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Production of infectious RNA transcripts from Sindbis virus cDNA clones: mapping of lethal mutations, rescue of a temperature-sensitive marker, and in vitro mutagenesis to generate defined mutants

机译:从Sindbis病毒cDNA克隆产生感染性RNA转录本:致死突变的定位,挽救温度敏感标记以及体外诱变以生成确定的突变体

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摘要

We constructed full-length cDNA clones of Sindbis virus that can be transcribed in vitro by SP6 RNA polymerase to produce infectious genome-length transcripts. Viruses produced from in vitro transcripts are identical to Sindbis virus and show strain-specific phenotypes reflecting the source of RNA used for cDNA synthesis. The cDNA clones were used to confirm the mapping of the causal mutation of ts2 to the capsid protein. A general strategy for mapping Sindbis virus mutations is described and was used to identify two lethal mutations in an original full-length construct which did not produce infectious transcripts. An XbaI linker was inserted in the cDNA clone near the transcriptional start of the subgenomic mRNA; the resulting virus retains the XbaI recognition sequence, thus providing formal evidence that viruses are derived from in vitro transcripts of cDNA clones. The potential applications of the cDNA clones are discussed.
机译:我们构建了Sindbis病毒的全长cDNA克隆,可以通过SP6 RNA聚合酶在体外转录以产生感染性基因组长度的转录本。由体外转录本产生的病毒与Sindbis病毒相同,并且显示出菌株特异性的表型,反映了用于cDNA合成的RNA的来源。 cDNA克隆用于确认ts2的因果突变到衣壳蛋白的作图。描述了一种映射Sindbis病毒突变的通用策略,该策略用于识别原始的全长构建体中的两个致死突变,该原始全长构建体不产生感染性转录本。将XbaI接头插入到亚基因组mRNA转录起点附近的cDNA克隆中。最终的病毒保留了XbaI识别序列,从而提供了正式的证据,证明病毒源自cDNA克隆的体外转录本。讨论了cDNA克隆的潜在应用。

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