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雀麦花叶病毒编码的假定RNA封端活性:复制酶蛋白1a对鸟苷酸的甲基化和共价结合。

Putative RNA capping activities encoded by brome mosaic virus: methylation and covalent binding of guanylate by replicase protein 1a.

作者信息

Ahola T, Ahlquist P

机构信息

Institute for Molecular Virology, Howard Hughes Medical Institute, University of Wisconsin-Madison, Madison, Wisconsin 53706, USA.

出版信息

J Virol. 1999 Dec;73(12):10061-9. doi: 10.1128/JVI.73.12.10061-10069.1999.

Abstract

Brome mosaic virus (BMV) RNA replication is directed by two virus-encoded proteins, 1a and 2a. The amino-terminal half of 1a is a distant homolog of alphavirus nonstructural protein nsP1, which has been implicated in capping viral RNAs. In this study, we examined the enzymatic activities of BMV 1a expressed in yeast, where the protein is fully functional in RNA replication. 1a methylated GTP, dGTP, and the cap analogs GpppG and GpppA, using S-adenosylmethionine (AdoMet) as the methyl donor. Product analysis by nuclear magnetic resonance spectroscopy showed that 1a methylation was specific for guanine position 7. Additionally, 1a interacted with GTP to form a covalent 1a-m(7)GMP complex. This reaction was specific for GTP, required AdoMet, and was accompanied by transfer of (3)H-methyl from AdoMet to the covalent 1a-guanylate complex. The covalent complex could be immunoprecipitated by 1a antibodies. The 1a-m(7)GMP complex was inhibited in catalyzing further methyltransferase reactions. Mutation of conserved amino acids in the N-terminal half of 1a reduced both methyltransferase and covalent complex formation activities to very low or undetectable levels. Covalent 1a-guanylate complex formation took place in similar, AdoMet-dependent fashion in extracts of BMV-infected barley protoplasts. These results show that BMV 1a has activities similar to those of alphavirus nsP1, demonstrating conservation of these putative capping functions across a wide span of sequence divergence within the alphavirus-like superfamily. Conservation of this unusual combination of functions also supports the inference that the superfamily caps viral RNAs by an unusual pathway proceeding via a m(7)GMP intermediate.

摘要

雀麦花叶病毒(BMV)的RNA复制由两种病毒编码蛋白1a和2a指导。1a的氨基末端一半是甲病毒非结构蛋白nsP1的远亲同源物,后者与病毒RNA的加帽有关。在本研究中,我们检测了在酵母中表达的BMV 1a的酶活性,该蛋白在RNA复制中具有完全功能。1a使用S-腺苷甲硫氨酸(AdoMet)作为甲基供体,使GTP、dGTP以及帽类似物GpppG和GpppA甲基化。通过核磁共振光谱进行的产物分析表明,1a甲基化对鸟嘌呤的7位具有特异性。此外,1a与GTP相互作用形成共价的1a-m(7)GMP复合物。该反应对GTP具有特异性,需要AdoMet,并伴随着(3)H-甲基从AdoMet转移到共价的1a-鸟苷酸复合物上。该共价复合物可被1a抗体免疫沉淀。1a-m(7)GMP复合物在催化进一步的甲基转移酶反应中受到抑制。1a氨基末端一半中保守氨基酸的突变将甲基转移酶和共价复合物形成活性都降低到非常低或无法检测的水平。在BMV感染的大麦原生质体提取物中,共价的1a-鸟苷酸复合物形成以类似的、依赖AdoMet的方式发生。这些结果表明,BMV 1a具有与甲病毒nsP1相似的活性,证明了在甲病毒样超家族内广泛序列差异的情况下,这些假定的加帽功能的保守性。这种不寻常的功能组合的保守性也支持了这样的推断,即该超家族通过一条经由m(7)GMP中间体的不寻常途径对病毒RNA进行加帽。

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本文引用的文献

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RNA capping enzyme and DNA ligase: a superfamily of covalent nucleotidyl transferases.
Mol Microbiol. 1995 Aug;17(3):405-10. doi: 10.1111/j.1365-2958.1995.mmi_17030405.x.

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