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液泡蛋白分选途径在埃博拉病毒释放中的作用独立于TSG101相互作用。

Involvement of vacuolar protein sorting pathway in Ebola virus release independent of TSG101 interaction.

作者信息

Silvestri Lynn S, Ruthel Gordon, Kallstrom George, Warfield Kelly L, Swenson Dana L, Nelle Timothy, Iversen Patrick L, Bavari Sina, Aman M Javad

机构信息

United States Army Medical Research Institute of Infectious Diseases, Fort Detrick, MD 21704, USA.

出版信息

J Infect Dis. 2007 Nov 15;196 Suppl 2:S264-70. doi: 10.1086/520610.

Abstract

Budding of Ebola virus (EBOV) particles from the plasma membrane of infected cells requires viral and host proteins. EBOV virus matrix protein VP40 recruits TSG101, an ESCRT-1 (host cell endosomal sorting complex required for transport-1) complex protein in the vacuolar protein sorting (vps) pathway, to the plasma membrane during budding. Involvement of other vps proteins in EBOV budding has not been established. Therefore, we used VP40 deletion analysis, virus-like particle-release assays, and confocal microscopy to investigate the potential role of ESCRT-1 proteins VPS4, VPS28, and VPS37B in EBOV budding. We found that VP40 could redirect each protein from endosomes to the cell surface independently of TSG101 interaction. A lack of VPS4 adenosine triphosphatase activity reduced budding by up to 80%. Inhibition of VPS4 gene expression by use of phosphorodiamidite morpholino antisense oligonucleotides protected mice from lethal EBOV infection. These data show that EBOV can use vps proteins independently of TSG101 for budding and reveal VPS4 as a potential target for filovirus therapeutics.

摘要

埃博拉病毒(EBOV)颗粒从受感染细胞的质膜出芽需要病毒蛋白和宿主蛋白。在出芽过程中,EBOV病毒基质蛋白VP40将液泡蛋白分选(vps)途径中的ESCRT-1(宿主细胞内体转运所需分选复合物-1)复合物蛋白TSG101募集到质膜。尚未确定其他vps蛋白是否参与EBOV出芽。因此,我们使用VP40缺失分析、病毒样颗粒释放试验和共聚焦显微镜来研究ESCRT-1蛋白VPS4、VPS28和VPS37B在EBOV出芽中的潜在作用。我们发现,VP40可以独立于TSG101相互作用将每种蛋白从内体重新定向到细胞表面。VPS4三磷酸腺苷酶活性的缺失使出芽减少高达80%。使用磷二酰胺吗啉代反义寡核苷酸抑制VPS4基因表达可保护小鼠免受致命的EBOV感染。这些数据表明,EBOV可以独立于TSG101使用vps蛋白进行出芽,并揭示VPS4是丝状病毒治疗的潜在靶点。

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