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在单纯疱疹病毒1的病毒体介导的α基因诱导的顺式位点结合的宿主蛋白的分化及DNA接触点

Differentiation and DNA contact points of host proteins binding at the cis site for virion-mediated induction of alpha genes of herpes simplex virus 1.

作者信息

Kristie T M, Roizman B

机构信息

Marjorie B. Kovler Viral Oncology Laboratories, University of Chicago, Illinois 60637.

出版信息

J Virol. 1988 Apr;62(4):1145-57. doi: 10.1128/JVI.62.4.1145-1157.1988.

Abstract

Transcriptional trans-activation of the five herpes simplex virus 1 alpha genes by the alpha trans-inducing factor requires a cis-acting site (alpha TIC; with the consensus 5'-GyATGnTAATGArATTCyTTGnGGG-3') located in the promoter-regulatory domains of the alpha genes. In DNA band shift assays with nuclear extracts from either mock-infected or infected cells, the DNA fragments containing an alpha TIC sequence from the alpha 0, alpha 4, and alpha 27 genes formed several cellular protein-DNA complexes designated alpha H1, alpha H2, and alpha H3. The host proteins that formed the alpha H2 and alpha H3 complexes were differentiated from those that formed the alpha H1 complex but not from each other by chromatography and specificity of the DNA-binding sites. The alpha H1 proteins protected the alpha TIC sequence of all three genes from DNase I digestion. Methylation of the purines in the sequence 5'-GyATGnTAAT-3' located at the 5' terminus of the alpha TIC sites precluded the binding of alpha H1. The binding site of the alpha H2-alpha H3 proteins in the alpha 27 gene alpha TIC overlapped, in part, with the alpha H1-binding site. The binding of these proteins was precluded by methylation of the purine residues in the sequence 5'-GCCACGTG-3' located at the 3' terminus of the DNase I footprint. The maximum apparent molecular weight of alpha H1 was 110,000, whereas that of alpha H2-alpha H3 was 64,000. A protein designated alpha H2', resembling alpha H2-alpha H3 with respect to molecular weight and chromatographic properties but differing in sequence specificity, bound to a site adjacent to the alpha H1 site in the fragment carrying an alpha TIC sequence of the alpha 4 gene. alpha H1 and alpha H2-alpha H3 or alpha H2' bound concurrently, notwithstanding the apparent overlap in the DNase I footprints.

摘要

α反式诱导因子对单纯疱疹病毒1型五个α基因的转录反式激活需要一个位于α基因启动子调控区域的顺式作用位点(αTIC;共有序列为5'-GyATGnTAATGArATTCyTTGnGGG-3')。在使用来自 mock 感染或感染细胞的核提取物进行的DNA条带迁移分析中,包含来自α0、α4和α27基因的αTIC序列的DNA片段形成了几种细胞蛋白-DNA复合物,分别命名为αH1、αH2和αH3。通过色谱法和DNA结合位点的特异性,形成αH2和αH3复合物的宿主蛋白与形成αH1复合物的宿主蛋白不同,但αH2和αH3复合物之间没有差异。αH1蛋白保护所有三个基因的αTIC序列不被DNase I消化。位于αTIC位点5'末端的序列5'-GyATGnTAAT-3'中嘌呤的甲基化阻止了αH1的结合。α27基因αTIC中αH2-αH3蛋白的结合位点部分与αH1结合位点重叠。位于DNase I足迹3'末端的序列5'-GCCACGTG-3'中嘌呤残基的甲基化阻止了这些蛋白的结合。αH1的最大表观分子量为110,000,而αH2-αH3的最大表观分子量为64,000。一种名为αH2'的蛋白,在分子量和色谱性质方面与αH2-αH3相似,但序列特异性不同,它与携带α4基因αTIC序列的片段中αH1位点相邻的位点结合。尽管在DNase I足迹中明显重叠,但αH1和αH2-αH3或αH2'同时结合。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/9bac/253122/f33173863104/jvirol00083-0063-a.jpg

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