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Influenza A viruses with different amino acid residues at PB2-627 displaydistinct replication properties in vitro and in vivo:revealing the sequence plasticity of PB2-627 position

机译:PB2-627上具有不同氨基酸残基的甲型流感病毒展示体外和体内独特的复制特性:揭示PB2-627位置的顺序可塑性

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摘要

Sequence analyses of influenza PB2 sequences indicate that the 627 position almost exclusively contains either lysine (K) or glutamic acid (E), suggesting a high sequence constraint at this genetic marker. Here, we used a site-directed random mutagenesis method to demonstrate that PB2-627 position has a high sequence plasticity. Recombinant viruses carrying various amino acid residues at this position are viable in cell cultures. These PB2-627 mutants showed various polymerase activities and replication kinetics in mammalian and avian cells as well as pathogenicity in mice. Serially passaging these mutants in MDCK cells generated some compensatory PB2 mutations that can restore polymerase activities of the PB2-627 mutants. Of these, PB2-D309N was identified as a novel one. Besides showing that influenza virus can tolerate a wide range of amino acid residues at the PB2-627 position, this study also demonstrates a potential strategy to identify novel mutations that can enhance viral polymerase.
机译:流感PB2序列的序列分析表明627位几乎只包含赖氨酸(K)或谷氨酸(E),这表明该遗传标记存在较高的序列限制。在这里,我们使用了定点随机诱变方法来证明PB2-627位置具有较高的序列可塑性。在此位置带有各种氨基酸残基的重组病毒在细胞培养物中是可行的。这些PB2-627突变体在哺乳动物和鸟类细胞中表现出各种聚合酶活性和复制动力学,并且在小鼠中具有致病性。将这些突变体在MDCK细胞中连续传代会产生一些补偿性PB2突变,这些突变可恢复PB2-627突变体的聚合酶活性。其中,PB2-D309N被鉴定为新型。除了表明流感病毒可以耐受PB2-627位置上的广泛氨基酸残基外,这项研究还证明了潜在的策略来鉴定可以增强病毒聚合酶的新突变。

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