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Comparative inhibition of cellular transcription by vesicular stomatitis virus serotypes New Jersey and Indiana: role of each viral leader RNA.

机译:新泽西州和印第安纳州水疱性口炎病毒血清型对细胞转录的比较抑制:每种病毒前导RNA的作用。

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摘要

We compared the ability of the leader RNAs of the New Jersey and Indiana serotypes of vesicular stomatitis virus to inhibit transcription in infected host cells. The level of cellular RNA synthesis in cells infected with either serotype was drastically reduced by 5 h after infection. Studies with UV-inactivated virus demonstrated that shutoff of cellular RNA synthesis directly correlated with the ability of the infecting virus to transcribe its plus-stranded leader RNA. Although both serotypes inhibited cellular RNA synthesis, the Indiana serotype reduced synthesis to lower levels. In addition, an examination of the kinetics of leader RNA synthesis in vivo indicated that up to four times more leader RNA was produced in cells infected with the Indiana serotype than in those infected with the New Jersey serotype. However, in vivo studies also suggested that the leader RNA of the New Jersey serotype was a more efficient RNA inhibitor than was the Indiana serotype leader RNA. Although up to 2,900 copies of the leader RNA per cell could be detected in infected cells, only 550 copies of the Indiana and 100 copies of the New Jersey leader RNAs per cell were present in infected cells that were demonstrating 50% of the maximal inhibition of RNA synthesis. In an in vitro system, leader RNAs of both serotypes inhibited DNA-dependent transcription of the adenovirus late promoter and adenovirus-associated RNA genes, but the New Jersey serotype leader was also a better inhibitor in this reconstituted system. Data from the dose response of inhibition by each leader suggest that polymerase III transcription was more sensitive to inhibition by viral leaders than was polymerase II transcription. Polyadenylated viral mRNAs and the NS and N gene starts transcribed by both serotypes did not significantly inhibit transcription at levels at which the corresponding leader RNAs were inhibitory. Overall, our results strongly suggest a role for the plus-stranded leader RNAs of the New Jersey and Indiana serotypes of vesicular stomatitis virus in inhibiting cellular transcription in vivo. We discuss differences in the nucleotide sequences of the two leader RNAs in relation to their differences in biological activity and to potential regulatory sequences.
机译:我们比较了新泽西州和印第安那水疱性口炎病毒血清型的前导RNA抑制感染宿主细胞中转录的能力。感染后5小时,两种血清型感染的细胞中细胞RNA合成水平均急剧降低。用紫外线灭活的病毒进行的研究表明,细胞RNA合成的关闭与感染病毒转录其正链前导RNA的能力直接相关。尽管两种血清型均抑制细胞RNA合成,但印第安纳州血清型将合成降低至较低水平。此外,对体内前导RNA合成动力学的研究表明,感染印第安纳血清型的细胞产生的前导RNA的产量是感染新泽西州血清型的细胞的多达四倍。但是,体内研究还表明,新泽西州血清型前导RNA比印第安纳州血清型前导RNA更有效。尽管在受感染的细胞中每个细胞最多可检测到2,900拷贝的前导RNA,但在受感染的细胞中,每个细胞仅存在550份印第安纳州和100份新泽西州的前导RNA,这显示了50%的最大抑制率。 RNA合成。在体外系统中,两种血清型的前导RNA均抑制腺病毒晚期启动子和与腺病毒相关的RNA基因的DNA依赖性转录,但在该重组系统中,新泽西州的血清型前导也是更好的抑制剂。来自每个前导物抑制作用的剂量响应的数据表明,聚合酶III转录比聚合酶II转录对病毒前导物的抑制更敏感。聚腺苷酸化的病毒mRNA和由两种血清型开始转录的NS和N基因在相应的前导RNA被抑制的水平上均未显着抑制转录。总体而言,我们的结果强烈暗示了新泽西州和印第安纳州血清型水疱性口炎病毒的正链前导RNA在体内抑制细胞转录中的作用。我们讨论了两个前导RNA的核苷酸序列在生物学活性和潜在的调控序列方面的差异。

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