首页> 美国卫生研究院文献>Journal of Virology >The Herpesvirus Saimiri Open Reading Frame (ORF) 50 (Rta) Protein Contains an AT Hook Required for Binding to the ORF 50 Response Element in Delayed-Early Promoters
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The Herpesvirus Saimiri Open Reading Frame (ORF) 50 (Rta) Protein Contains an AT Hook Required for Binding to the ORF 50 Response Element in Delayed-Early Promoters

机译:疱疹病毒Saimiri开放阅读框(ORF)50(Rta)蛋白包含与延迟早期启动子中的ORF 50响应元件结合所需的AT钩

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摘要

The herpesvirus saimiri open reading frame (ORF) 50 encodes two proteins, which activate transcription directly, following interactions with delayed-early (DE) promoters containing a specific motif. In this report, we demonstrate that ORF 50 contains a DNA binding domain that has homology to an AT hook DNA binding motif. Deletion analysis of this domain reduces ORF 50-mediated transactivation of the DE ORF 6 and ORF 57 promoters by 100 and 90%, respectively. Furthermore, gel retardation experiments demonstrated that the AT hook motif is required for binding the ORF 50 response element in the promoters of DE genes. Single site-directed mutagenesis of the AT hook revealed that mutation of the glycine residue at position 408 to an alanine reduces ORF 50 transactivation of the ORF 57 promoter by 40%. Moreover, the mutation of multiple basic residues in conjunction with the glycine residue within the core element of the AT hook abolishes ORF 50-mediated transactivation. In addition, p50GFPΔAT-hook is capable of functioning as a trans-dominant mutant, leading to a reduction in virus production of approximately 50% compared to that for wild-type ORF 50.
机译:疱疹病毒赛密里开放阅读框(ORF)50编码两个蛋白质,它们与包含特定基序的延迟早期(DE)启动子相互作用后直接激活转录。在此报告中,我们证明ORF 50包含与AT钩DNA结合基序具有同源性的DNA结合域。该结构域的缺失分析分别将ORF 50介导的DE ORF 6和ORF 57启动子的反式激活分别降低了100%和90%。此外,凝胶阻滞实验表明,AT钩基序是结合DE基因启动子中的ORF 50反应元件所必需的。 AT钩的单点定向诱变显示,第408位甘氨酸残基突变为丙氨酸可使ORF 57启动子的ORF 50反式激活降低40%。此外,多个基本残基的突变与AT钩核心元件内的甘氨酸残基一起消除了ORF 50介导的反式激活。另外,p50GFPΔAT-钩能够作为反式突变体起作用,与野生型ORF 50相比,导致病毒产量降低约50%。

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