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Ded1p, a conserved DExD/H-box translation factor, can promote yeast L-A virus negative-strand RNA synthesis in vitro

机译:保守的DExD / H盒翻译因子Ded1p可在体外促进酵母L-A病毒负链RNA合成

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Viruses are intracellular parasites that must use the host machinery to multiply. Identification of the host factors that perform essential functions in viral replication is thus of crucial importance to the understanding of virus–host interactions. Here we describe Ded1p, a highly conserved DExD/H-box translation factor, as a possible host factor recruited by the yeast L-A double-stranded RNA (dsRNA) virus. We found that Ded1p interacts specifically and strongly with Gag, the L-A virus coat protein. Further analysis revealed that Ded1p interacts with the L-A virus in an RNA-independent manner and, as a result, L-A particles can be affinity purified via this interaction. The affinity-purified L-A particles are functional, as they are capable of synthesizing RNA in vitro. Critically, using purified L-A particles, we demonstrated that Ded1p specifically promotes L-A dsRNA replication by accelerating the rate of negative-strand RNA synthesis in vitro. In light of these data, we suggest that Ded1p may be a part of the long sought after activity shown to promote yeast viral dsRNA replication. This and the fact that Ded1p is also required for translating brome mosaic virus RNA2 in yeast thus raise the intriguing possibility that Ded1p is one of the key host factors favored by several evolutionarily related RNA viruses, including the human hepatitis C virus.
机译:病毒是必须使用宿主机制繁殖的细胞内寄生虫。因此,鉴定在病毒复制中起关键作用的宿主因子对于理解病毒与宿主的相互作用至关重要。在这里,我们将高度保守的DExD / H-box翻译因子Ded1p描述为酵母L-A双链RNA(dsRNA)病毒募集的可能宿主因子。我们发现Ded1p与L-A病毒外壳蛋白Gag特异性强相互作用。进一步的分析表明,Ded1p以不依赖RNA的方式与L-A病毒相互作用,因此,可以通过这种相互作用亲和纯化L-A颗粒。亲和纯化的L-A颗粒具有功能性,因为它们能够在体外合成RNA。至关重要的是,使用纯化的L-A颗粒,我们证明Ded1p通过加速体外负链RNA的合成速率来特异性地促进L-A dsRNA复制。根据这些数据,我们建议Ded1p可能是长期以来寻求促进酵母病毒dsRNA复制的活性的一部分。这以及在酵母中翻译溴化花叶病毒RNA2也需要Ded1p的事实,因此增加了一种有趣的可能性,即Ded1p是几种进化相关RNA病毒(包括人类丙型肝炎病毒)偏爱的关键宿主因子之一。

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