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利用双分子互补技术鉴定哺乳动物细胞中的丝状病毒蛋白-蛋白相互作用。

Characterization of filovirus protein-protein interactions in mammalian cells using bimolecular complementation.

机构信息

Department of Pathobiology, School of Veterinary Medicine, University of Pennsylvania, Philadelphia, PA 19104, USA.

出版信息

J Infect Dis. 2011 Nov;204 Suppl 3(Suppl 3):S817-24. doi: 10.1093/infdis/jir293.

DOI:10.1093/infdis/jir293
PMID:21987757
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3189979/
Abstract

The virion protein 40 (VP40) and nucleoprotein (NP) of Ebola (EBOV) and Marburg viruses (MARV) play key roles during virion assembly and egress. The ability to detect interactions between VP40-VP40, VP40-NP, and NP-NP and follow these complexes as they traffic through mammalian cells would enhance our understanding of the molecular events leading to filovirus assembly and budding, and provide new insights into filovirus replication and pathogenesis. Here, we successfully employed a bimolecular complementation (BiMC) approach to visualize interactions between EBOV and MARV VP40-VP40, NP-NP, and VP40-NP proteins and localize these protein complexes in mammalian cells using confocal microscopy. We demonstrate that VP40-VP40 complexes localized predominantly at the plasma membrane, whereas VP40-NP and NP-NP complexes displayed a more dispersed pattern throughout the cytoplasm. As expected based on previous findings, efficient interactions between EBOV or MARV VP40-VP40 proteins were independent of L-domains PTAPPEY and PPPY, respectively. In contrast, the formation of EBOV or MARV VP40-VP40 complexes was dependent on the previously characterized LPLGVA and LPLGIM motifs of EBOV and MARV VP40 proteins, respectively, indicating that these motifs are important for VP40 oligomerization and subsequent budding. These results highlight the feasibility and usefulness of the BiMC approach as a strategy to further characterize both filovirus protein interactions as well as filovirus-host interactions in real time in the natural environment of the cell.

摘要

埃博拉病毒(EBOV)和马尔堡病毒(MARV)的病毒蛋白 40(VP40)和核蛋白(NP)在病毒体组装和出芽过程中发挥关键作用。能够检测 VP40-VP40、VP40-NP 和 NP-NP 之间的相互作用,并跟踪这些复合物在哺乳动物细胞中的运输,将增强我们对导致丝状病毒组装和出芽的分子事件的理解,并为丝状病毒复制和发病机制提供新的见解。在这里,我们成功地采用双分子互补(BiMC)方法来可视化 EBOV 和 MARV VP40-VP40、NP-NP 和 VP40-NP 蛋白之间的相互作用,并使用共焦显微镜在哺乳动物细胞中定位这些蛋白复合物。我们证明 VP40-VP40 复合物主要定位于质膜,而 VP40-NP 和 NP-NP 复合物在细胞质中呈现更分散的模式。根据先前的发现,EBOV 或 MARV VP40-VP40 蛋白之间的有效相互作用分别独立于 L 结构域 PTAPPEY 和 PPPY。相比之下,EBOV 或 MARV VP40-VP40 复合物的形成依赖于 EBOV 和 MARV VP40 蛋白分别以前表征的 LPLGVA 和 LPLGIM 基序,表明这些基序对 VP40 寡聚化和随后的出芽很重要。这些结果突出了 BiMC 方法作为一种策略的可行性和有用性,可实时在细胞的自然环境中进一步表征丝状病毒蛋白相互作用以及丝状病毒-宿主相互作用。

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Viral and host proteins that modulate filovirus budding.调节丝状病毒出芽的病毒蛋白和宿主蛋白。
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Tsg101 is recruited by a late domain of the nucleocapsid protein to support budding of Marburg virus-like particles.Tsg101 通过核衣壳蛋白的晚期结构域招募,以支持马尔堡病毒样颗粒的出芽。
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Interaction of Tsg101 with Marburg virus VP40 depends on the PPPY motif, but not the PT/SAP motif as in the case of Ebola virus, and Tsg101 plays a critical role in the budding of Marburg virus-like particles induced by VP40, NP, and GP.Tsg101与马尔堡病毒VP40的相互作用依赖于PPPY基序,而不像埃博拉病毒那样依赖于PT/SAP基序,并且Tsg101在由VP40、NP和GP诱导的马尔堡病毒样颗粒出芽过程中起关键作用。
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Role of the transmembrane domain of marburg virus surface protein GP in assembly of the viral envelope.马尔堡病毒表面蛋白GP的跨膜结构域在病毒包膜组装中的作用。
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