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RNA-dependent activation of primer RNA production by influenza virus polymerase: different regions of the same protein subunit constitute the two required RNA-binding sites.

机译:流感病毒聚合酶产生引物RNA的RNA依赖性激活:同一蛋白质亚基的不同区域构成了两个必需的RNA结合位点。

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摘要

The capped RNA primers required for the initiation of influenza virus mRNA synthesis are produced by the viral polymerase itself, which consists of three proteins PB1, PB2 and PA. Production of primers is activated only when the 5'- and 3'-terminal sequences of virion RNA (vRNA) bind sequentially to the polymerase, indicating that vRNA molecules function not only as templates for mRNA synthesis but also as essential cofactors which activate catalytic functions. Using thio U-substituted RNA and UV crosslinking, we demonstrate that the 5' and 3' sequences of vRNA bind to different amino acid sequences in the same protein subunit, the PB1 protein. Mutagenesis experiments proved that these two amino acid sequences constitute the functional RNA-binding sites. The 5' sequence of vRNA binds to an amino acid sequence centered around two arginine residues at positions 571 and 572, causing an allosteric alteration which activates two new functions of the polymerase complex. In addition to the PB2 protein subunit acquiring the ability to bind 5'-capped ends of RNAs, the PB1 protein itself acquires the ability to bind the 3' sequence of vRNA, via a ribonucleoprotein 1 (RNP1)-like motif, amino acids 249-256, which contains two phenylalanine residues required for binding. Binding to this site induces a second allosteric alteration which results in the activation of the endonuclease that produces the capped RNA primers needed for mRNA synthesis. Hence, the PB1 protein plays a central role in the catalytic activity of the viral polymerase, not only in the catalysis of RNA-chain elongation but also in the activation of the enzyme activities that produce capped RNA primers.
机译:流感病毒mRNA合成所需的带帽RNA引物由病毒聚合酶本身产生,该酶由三种蛋白PB1,PB2和PA组成。仅当病毒粒子RNA(vRNA)的5'和3'末端序列顺序结合到聚合酶上时,才激活引物的产生,这表明vRNA分子不仅充当mRNA合成的模板,而且还充当激活催化功能的必需辅因子。使用硫代U-取代的RNA和UV交联,我们证明了vRNA的5'和3'序列与同一蛋白亚基PB1蛋白中的不同氨基酸序列结合。诱变实验证明这两个氨基酸序列构成了功能性RNA结合位点。 vRNA的5'序列与一个氨基酸序列结合,该氨基酸序列位于位置571和572的两个精氨酸残基周围,从而引起变构改变,从而激活了聚合酶复合物的两个新功能。除了PB2蛋白亚基具有结合RNA的5'末端的能力外,PB1蛋白本身还具有通过核糖蛋白1(RNP1)样基序,氨基酸249结合vRNA 3'序列的能力。 -256,含有两个结合所需的苯丙氨酸残基。与该位点的结合诱导第二个变构改变,其导致核酸内切酶的激活,从而产生mRNA合成所需的带帽RNA引物。因此,PB1蛋白在病毒聚合酶的催化活性中起着中心作用,不仅在RNA链延长的催化中,而且在产生带帽RNA引物的酶活性的激活中都起着重要作用。

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