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爱泼斯坦-巴尔病毒蛋白激酶BGLF4和核酸外切酶BGLF5对病毒蛋白产生的调节具有相反的作用。

The Epstein-Barr virus protein kinase BGLF4 and the exonuclease BGLF5 have opposite effects on the regulation of viral protein production.

作者信息

Feederle Regina, Mehl-Lautscham Anja M, Bannert Helmut, Delecluse Henri-Jacques

机构信息

German Cancer Research Center, ATV-F100, Im Neuenheimer Feld 242, 69120 Heidelberg, Germany.

出版信息

J Virol. 2009 Nov;83(21):10877-91. doi: 10.1128/JVI.00525-09. Epub 2009 Aug 26.

Abstract

The Epstein-Barr virus BGLF4 and BGLF5 genes encode a protein kinase and an alkaline exonuclease, respectively. Both proteins were previously found to regulate multiple steps of virus replication, including lytic DNA replication and primary egress. However, while inactivation of BGLF4 led to the downregulation of several viral proteins, the absence of BGLF5 had the opposite effect. Using recombinant viruses that lack both viral enzymes, we confirm and extend these initial observations, e.g., by showing that both BGLF4 and BGLF5 are required for proper phosphorylation of the DNA polymerase processivity factor BMRF1. We further found that neither BGLF4 nor BGLF5 is required for baseline viral protein production. Complementation with BGLF5 downregulated mRNA levels and translation of numerous viral genes, though to various degrees, whereas BGLF4 had the opposite effect. BGLF4 and BGLF5 influences on viral expression were most pronounced for BFRF1 and BFLF2, two proteins essential for nuclear egress. For most viral genes studied, cotransfection of BGLF4 and BGLF5 had only a marginal influence on their expression patterns, showing that BGLF4 antagonizes BGLF5-mediated viral gene shutoff. To be able to exert its functions on viral gene expression, BGLF4 must be able to escape BGLF5's shutoff activities. Indeed, we found that BGLF5 stimulated the BGLF4 gene's transcription through an as yet uncharacterized molecular mechanism. The BGLF4/BGLF5 enzyme pair builds a regulatory loop that allows fine-tuning of virus protein production, which is required for efficient viral replication.

摘要

爱泼斯坦-巴尔病毒的BGLF4和BGLF5基因分别编码一种蛋白激酶和一种碱性核酸外切酶。此前发现这两种蛋白都能调节病毒复制的多个步骤,包括裂解性DNA复制和初次释放。然而,虽然BGLF4失活导致几种病毒蛋白表达下调,但BGLF5缺失却产生相反的效果。利用缺乏这两种病毒酶的重组病毒,我们证实并扩展了这些初步观察结果,例如,通过表明DNA聚合酶持续性因子BMRF1的正确磷酸化需要BGLF4和BGLF5。我们还进一步发现,基线病毒蛋白产生不需要BGLF4和BGLF5。用BGLF5互补会下调多种病毒基因的mRNA水平和翻译,不过程度各异,而BGLF4则产生相反的效果。对于核释放所必需的两种蛋白BFRF1和BFLF2,BGLF4和BGLF5对病毒表达的影响最为显著。对于大多数所研究的病毒基因,共转染BGLF4和BGLF5对其表达模式只有轻微影响,表明BGLF4拮抗BGLF5介导的病毒基因关闭。为了能够对病毒基因表达发挥其功能,BGLF4必须能够逃避BGLF5的关闭活性。事实上,我们发现BGLF5通过一种尚未明确的分子机制刺激BGLF4基因的转录。BGLF4/BGLF5酶对构建了一个调节回路,可对病毒蛋白产生进行微调,这是高效病毒复制所必需的。

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本文引用的文献

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Efficient production of infectious viruses requires enzymatic activity of Epstein-Barr virus protein kinase.
Virology. 2009 Jun 20;389(1-2):75-81. doi: 10.1016/j.virol.2009.04.007. Epub 2009 May 8.
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The Epstein-Barr virus alkaline exonuclease BGLF5 serves pleiotropic functions in virus replication.
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