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The Cap Snatching of Segmented Negative Sense RNA Viruses as a Tool to Map the Transcription Start Sites of Heterologous Co-infecting Viruses

机译:分段负义RNA病毒的帽抢夺作为一种工具来映射异源共感染病毒的转录起始位点

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Identification of the transcription start sites (TSSs) of a virus is of great importance to understand and dissect the mechanism of viral genome transcription but this often requires costly and laborious experiments. Many segmented negative-sense RNA viruses (sNSVs) cleave capped leader sequences from a large variety of mRNAs and use these cleaved leaders as primers for transcription in a conserved process called cap snatching. The recent developments in high-throughput sequencing have made it possible to determine most, if not all, of the capped RNAs snatched by a sNSV. Here, we show that rice stripe tenuivirus (RSV), a plant-infecting sNSV, co-infects Nicotiana benthamiana with two different begomoviruses and snatches capped leader sequences from their mRNAs. By determining the 5′ termini of a single RSV mRNA with high-throughput sequencing, the 5′ ends of almost all the mRNAs of the co-infecting begomoviruses could be identified and mapped on their genomes. The findings in this study provide support for the using of the cap snatching of sNSVs as a tool to map viral TSSs.
机译:病毒转录起始位点(TSS)的识别对于理解和剖析病毒基因组转录的机制非常重要,但这通常需要昂贵且费力的实验。许多分段的负义RNA病毒(sNSV)会从多种mRNA中切割带帽的前导序列,并使用这些裂解的前导序列作为转录的引物,称为保守的抓帽过程。高通量测序的最新进展使得有可能确定大多数(即使不是全部)被sNSV捕获的带帽RNA。在这里,我们显示出水稻条纹腱炎病毒(RSV),一种植物感染性sNSV,与两种不同的bemomovirus病毒共同感染了本氏烟草,并从其mRNA中捕获了加帽的前导序列。通过用高通量测序确定单个RSV mRNA的5'末端,可以鉴定出共感染的bemomovirus几乎所有mRNA的5'末端,并将其定位在其基因组上。这项研究的发现为使用sNSV的抢帽作为绘制病毒TSS的工具提供了支持。

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