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与带帽RNA结合的人源IFIT1结构揭示了适应性mRNA结合以及识别N1和N2核糖2'-O甲基化的机制。

Structure of human IFIT1 with capped RNA reveals adaptable mRNA binding and mechanisms for sensing N1 and N2 ribose 2'-O methylations.

作者信息

Abbas Yazan M, Laudenbach Beatrice Theres, Martínez-Montero Saúl, Cencic Regina, Habjan Matthias, Pichlmair Andreas, Damha Masad J, Pelletier Jerry, Nagar Bhushan

机构信息

Department of Biochemistry and Groupe de Recherche Axe sur la Structure des Proteines, McGill University, Montreal, QC, Canada H3G 0B1.

Innate Immunity Laboratory, Max-Planck Institute of Biochemistry, 82152 Martinsried/Munich, Germany.

出版信息

Proc Natl Acad Sci U S A. 2017 Mar 14;114(11):E2106-E2115. doi: 10.1073/pnas.1612444114. Epub 2017 Mar 1.

Abstract

IFIT1 (IFN-induced protein with tetratricopeptide repeats-1) is an effector of the host innate immune antiviral response that prevents propagation of virus infection by selectively inhibiting translation of viral mRNA. It relies on its ability to compete with the translation initiation factor eIF4F to specifically recognize foreign capped mRNAs, while remaining inactive against host mRNAs marked by ribose 2'-O methylation at the first cap-proximal nucleotide (N1). We report here several crystal structures of RNA-bound human IFIT1, including a 1.6-Å complex with capped RNA. IFIT1 forms a water-filled, positively charged RNA-binding tunnel with a separate hydrophobic extension that unexpectedly engages the cap in multiple conformations ( and ) giving rise to a relatively plastic and nonspecific mode of binding, in stark contrast to eIF4E. Cap-proximal nucleotides encircled by the tunnel provide affinity to compete with eIF4F while allowing IFIT1 to select against N1 methylated mRNA. Gel-shift binding assays confirm that N1 methylation interferes with IFIT1 binding, but in an RNA-dependent manner, whereas translation assays reveal that N1 methylation alone is not sufficient to prevent mRNA recognition at high IFIT1 concentrations. Structural and functional analysis show that 2'-O methylation at N2, another abundant mRNA modification, is also detrimental for RNA binding, thus revealing a potentially synergistic role for it in self- versus nonself-mRNA discernment. Finally, structure-guided mutational analysis confirms the importance of RNA binding for IFIT1 restriction of a human coronavirus mutant lacking viral N1 methylation. Our structural and biochemical analysis sheds new light on the molecular basis for IFIT1 translational inhibition of capped viral RNA.

摘要

IFIT1(干扰素诱导的具有四肽重复序列的蛋白-1)是宿主先天免疫抗病毒反应的效应器,它通过选择性抑制病毒mRNA的翻译来阻止病毒感染的传播。它依靠与翻译起始因子eIF4F竞争的能力,特异性识别外来的带帽mRNA,而对在第一个帽近端核苷酸(N1)处被核糖2'-O甲基化标记的宿主mRNA保持无活性。我们在此报告了RNA结合的人IFIT1的几个晶体结构,包括与带帽RNA形成的1.6 Å复合物。IFIT1形成一个充满水的带正电荷的RNA结合通道,带有一个单独的疏水延伸,该延伸意外地以多种构象与帽结合(和),产生相对可塑性和非特异性的结合模式,这与eIF4E形成鲜明对比。通道环绕的帽近端核苷酸提供亲和力以与eIF4F竞争,同时允许IFIT1选择N1甲基化的mRNA。凝胶迁移结合试验证实N1甲基化会干扰IFIT1结合,但以RNA依赖的方式,而翻译试验表明仅N1甲基化不足以在高IFIT1浓度下阻止mRNA识别。结构和功能分析表明,N2处的2'-O甲基化,另一种丰富的mRNA修饰,对RNA结合也有害,从而揭示了其在自身与非自身mRNA识别中的潜在协同作用。最后,结构导向的突变分析证实了RNA结合对于IFIT1限制缺乏病毒N1甲基化的人冠状病毒突变体的重要性。我们的结构和生化分析为IFIT1对带帽病毒RNA的翻译抑制的分子基础提供了新的见解。

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