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SuPReMe: a rapid reverse genetics method to generate clonal populations of recombinant RNA viruses

机译:SuPReMe:一种快速反向遗传学方法,可产生重组RNA病毒的克隆种群

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Reverse genetics systems enable the manipulation of viral genomes and are proving to be essential for studying RNA viruses. Methods for generating clonal virus populations are particularly useful for studying the impact of genomic modifications on viral properties. Here, by exploiting a chikungunya virus model, we compare viral populations and their replicative fitness when generated using either the rapid and user-friendly PCR-based ISA (Infectious Subgenomic Amplicons) method or classical infectious clone technology. As anticipated, the ISA method resulted in greater genetic diversity of the viral populations, but no significant difference in viral fitness in vitro was observed. On the basis of these results, a new ISA-derived reverse genetics procedure was developed. This method, designated ‘SuPReMe’ (Subgenomic Plasmids Recombination Method), in which digested plasmids containing subgenomic DNA fragments were directly transfected into permissive cells,?retains the following major advantages of the ISA method: it is rapid, flexible and does not require the cloning of complete genomes. Moreover, SuPReMe has been shown to produce virus populations with genetic diversity and replicative fitness similar to those obtained using conventional infectious clone technology. SuPReMe, therefore, represents an effective and promising option for the rapid generation of clonal recombinant populations of single-stranded positive-sense RNA viruses.
机译:逆向遗传学系统可以操纵病毒基因组,并且被证明对于研究RNA病毒至关重要。产生克隆病毒种群的方法对于研究基因组修饰对病毒特性的影响特别有用。在这里,通过利用基孔肯雅病毒模型,我们比较了使用快速且用户友好的基于PCR的ISA(传染性亚基因组扩增子)方法或经典传染性克隆技术生成的病毒种群及其复制适应性。如预期的那样,ISA方法导致病毒种群具有更大的遗传多样性,但在体外病毒适应性方面没有观察到明显差异。基于这些结果,开发了一种新的ISA衍生的反向遗传学程序。这种方法称为“ SuPReMe”(亚基因组质粒重组方法),其中将含有亚基因组DNA片段的消化质粒直接转染到允许的细胞中,保留了ISA方法的以下主要优点:快速,灵活且不需要完整基因组的克隆。而且,已证明SuPReMe可以产生具有遗传多样性和复制适应性的病毒种群,类似于使用常规传染性克隆技术获得的病毒种群。因此,SuPReMe代表了快速生成单链正义RNA病毒克隆重组种群的有效且有前途的选择。

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