首页> 外文期刊>Current Microbiology: An International Journal >Host filamentous actin is associated with Heliothis armigera single nucleopolyhedrosis virus (HaSNPV) nucleocapsid transport to the host nucleus.
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Host filamentous actin is associated with Heliothis armigera single nucleopolyhedrosis virus (HaSNPV) nucleocapsid transport to the host nucleus.

机译:宿主丝状肌动蛋白与棉铃虫单核多角体病毒(HaSNPV)核衣壳转运到宿主核有关。

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VP39 is the major capsid protein of Heliothis armigera nucleopolyhedrovirus (HaSNPV), and it might have induced the aggregation of host cellular actin in vitro in our previous study. We demonstrated here that VP39 could interact with host actin in vivo in Helicoverpazea (Hz-AM1 cells) through coimmunoprecipitation assay. With confocal immunofluorescence microscopy, it was confirmed further that the released HaSNPV nucleocapsids/VP39s in the host cytoplasm (0.5 hours after infection) colocalized where the actin aggregated and that the nucleocapsids/VP39s were transported from the host cytoplasm to the nucleus (2 hours after infection). Because cytochalasin D (CD) was used to prevent host global actin from forming filamentous structures, the infection efficiency of the recombinant virus HaSNPV/gfp Delta p74, with the gfp gene inserted into HaSNPV p74 gene loci, was decreased to 7.34%, whereas it was 34.7% in normal host cells and 55.7% in the cells whose microtubules had been destroyed by colchicin. Ultramicroscopy assay revealed that HaSNPV nucleocapsids could enter the cytoplasm of CD-treated cells but could not be transported to the nucleus, which resulted in the lower infection efficiency of HaSNPV/gfp Delta p74 in CD-treated cells. However, transportation of the nucleocapsids was not inhibited in colchicin-treated cells, demonstrating that the transportation of HaSNPV nucleocapsid from the cytoplasm to the nucleus was associated with actin filaments but not with microtubules, a conclusion that is also strongly supported by evidence from the RNAi interference of host actin during HaSNPV infection..
机译:VP39是棉铃虫核多角体病毒(HaSNPV)的主要衣壳蛋白,在我们先前的研究中,它可能在体外诱导了宿主细胞肌动蛋白的聚集。我们在这里证明了VP39可以通过共免疫沉淀试验在Helicoverpazea(Hz-AM1细胞)体内与宿主肌动蛋白相互作用。通过共聚焦免疫荧光显微镜检查,进一步证实释放的HaSNPV核衣壳/ VP39s在宿主细胞质中(感染后0.5小时)共定位在肌动蛋白聚集的地方,并且核衣壳/ VP39s从宿主细胞质中转运到细胞核(2小时后)感染)。由于使用细胞松弛素D(CD)来阻止宿主全局肌动蛋白形成丝状结构,因此将带有gfp基因插入HaSNPV p74基因位点的重组病毒HaSNPV / gfp Delta p74的感染效率降低至7.34%,而在正常宿主细胞中,其为34.7%,在其微管被秋水仙素破坏的细胞中为55.7%。显微检测结果表明,HaSNPV核衣壳可以进入CD处理细胞的胞质,但不能转运到细胞核,导致HaSNPV / gfp Delta p74在CD处理细胞中的感染效率较低。然而,在秋水仙素处理过的细胞中,核衣壳的转运并没有受到抑制,这表明HaSNPV核衣壳从细胞质到核的转运与肌动蛋白丝相关,而与微管无关,这一结论也得到了RNAi证据的有力支持。 HaSNPV感染过程中宿主肌动蛋白的干扰

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