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仅用 11 个 cDNA 即可生成编码病毒基因组的重组轮状病毒。

Generation of recombinant rotaviruses from just 11 cDNAs encoding a viral genome.

机构信息

Department of Virology and Parasitology, Fujita Health University School of Medicine, Toyoake, Aichi 470-1192, Japan.

Department of Virology and Parasitology, Fujita Health University School of Medicine, Toyoake, Aichi 470-1192, Japan.

出版信息

Virus Res. 2020 Sep;286:198075. doi: 10.1016/j.virusres.2020.198075. Epub 2020 Jun 24.

Abstract

Reverse genetics technology allows one to engineer replication-competent viruses from cloned cDNAs at will. Since the establishment of the initial reverse genetics system for species A rotaviruses (RVAs) requiring a helper virus in 2006, attempts have been successfully made to improve this technology. Efficient generation of replication-competent RVAs is now possible from just 11 T7-driven plasmids encoding an RVA genome when the quantity ratio of the two rescue T7-driven plasmids for the NSP2 and NSP5 segments is increased by 3-fold in relation to that of the other nine plasmids (11 plasmid-only system). Further, it is now possible to generate recombinant RVAs even with severely less efficient infectivity by using the 11 plasmid-only system, which has not been possible with the existing approaches. More importantly, the 11 plasmid-only system does not need any helper expression plasmid, and thus this simplest and robust system has a clear advantage over the existing systems in terms of safety. This 11 plasmid-only system should contribute to the development of safe next-generation vaccines and vaccine vectors.

摘要

反向遗传学技术使人们能够随心所欲地从克隆 cDNA 中构建具有复制能力的病毒。自 2006 年建立了需要辅助病毒的 A 群轮状病毒(RVA)的初始反向遗传学系统以来,人们一直试图改进这项技术。现在,只需 11 个 T7 驱动的质粒就能有效地生成具有复制能力的 RVAs,这些质粒编码 RVA 基因组,当用于 NSP2 和 NSP5 片段的两个拯救 T7 驱动质粒的数量比相对于其他九个质粒增加 3 倍时(11 质粒系统)。此外,现在即使使用感染效率严重降低的 11 质粒系统也可以生成重组 RVAs,这是现有方法无法实现的。更重要的是,11 质粒系统不需要任何辅助表达质粒,因此与现有系统相比,该系统在安全性方面具有明显优势。这种 11 质粒系统应有助于开发安全的下一代疫苗和疫苗载体。

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