靠近对出芽至关重要的劳氏肉瘤病毒晚期结构域的赖氨酸。
Lysines close to the Rous sarcoma virus late domain critical for budding.
作者信息
Spidel Jared L, Craven Rebecca C, Wilson Carol B, Patnaik Akash, Wang Huating, Mansky Louis M, Wills John W
机构信息
Department of Microbiology and Immunology, Pennsylvania State University College of Medicine, 500 University Dr., P.O. Box 850, Hershey, PA 17033, USA.
出版信息
J Virol. 2004 Oct;78(19):10606-16. doi: 10.1128/JVI.78.19.10606-10616.2004.
The release of retroviruses from the plasma membrane requires host factors that are believed to be recruited to the site of budding by the late (L) domain of the virus-encoded Gag protein. The L domain of Rous sarcoma virus (RSV) has been shown to interact with a ubiquitin (Ub) ligase, and budding of this virus is dependent on Ub. RSV is similar to other retroviruses in that it contains approximately 100 molecules of Ub, but it is unique in that none of these molecules has been found to be conjugated to Gag. If transient ubiquitination of RSV Gag is required for budding, then replacement of the target lysine(s) with arginine should prevent the addition of Ub and reduce budding. Based on known sites of ubiquitination in other viruses, the important lysines would likely reside near the L domain. In RSV, there are five lysines located just upstream of the L domain in a region of the matrix (MA) protein that is dispensable for membrane binding, and replacement of these with arginine (mutant 1-5KR) reduced budding 80 to 90%. The block to budding was found to be on the plasma membrane; however, the few virions that were released had normal size, morphology, and infectivity. Budding was restored when any one of the residues was changed back to lysine or when lysines were inserted in novel positions, either within this region of MA or within the downstream p10 sequence. Moreover, the 1-5KR mutant could be rescued into particles by coexpression of budding-competent Gag molecules. These data argue that the phenotype of mutant 1-5KR is not due to a conformational defect. Consistent with the idea that efficient budding requires a specific role for lysines, human T-cell leukemia virus type 1, which does not bud well compared to RSV and lacks lysines close to its L domain, was found to be released at a higher level upon introduction of lysines near its L domain. This report strongly supports the hypothesis that ubiquitination of the RSV Gag protein (and perhaps those of other retroviruses) is needed for efficient budding.
逆转录病毒从质膜释放需要宿主因子,据信这些宿主因子由病毒编码的Gag蛋白的晚期(L)结构域招募至出芽位点。劳氏肉瘤病毒(RSV)的L结构域已被证明与一种泛素(Ub)连接酶相互作用,且该病毒的出芽依赖于Ub。RSV与其他逆转录病毒相似之处在于它含有约100个Ub分子,但独特之处在于尚未发现这些分子中有任何一个与Gag共价结合。如果RSV Gag的瞬时泛素化是出芽所必需的,那么用精氨酸取代靶赖氨酸应该会阻止Ub的添加并减少出芽。基于其他病毒中已知的泛素化位点,重要的赖氨酸可能位于L结构域附近。在RSV中,基质(MA)蛋白区域中L结构域上游紧邻有五个赖氨酸,该区域对于膜结合并非必需,用精氨酸取代这些赖氨酸(突变体1 - 5KR)使出芽减少了80%至90%。发现出芽受阻发生在质膜上;然而,少数释放出的病毒粒子具有正常的大小、形态和感染性。当任何一个残基变回赖氨酸或在MA的该区域内或下游p10序列中的新位置插入赖氨酸时,出芽得以恢复。此外,通过共表达具有出芽能力的Gag分子,1 - 5KR突变体可以被拯救到病毒颗粒中。这些数据表明突变体1 - 5KR的表型并非由于构象缺陷。与有效出芽需要赖氨酸发挥特定作用这一观点一致的是,与RSV相比出芽不佳且其L结构域附近缺乏赖氨酸的1型人类T细胞白血病病毒,在其L结构域附近引入赖氨酸后被发现释放水平更高。本报告有力地支持了以下假说:RSV Gag蛋白(可能还有其他逆转录病毒的Gag蛋白)的泛素化是有效出芽所必需的。
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