhibition most likely because it mimics an acid-induced intermediate conformation more prone to membrane fusion. It remains unclear how the multiprotein entry fusion complex of vaccinia virus mediates membrane fusion. Moreover, vaccinia virus contains fusion suppressor proteins to prevent the aberrant activation of this multiprotein complex. Here, we used experimental evolution to identify adaptive mutant viruses that overcome membrane fusion inhibition mediated by the A56/K2 protein complex. We show that the H44Y mutation of the G9 protein is sufficient to overcome A56/K2-mediated membrane fusion inhibition. Treatment of virus-infected cells at different pHs indicated that the H44Y mutation lowers the threshold of fusion inhibition by A56/K2. Our study provides evidence that A56/K2 inhibits the viral fusion complex via the latter's G9 subcomponent. Although the G9 mutant protein still binds to A56/K2 at neutral pH, it is less dependent on low pH for fusion activation, implying that it may adopt a subtle conformational change that mimics a structural intermediate induced by low pH.
对于细胞进入,牛痘病毒需要通过 11 种蛋白质的病毒融合复合物与宿主膜融合,但机制尚不清楚。先前已经表明,病毒蛋白 A56 和 K2 在感染细胞上表达,通过与病毒融合复合物的两个成分(G9 和 A16)结合,防止细胞外牛痘病毒的超感染,从而抑制膜融合。为了研究 A56/K2 复合物如何抑制膜融合,我们通过在过表达 A56 和 K2 蛋白的 HeLa 细胞中反复传代牛痘病毒来进行实验进化分析,以分离适应性突变病毒。适应性突变体的基因组测序表明,它们积累了一个独特的 G9R 开放阅读框(ORF)突变,导致单个 His44Tyr 氨基酸变化。我们设计了一种表达 G9 突变蛋白的重组牛痘病毒,并在 HeLa-A56/K2 细胞中进行了表达。此外,与 ΔA56 病毒类似,G9 突变病毒在 HeLa 细胞上具有细胞融合表型,表明 G9 介导的膜融合不太容易受到 A56/K2 的抑制。共免疫沉淀实验表明,G9 蛋白在中性 pH 下与 A56/K2 结合,表明 H44Y 突变并未消除 G9 与 A56/K2 的结合。有趣的是,在用酸处理使 A56/K2 介导的融合抑制失活后,G9 突变病毒在 pH6 时诱导强烈的细胞-细胞融合,而对照和回复突变牛痘病毒则需要 pH4.7。因此,A56/K2 融合抑制主要针对 G9 蛋白。此外,G9 突变蛋白很可能通过模拟更倾向于膜融合的酸性诱导中间构象来逃避 A56/K2 介导的膜融合抑制。牛痘病毒的多蛋白进入融合复合物如何介导膜融合仍不清楚。此外,牛痘病毒含有融合抑制蛋白,以防止该多蛋白复合物的异常激活。在这里,我们使用实验进化来鉴定克服 A56/K2 蛋白复合物介导的膜融合抑制的适应性突变病毒。我们表明,G9 蛋白的 H44Y 突变足以克服 A56/K2 介导的膜融合抑制。用不同 pH 值处理感染病毒的细胞表明,H44Y 突变降低了 A56/K2 介导的融合抑制的阈值。我们的研究提供了证据表明,A56/K2 通过后者的 G9 亚基抑制病毒融合复合物。尽管 G9 突变蛋白在中性 pH 值下仍与 A56/K2 结合,但它对融合激活的依赖程度较低 pH 值,这意味着它可能采用微妙的构象变化,模拟由低 pH 值诱导的结构中间态。
