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Identification of two ATR-dependent phosphorylation sites on coronavirus nucleocapsid protein with nonessential functions in viral replication and infectivity in cultured cells

机译:鉴定冠状病毒核衣壳蛋白上两个ATR依赖的磷酸化位点它们在培养细胞的病毒复制和感染力中具有非必需功能

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摘要

Coronavirus encodes an extensively phosphorylated and highly basic nucleocapsid (N) protein. Previous studies have identified Ser190, Ser192, Thr378 and Ser379 as the phosphorylation sites for coronavirus infectious bronchitis virus (IBV) N protein. In this study, we show that phosphorylation at Thr378 and Ser379 sites is dependent on the ataxia-telangiectasia mutated (ATM) and Rad3-related (ATR), a kinase activated during IBV replication. Introduction of Ala substitutions at these two sites individually, in combination of the two and together with other two sites (Ser190 and Ser192) into an infectious IBV clone did not affect recovery of the recombinant viruses containing the mutations. A mutant virus (rIBV-Nm4) carrying the four Ala substitutions grew at a similar, if not better, growth rate as wild type virus. This study reveals a cellular kinase responsible for phosphorylation of a coronavirus N protein at two positions and the functional consequence of this modification on coronavirus replication.
机译:冠状病毒编码广泛磷酸化和高度碱性的核衣壳(N)蛋白。先前的研究已将Ser190,Ser192,Thr378和Ser379鉴定为冠状病毒感染性支气管炎病毒(IBV)N蛋白的磷酸化位点。在这项研究中,我们显示Thr378和Ser379位点的磷酸化取决于共济失调毛细血管扩张突变(ATM)和Rad3相关(ATR),这是一种在IBV复制过程中激活的激酶。分别在这两个位点,两个位点以及其他两个位点(Ser190和Ser192)的组合中将Ala取代引入感染性IBV克隆中,不会影响包含该突变的重组病毒的恢复。带有四个Ala取代的突变病毒(rIBV-Nm4)的生长速度与野生型病毒相近,甚至更高。这项研究揭示了负责在两个位置上冠状病毒N蛋白磷酸化的细胞激酶,以及这种修饰对冠状病毒复制的功能性后果。

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