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The EHV-1 UL4 protein that tempers viral gene expression interacts with cellular transcription factors

机译:调节病毒基因表达的EHV-1 UL4蛋白与细胞转录因子相互作用

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The UL4 gene is conserved within the genome of defective interfering particles of equine herpesvirus type 1 (EHV-1) that mediate persistent infection. Here, we show that the UL4 protein inhibits EHV-1 reporter gene expression by decreasing the level of transcribed mRNA. The UL4 protein did not bind any gene class of EHV-1 promoters in electromobility or chromatin immunoprecipitation assays, but directly interacted with the TATA box-binding protein (TBP) and the carboxy-terminal domain of RNA polymerase II both in vitro (GST-pulldown assays) and in infected cells (coimmunoprecipitation analyses). Microarray analyses of the expression of the 78 EHV-1 genes revealed that viral late genes important for virion assembly displayed enhanced expression in cells infected with UL4-null virus as compared to wild-type or UL4-restored EHV-1. Quantitative PCR analyses showed that viral DNA replication was not retarded in cells infected with the UL4-null virus as compared to wild-type EHV-1.
机译:UL4基因在介导持续感染的1型马疱疹病毒(EHV-1)的有缺陷干扰颗粒的基因组内是保守的。在这里,我们显示UL4蛋白通过降低转录的mRNA水平抑制EHV-1报告基因的表达。 UL4蛋白在电动性或染色质免疫沉淀试验中不结合EHV-1启动子的任何基因类别,但在体外均与TATA盒结合蛋白(TBP)和RNA聚合酶II的羧基末端结构域直接相互作用(GST-下拉检测)和感染细胞中(免疫共沉淀分析)。对78个EHV-1基因表达的微阵列分析表明,与野生型或经UL4还原的EHV-1相比,对于病毒体装配重要的病毒晚期基因在感染UL4无效病毒的细胞中显示出增强的表达。定量PCR分析表明,与野生型EHV-1相比,在感染了UL4-无效病毒的细胞中病毒DNA复制没有受到阻碍。

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