细胞抑制因子抑制人巨细胞病毒从UL127启动子的转录。
Cellular repressor inhibits human cytomegalovirus transcription from the UL127 promoter.
作者信息
Lashmit Philip E, Lundquist Christopher A, Meier Jeffery L, Stinski Mark F
机构信息
Department of Microbiology, Carver College of Medicine, University of Iowa, Iowa City, IA 52242, USA.
出版信息
J Virol. 2004 May;78(10):5113-23. doi: 10.1128/jvi.78.10.5113-5123.2004.
The region of the human cytomegalovirus (HCMV) genome between the UL127 promoter and the major immediate-early (MIE) enhancer is referred to as the unique region. The role of this region during a viral infection is not known. In wild-type HCMV-infected permissive fibroblasts, there is no transcription from the UL127 promoter at any time during productive infection. Our investigators previously reported that the region upstream of the UL127 TATA box repressed expression from the UL127 promoter (C. A. Lundquist et al., J. Virol. 73:9039-9052, 1999). The region was reported to contain functional NF1 DNA binding sites (L. Hennighausen and B. Fleckenstein, EMBO J. 5:1367-1371, 1986). Sequence analysis of this region detected additional consensus binding sites for three transcriptional regulatory proteins, FoxA (HNF-3), suppressor of Hairy wing, and CAAT displacement protein. The cis-acting elements in the unique region prevented activation of the early UL127 promoter by the HCMV MIE proteins. In contrast, deletion of the region permitted very high activation of the UL127 promoter by the viral MIE proteins. Mutation of the NF1 sites had no effect on the basal activity of the promoter. To determine the role of the other sites in the context of the viral genome, recombinant viruses were generated in which each putative repressor site was mutated and the effect on the UL127 promoter was analyzed. Mutation of the putative Fox-like site resulted in a significant increase in expression from the viral early UL127 promoter. Insertion of wild-type Fox-like sites between the HCMV immediate-early (IE) US3 TATA box and the upstream NF-kappaB-responsive enhancer (R2) also significantly decreased gene expression, but mutated Fox-like sites did not. The wild-type Fox-like site inhibits activation of a viral IE enhancer-containing promoter. Cellular protein, which is present in uninfected or infected permissive cell nuclear extracts, binds to the wild-type Fox-like site but not to mutated sites. Reasons for repression of UL127 gene transcription during productive infection are discussed.
人巨细胞病毒(HCMV)基因组中位于UL127启动子和主要立即早期(MIE)增强子之间的区域被称为独特区域。该区域在病毒感染过程中的作用尚不清楚。在野生型HCMV感染的允许性成纤维细胞中,在生产性感染的任何时候,UL127启动子都没有转录。我们的研究人员之前报道过,UL127 TATA框上游的区域抑制了UL127启动子的表达(C.A.伦德奎斯特等人,《病毒学杂志》73:9039 - 9052,1999)。据报道,该区域含有功能性NF1 DNA结合位点(L.亨尼豪森和B.弗莱肯斯坦,《欧洲分子生物学组织杂志》5:1367 - 1371,1986)。对该区域的序列分析检测到另外三个转录调节蛋白的共有结合位点,即FoxA(肝细胞核因子3)、毛翅抑制因子和CAAT置换蛋白。独特区域中的顺式作用元件阻止了HCMV MIE蛋白对早期UL127启动子的激活。相反,删除该区域允许病毒MIE蛋白对UL127启动子进行非常高的激活。NF1位点的突变对启动子的基础活性没有影响。为了确定病毒基因组背景下其他位点的作用,构建了重组病毒,其中每个假定的抑制位点都发生了突变,并分析了对UL127启动子的影响。假定的Fox样位点的突变导致病毒早期UL127启动子的表达显著增加。在HCMV立即早期(IE)US3 TATA框和上游NF-κB反应性增强子(R2)之间插入野生型Fox样位点也显著降低了基因表达,但突变的Fox样位点则没有。野生型Fox样位点抑制含病毒IE增强子的启动子的激活。存在于未感染或感染的允许性细胞核提取物中的细胞蛋白与野生型Fox样位点结合,但不与突变位点结合。文中讨论了生产性感染期间UL127基因转录受抑制的原因。
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