Wilkie Adrian R, Lawler Jessica L, Coen Donald M
Department of Biological Chemistry and Molecular Pharmacology and Committee on Virology, Harvard Medical School, Boston, Massachusetts, USA.
Department of Biological Chemistry and Molecular Pharmacology and Committee on Virology, Harvard Medical School, Boston, Massachusetts, USA
mBio. 2016 Aug 23;7(4):e01254-16. doi: 10.1128/mBio.01254-16.
Herpesviruses, which include important pathogens, remodel the host cell nucleus to facilitate infection. This remodeling includes the formation of structures called replication compartments (RCs) in which herpesviruses replicate their DNA. During infection with the betaherpesvirus, human cytomegalovirus (HCMV), viral DNA synthesis occurs at the periphery of RCs within the nuclear interior, after which assembled capsids must reach the inner nuclear membrane (INM) for translocation to the cytoplasm (nuclear egress). The processes that facilitate movement of HCMV capsids to the INM during nuclear egress are unknown. Although an actin-based mechanism of alphaherpesvirus capsid trafficking to the INM has been proposed, it is controversial. Here, using a fluorescently-tagged, nucleus-localized actin-binding peptide, we show that HCMV, but not herpes simplex virus 1, strongly induced nuclear actin filaments (F-actin) in human fibroblasts. Based on studies using UV inactivation and inhibitors, this induction depended on viral gene expression. Interestingly, by 24 h postinfection, nuclear F-actin formed thicker structures that appeared by super-resolution microscopy to be bundles of filaments. Later in infection, nuclear F-actin primarily localized along the RC periphery and between the RC periphery and the nuclear rim. Importantly, a drug that depolymerized nuclear F-actin caused defects in production of infectious virus, capsid accumulation in the cytoplasm, and capsid localization near the nuclear rim, without decreasing capsid accumulation in the nucleus. Thus, our results suggest that for at least one herpesvirus, nuclear F-actin promotes capsid movement to the nuclear periphery and nuclear egress. We discuss our results in terms of competing models for these processes.
The mechanisms underlying herpesvirus nuclear egress have not been fully determined. In particular, how newly assembled capsids move to the inner nuclear membrane for envelopment is uncertain and controversial. In this study, we show that HCMV, an important human pathogen, induces actin filaments in the nuclei of infected cells and that an inhibitor of nuclear F-actin impairs nuclear egress and capsid localization toward the nuclear periphery. Herpesviruses are widespread pathogens that cause or contribute to an array of human diseases. A better understanding of how herpesvirus capsids traffic in the nucleus may uncover novel targets for antiviral intervention and elucidate aspects of the nuclear cytoskeleton, about which little is known.
疱疹病毒包括重要的病原体,它会重塑宿主细胞核以促进感染。这种重塑包括形成称为复制区室(RCs)的结构,疱疹病毒在其中复制其DNA。在感染β疱疹病毒——人巨细胞病毒(HCMV)期间,病毒DNA合成发生在核内RCs的周边,之后组装好的衣壳必须到达内核膜(INM)以便转运到细胞质(核输出)。在核输出过程中促进HCMV衣壳向INM移动的过程尚不清楚。尽管有人提出了基于肌动蛋白的α疱疹病毒衣壳转运到INM的机制,但存在争议。在这里,我们使用荧光标记的、定位于细胞核的肌动蛋白结合肽,发现HCMV而非单纯疱疹病毒1能在人成纤维细胞中强烈诱导细胞核肌动蛋白丝(F-肌动蛋白)。基于紫外线灭活和抑制剂的研究,这种诱导依赖于病毒基因表达。有趣的是,在感染后24小时,细胞核F-肌动蛋白形成了更厚的结构,通过超分辨率显微镜观察,这些结构似乎是细丝束。在感染后期,细胞核F-肌动蛋白主要定位于RCs周边以及RCs周边与核边缘之间。重要的是,一种使细胞核F-肌动蛋白解聚的药物导致感染性病毒产生缺陷、衣壳在细胞质中积累以及衣壳在核边缘附近定位,而不会减少衣壳在细胞核中的积累。因此,我们的结果表明,对于至少一种疱疹病毒,细胞核F-肌动蛋白促进衣壳向核周边移动和核输出。我们根据这些过程的竞争模型讨论了我们的结果。
疱疹病毒核输出的潜在机制尚未完全确定。特别是,新组装的衣壳如何移动到内核膜进行包裹尚不确定且存在争议。在这项研究中,我们表明,重要的人类病原体HCMV会在受感染细胞的细胞核中诱导肌动蛋白丝,并且细胞核F-肌动蛋白的抑制剂会损害核输出和衣壳向核周边的定位。疱疹病毒是广泛传播的病原体,可导致或促成一系列人类疾病。更好地了解疱疹病毒衣壳在细胞核中的转运方式可能会发现抗病毒干预的新靶点,并阐明核细胞骨架的相关方面,而目前对此了解甚少。
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