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通过串联蛋白质组学分析和 RNAi 筛选鉴定丝状病毒相关的必需宿主因子。

Identification of essential filovirion-associated host factors by serial proteomic analysis and RNAi screen.

机构信息

The United States Army Medical Research Institute of Infectious Diseases, 1425 Porter Street, Fort Detrick, Frederick, MD 21702, USA.

出版信息

Mol Cell Proteomics. 2010 Dec;9(12):2690-703. doi: 10.1074/mcp.M110.003418. Epub 2010 Aug 11.

Abstract

An assessment of the total protein composition of filovirus (ebolavirus and marburgvirus) virions is currently lacking. In this study, liquid chromatography-linked tandem mass spectrometry of purified ebola and marburg virions was performed to identify associated cellular proteins. Host proteins involved in cell adhesion, cytoskeleton, cell signaling, intracellular trafficking, membrane organization, and chaperones were identified. Significant overlap exists between this data set and proteomic studies of disparate viruses, including HIV-1 and influenza A, generated in multiple cell types. However, the great majority of proteins identified here have not been previously described to be incorporated within filovirus particles. Host proteins identified by liquid chromatography-linked tandem mass spectrometry could lack biological relevance because they represent protein contaminants in the virus preparation, or because they are incorporated within virions by chance. These issues were addressed using siRNA library-mediated gene knockdown (targeting each identified virion-associated host protein), followed by filovirus infection. Knockdown of several host proteins (e.g. HSPA5 and RPL18) significantly interfered with ebolavirus and marburgvirus infection, suggesting specific and relevant virion incorporation. Notably, select siRNAs inhibited ebolavirus, but enhanced marburgvirus infection, suggesting important differences between the two viruses. The proteomic analysis presented here contributes to a greater understanding of filovirus biology and potentially identifies host factors that can be targeted for antiviral drug development.

摘要

目前缺乏对丝状病毒(埃博拉病毒和马尔堡病毒)病毒粒子的总蛋白组成的评估。在这项研究中,对纯化的埃博拉病毒和马尔堡病毒进行了液相色谱串联质谱分析,以鉴定相关的细胞蛋白。鉴定到了涉及细胞黏附、细胞骨架、细胞信号转导、细胞内运输、膜组织和伴侣蛋白的宿主蛋白。与在多种细胞类型中生成的不同病毒(包括 HIV-1 和流感 A 病毒)的蛋白质组学研究相比,该数据集存在显著重叠。然而,这里鉴定到的绝大多数蛋白以前没有被描述为包含在丝状病毒粒子中。通过液相色谱串联质谱鉴定到的宿主蛋白可能缺乏生物学相关性,因为它们代表病毒制剂中的蛋白污染物,或者因为它们偶然包含在病毒粒子中。通过使用 siRNA 文库介导的基因敲低(针对每个鉴定到的病毒相关宿主蛋白)解决了这些问题,然后进行了丝状病毒感染。敲低几种宿主蛋白(例如 HSPA5 和 RPL18)显著干扰了埃博拉病毒和马尔堡病毒感染,表明特定且相关的病毒粒子掺入。值得注意的是,一些 siRNA 抑制了埃博拉病毒,但增强了马尔堡病毒感染,表明这两种病毒之间存在重要差异。这里呈现的蛋白质组学分析有助于更好地理解丝状病毒生物学,并可能鉴定出可作为抗病毒药物开发目标的宿主因子。

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