McKell Allison O, LaConte Leslie E W, McDonald Sarah M
Virginia Tech Carilion School of Medicine and Research Institute, Roanoke, Virginia, USA.
Department of Biomedical Sciences and Pathobiology, Virginia-Maryland College of Veterinary Medicine, Blacksburg, Virginia, USA.
J Virol. 2017 Mar 13;91(7). doi: 10.1128/JVI.00062-17. Print 2017 Apr 1.
Temperature-sensitive () mutants of simian rotavirus (RV) strain SA11 have been previously created to investigate the functions of viral proteins during replication. One mutant, SA11-C, has a mutation that maps to the gene encoding the VP1 polymerase and shows diminished growth and RNA synthesis at 39°C compared to that at 31°C. In the present study, we sequenced all 11 genes of SA11-C, confirming the presence of an L138P mutation in the VP1 N-terminal domain and identifying 52 additional mutations in four other viral proteins (VP4, VP7, NSP1, and NSP2). To investigate whether the L138P mutation induces a phenotype in VP1 outside the SA11-C genetic context, we employed ectopic expression systems. Specifically, we tested whether the L138P mutation affects the ability of VP1 to localize to viroplasms, which are the sites of RV RNA synthesis, by expressing the mutant form as a green fluorescent protein (GFP) fusion protein (VP1-GFP) (i) in wild-type SA11-infected cells or (ii) in uninfected cells along with viroplasm-forming proteins NSP2 and NSP5. We found that VP1-GFP localized to viroplasms and interacted with NSP2 and/or NSP5 at 31°C but not at 39°C. Next, we tested the enzymatic activity of a recombinant mutant polymerase (rVP1) and found that it synthesized less RNA at 39°C than at 31°C, as well as less RNA than the control at all temperatures. Together, these results provide a mechanistic basis for the phenotype of SA11-C and raise important questions about the role of leucine 138 in supporting key protein interactions and the catalytic function of the VP1 polymerase. RVs cause diarrhea in the young of many animal species, including humans. Despite their medical and economic importance, gaps in knowledge exist about how these viruses replicate inside host cells. Previously, a mutant simian RV (SA11-C) that replicates worse at higher temperatures was identified. This virus has an amino acid mutation in VP1, which is the enzyme responsible for copying the viral RNA genome. The mutation is located in a poorly understood region of the polymerase called the N-terminal domain. In this study, we determined that the mutation reduces the ability of VP1 to properly localize within infected cells at high temperatures, as well as reduced the ability of the enzyme to copy viral RNA in a test tube. The results of this study explain the temperature sensitivity of SA11-C and shed new light on functional protein-protein interaction sites of VP1.
先前已构建了猿猴轮状病毒(RV)SA11株的温度敏感(ts)突变体,以研究病毒蛋白在复制过程中的功能。其中一个突变体SA11-C发生了一个映射到编码VP1聚合酶基因的突变,与31°C时相比,其在39°C时生长和RNA合成减少。在本研究中,我们对SA11-C的所有11个基因进行了测序,证实了VP1 N端结构域中存在L138P突变,并在其他四种病毒蛋白(VP4、VP7、NSP1和NSP2)中鉴定出另外52个突变。为了研究L138P突变在SA11-C基因背景之外是否会在VP1中诱导ts表型,我们采用了异位表达系统。具体而言,我们通过在野生型SA11感染的细胞中(i)或在未感染细胞中与形成病毒工厂的蛋白NSP2和NSP5一起(ii)将突变形式表达为绿色荧光蛋白(GFP)融合蛋白(VP1-GFP),来测试L138P突变是否影响VP1定位于病毒工厂(RV RNA合成位点)的能力。我们发现VP1-GFP在31°C时定位于病毒工厂并与NSP2和/或NSP5相互作用,但在39°C时则不然。接下来,我们测试了重组突变聚合酶(rVP1)的酶活性,发现其在39°C时合成的RNA比在31°C时少,并且在所有温度下合成的RNA都比对照少。总之,这些结果为SA11-C的ts表型提供了机制基础,并提出了关于亮氨酸138在支持关键蛋白相互作用和VP1聚合酶催化功能中的作用的重要问题。轮状病毒可导致包括人类在内的许多动物幼崽腹泻。尽管它们具有医学和经济重要性,但对于这些病毒如何在宿主细胞内复制仍存在知识空白。先前已鉴定出一种在较高温度下复制较差的突变猿猴轮状病毒(SA11-C)。这种病毒在VP1中有一个氨基酸突变,VP1是负责复制病毒RNA基因组的酶。该突变位于聚合酶中一个了解较少的区域,称为N端结构域。在本研究中,我们确定该突变降低了VP1在高温下在感染细胞内正确定位的能力,以及该酶在试管中复制病毒RNA的能力。本研究结果解释了SA11-C的温度敏感性,并为VP1的功能性蛋白-蛋白相互作用位点提供了新的线索。
