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An improved reverse genetics system for mammalian orthoreoviruses.

机译:哺乳动物正咽病毒的改良反向遗传学系统。

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摘要

Mammalian orthoreoviruses (reoviruses) are highly useful models for studies of double-stranded RNA virus replication and pathogenesis. We previously developed a strategy to recover prototype reovirus strain T3D from cloned cDNAs transfected into murine L929 fibroblast cells. Here, we report the development of a second-generation reovirus reverse genetics system featuring several major improvements: (1) the capacity to rescue prototype reovirus strain T1L, (2) reduction of required plasmids from 10 to 4, and (3) isolation of recombinant viruses following transfection of baby hamster kidney cells engineered to express bacteriophage T7 RNA polymerase. The efficiency of virus rescue using the 4-plasmid strategy was substantially increased in comparison to the original 10-plasmid system. We observed full compatibility of T1L and T3D rescue vectors when intermixed to produce a panel of T1LxT3D monoreassortant viruses. Improvements to the reovirus reverse genetics system enhance its applicability for studies of reovirus biology and clinical use.
机译:哺乳动物正咽病毒(呼肠孤病毒)是用于研究双链RNA病毒复制和发病机制的高度有用的模型。我们先前开发了一种策略,用于从转染到鼠L929成纤维细胞的克隆cDNA中恢复原型呼肠孤病毒株T3D。在这里,我们报告了第二代呼肠孤病毒反向遗传学系统的开发,该系统具有几个主要改进:(1)拯救呼肠孤病毒原型T1L的能力,(2)将所需质粒从10减少到4,以及(3)重组仓鼠肾细胞转染后重组病毒,可表达噬菌体T7 RNA聚合酶。与原始的10个质粒系统相比,使用4个质粒策略的病毒救援效率大大提高了。当混合产生一组T1LxT3D单重排列病毒时,我们观察到T1L和T3D救援载体的完全相容性。呼肠孤病毒反向遗传学系统的改进增强了其在呼肠孤病毒生物学和临床应用研究中的适用性。

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