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RNA 病毒的反向遗传学:不改变病毒表型控制病毒种群多样性的基于 ISA 的方法。

Reverse Genetics of RNA Viruses: ISA-Based Approach to Control Viral Population Diversity without Modifying Virus Phenotype.

机构信息

Unité des Virus Émergents (UVE: Aix-Marseille Univ-IRD 190-Inserm 1207-IHU Méditerranée Infection), 13005 Marseille, France.

出版信息

Viruses. 2019 Jul 20;11(7):666. doi: 10.3390/v11070666.

Abstract

Reverse genetic systems are essential for the study of RNA viruses. Infectious clones remain the most widely used systems to manipulate viral genomes. Recently, a new PCR-based method called ISA (infectious subgenomic amplicons) has been developed. This approach has resulted in greater genetic diversity of the viral populations than that observed using infectious clone technology. However, for some studies, generation of clonal viral populations is necessary. In this study, we used the tick-borne encephalitis virus as model to demonstrate that utilization of a very high-fidelity, DNA-dependent DNA polymerase during the PCR step of the ISA procedure gives the possibility to reduce the genetic diversity of viral populations. We also concluded that the fidelity of the polymerase is not the only factor influencing this diversity. Studying the impact of genotype modification on virus phenotype is a crucial step for the development of reverse genetic methods. Here, we also demonstrated that the utilization of different PCR polymerases did not affect the phenotype (replicative fitness in cellulo and virulence in vivo) compared to the initial ISA procedure and the use of an infectious clone. In conclusion, we provide here an approach to control the genetic diversity of RNA viruses without modifying their phenotype.

摘要

反向遗传学系统对于研究 RNA 病毒至关重要。传染性克隆仍然是最广泛用于操纵病毒基因组的系统。最近,开发了一种称为 ISA(感染性亚基因组扩增子)的新基于 PCR 的方法。与使用传染性克隆技术相比,该方法导致病毒群体的遗传多样性更大。然而,对于某些研究,需要生成克隆病毒群体。在这项研究中,我们使用蜱传脑炎病毒作为模型,证明在 ISA 程序的 PCR 步骤中使用非常高保真的 DNA 依赖性 DNA 聚合酶,有可能降低病毒群体的遗传多样性。我们还得出结论,聚合酶的保真度不是影响这种多样性的唯一因素。研究基因型修饰对病毒表型的影响是开发反向遗传学方法的关键步骤。在这里,我们还证明与初始 ISA 程序和使用传染性克隆相比,使用不同的 PCR 聚合酶不会影响表型(细胞内复制适应性和体内毒力)。总之,我们在此提供了一种控制 RNA 病毒遗传多样性而不改变其表型的方法。

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