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Comparative analysis of Reoviridae reverse genetics methods

机译:呼肠孤病毒科反向遗传学方法的比较分析

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Effective methods to engineer the segmented, double-stranded RNA genomes of Reoviridae viruses have only recently been developed. Mammalian orthoreoviruses (MRV) and bluetongue virus (BTV) can be recovered from entirely recombinant reagents, significantly improving the capacity to study the replication, pathogenesis, and transmission of these viruses. Conversely, rotaviruses (RVs), which are the major etiological agent of severe gastroenteritis in infants and children, have thus far only been modified using single-segment replacement methods. Reoviridae reverse genetics techniques universally rely on site-specific initiation of transcription by T7 RNA polymerase to generate the authentic 5' end of recombinant RNA segments, but they vary in how the RNAs are introduced into cells: recombinant BTV is recovered by transfection of in vitro transcribed RNAs, whereas recombinant MRV and RV RNAs are transcribed intracellularly from transfected plasmid cDNAs. Additionally, several parameters have been identified in each system that are essential for recombinant virus recovery. Generating recombinant BTV requires the use of 5' capped RNAs and is enhanced by multiple rounds of RNA transfection, suggesting that translation of viral proteins is likely the rate-limiting step. For RV, the efficiency of recovery is almost entirely dependent on the strength of the selection mechanism used to isolate the single-segment recombinant RV from the unmodified helper virus. The reverse genetics methods for BTV and RV are presented and compared to the previously described MRV methods. Analysis and comparison of each method suggest several key lines of research that might lead to a reverse genetics system for RV, analogous to those used for MRV and BTV. ? 2012.
机译:工程化呼肠孤病毒科的分段,双链RNA基因组的有效方法只是最近才被开发出来。哺乳动物正咽病毒(MRV)和蓝舌病毒(BTV)可以从完全重组的试剂中回收,从而大大提高了研究这些病毒的复制,发病机制和传播的能力。相反,轮状病毒(RVs)是婴儿和儿童中严重胃肠炎的主要病因,迄今仅使用单段替代方法进行了修饰。 Reoviridae逆向遗传学技术普遍依靠T7 RNA聚合酶的特定位点起始转录来生成重组RNA片段的真实5'末端,但是它们在将RNA引入细胞中的方式有​​所不同:重组BTV通过体外转染来回收转录的RNA,而重组MRV和RV RNA是从转染的质粒cDNA细胞内转录的。另外,在每个系统中已经鉴定了几个对于重组病毒回收必不可少的参数。产生重组BTV需要使用5'帽RNA,并通过多轮RNA转染而增强,这表明病毒蛋白的翻译可能是限速步骤。对于RV,恢复效率几乎完全取决于用于从未修饰的辅助病毒中分离单段重组RV的选择机制的强度。介绍了BTV和RV的反向遗传学方法,并将其与先前描述的MRV方法进行了比较。对每种方法的分析和比较表明,有几个关键的研究领域可能会导致RV的反向遗传学系统,类似于用于MRV和BTV的系统。 ? 2012。

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