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委内瑞拉马脑炎病毒nsP1对mRNA的加帽作用:功能特性及对抗病毒研究的意义

mRNA Capping by Venezuelan Equine Encephalitis Virus nsP1: Functional Characterization and Implications for Antiviral Research.

作者信息

Li Changqing, Guillén Jaime, Rabah Nadia, Blanjoie Alexandre, Debart Françoise, Vasseur Jean-Jacques, Canard Bruno, Decroly Etienne, Coutard Bruno

机构信息

CNRS, AFMB UMR 7257, Marseille, France Aix-Marseille Université, AFMB UMR 7257, Marseille, France.

IBMM UMR 5247 CNRS-Université Montpellier-ENSCM, Montpellier, France.

出版信息

J Virol. 2015 Aug;89(16):8292-303. doi: 10.1128/JVI.00599-15. Epub 2015 Jun 3.

Abstract

UNLABELLED

Alphaviruses are known to possess a unique viral mRNA capping mechanism involving the viral nonstructural protein nsP1. This enzyme harbors methyltransferase (MTase) and nsP1 guanylylation (GT) activities catalyzing the transfer of the methyl group from S-adenosylmethionine (AdoMet) to the N7 position of a GTP molecule followed by the formation of an m(7)GMP-nsP1 adduct. Subsequent transfer of m(7)GMP onto the 5' end of the viral mRNA has not been demonstrated in vitro yet. Here we report the biochemical characterization of Venezuelan equine encephalitis virus (VEEV) nsP1. We have developed enzymatic assays uncoupling the different reactions steps catalyzed by nsP1. The MTase and GT reaction activities were followed using a nonhydrolyzable GTP (GIDP) substrate and an original Western blot assay using anti-m3G/m(7)G-cap monoclonal antibody, respectively. The GT reaction is stimulated by S-adenosyl-l-homocysteine (Ado-Hcy), the product of the preceding MTase reaction, and metallic ions. The covalent linking between nsP1 and m(7)GMP involves a phosphamide bond between the nucleotide and a histidine residue. Final guanylyltransfer onto RNA was observed for the first time with an alphavirus nsP1 using a 5'-diphosphate RNA oligonucleotide whose sequence corresponds to the 5' end of the viral genome. Alanine scanning mutagenesis of residues H37, H45, D63, E118, Y285, D354, R365, N369, and N375 revealed their respective roles in MT and GT reactions. Finally, the inhibitory effects of sinefungin, aurintricarboxylic acid (ATA), and ribavirin triphosphate on MTase and capping reactions were investigated, providing possible avenues for antiviral research.

IMPORTANCE

Emergence or reemergence of alphaviruses represents a serious health concern, and the elucidation of their replication mechanisms is a prerequisite for the development of specific inhibitors targeting viral enzymes. In particular, alphaviruses are able, through an original reaction sequence, to add to their mRNA a cap required for their protection against cellular nucleases and initiation of viral proteins translation. In this study, the capping of a 5' diphosphate synthetic RNA mimicking the 5' end of an alphavirus mRNA was observed in vitro for the first time. The different steps for this capping are performed by the nonstructural protein 1 (nsP1). Reference compounds known to target the viral capping inhibited nsP1 enzymatic functions, highlighting the value of this enzyme in antiviral development.

摘要

未标记

已知甲病毒具有一种独特的病毒mRNA加帽机制,该机制涉及病毒非结构蛋白nsP1。这种酶具有甲基转移酶(MTase)和nsP1鸟苷酸化(GT)活性,催化甲基从S-腺苷甲硫氨酸(AdoMet)转移到GTP分子的N7位,随后形成m(7)GMP-nsP1加合物。m(7)GMP随后转移到病毒mRNA的5'端在体外尚未得到证实。在这里,我们报告了委内瑞拉马脑炎病毒(VEEV)nsP1的生化特性。我们开发了酶促测定法,将nsP1催化的不同反应步骤解偶联。分别使用不可水解的GTP(GIDP)底物和使用抗m3G/m(7)G帽单克隆抗体的原始蛋白质印迹法跟踪MTase和GT反应活性。GT反应受到前一个MTase反应的产物S-腺苷-L-高半胱氨酸(Ado-Hcy)和金属离子的刺激。nsP1与m(7)GMP之间的共价连接涉及核苷酸与组氨酸残基之间的磷酰胺键。首次使用与病毒基因组5'端序列对应的5'-二磷酸RNA寡核苷酸,观察到甲病毒nsP1将鸟苷酸最终转移到RNA上。对H37、H45、D63、E118、Y285、D354、R365、N369和N375残基进行丙氨酸扫描诱变,揭示了它们在MT和GT反应中的各自作用。最后,研究了杀稻瘟菌素、金精三羧酸(ATA)和三磷酸利巴韦林对MTase和加帽反应的抑制作用,为抗病毒研究提供了可能的途径。

重要性

甲病毒的出现或重新出现是一个严重的健康问题,阐明其复制机制是开发针对病毒酶的特异性抑制剂的先决条件。特别是,甲病毒能够通过一个原始的反应序列,在其mRNA上添加一个帽,以保护其免受细胞核酸酶的攻击并启动病毒蛋白的翻译。在这项研究中,首次在体外观察到模拟甲病毒mRNA 5'端的5'-二磷酸合成RNA的加帽。这种加帽的不同步骤由非结构蛋白1(nsP1)执行。已知靶向病毒加帽的参考化合物抑制了nsP1的酶功能,突出了这种酶在抗病毒开发中的价值。

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