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HIV-1 Gag-RNA interaction occurs at a perinuclear/centrosomal site; Analysis by confocal microscopy and FRET

机译:HIV-1 Gag-RNA相互作用发生在核周围/中央体位点;共聚焦显微镜和FRET分析

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The Gag polyprotein is the major structural protein of human immunodeficiency virus-1 (HIV-1) constituting the viral core. Between translation on cytoplasmic polysomes and assembly into viral particles at the plasma membrane, it specifically captures the RNA genome of the virus through binding RNA structural motifs (packaging signals -Psi) in the RNA. RNA is believed to be a structural facilitator of Gag assembly. Using a combined approach of immunofluorescence detection of Gag protein and in situ hybridisation detection of viral genomic RNA, we demonstrate that Gag protein colocalises early after expression with Psi+ RNA in the perinuclear region and also colocalises with centrioles. Colocalised RNA and protein subsequently traffic through the cytoplasm to the plasma membrane of the cell. Gag expressed from Psi- RNA diffuses throughout the cell. It is not found at centrioles and shows delayed cytoplasmic colocalisation with the RNA genome. RNA capture through Psi does not influence binding of Gag to microfilaments. Gag does not bind to tubulin during export. The presence of the packaging signal may coordinate capture of Psi+ RNA by Gag protein at the centrosome followed by their combined transport to the site of budding. HIV-1 Psi thus acts as a subcellular localisation signal as well as a high-affinity-binding site for Gag.
机译:Gag多蛋白是构成病毒核心的人类免疫缺陷病毒1(HIV-1)的主要结构蛋白。在细胞质多核糖体的翻译和质膜上组装成病毒颗粒之间,它通过结合RNA中的RNA结构基序(包装信号-Psi)来特异性捕获病毒的RNA基因组。 RNA被认为是Gag装配的结构促进剂。使用Gag蛋白的免疫荧光检测和病毒基因组RNA的原位杂交检测相结合的方法,我们证明了Gag蛋白与Psi + RNA表达后在核周区域中早期共定位,并与中心粒共定位。随后,共定位的RNA和蛋白质通过细胞质运输到细胞的质膜。由Psi-RNA表达的Gag扩散到整个细胞中。它在中心体上没有发现,并且显示出与RNA基因组的细胞质共定位延迟。通过Psi捕获RNA不会影响Gag与微丝的结合。出口期间,堵嘴不与微管蛋白结合。包装信号的存在可以协调Gag蛋白在中心体上捕获Psi + RNA,然后将它们组合转运到出芽部位。因此,HIV-1 Psi充当亚细胞定位信号以及Gag的高亲和力结合位点。

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