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一种用于人巨细胞病毒立即早期2蛋白(IE2)介导的位点依赖性转录抑制以及IE2与主要立即早期启动子直接结合的体外系统。

An in vitro system for human cytomegalovirus immediate early 2 protein (IE2)-mediated site-dependent repression of transcription and direct binding of IE2 to the major immediate early promoter.

作者信息

Macias M P, Stinski M F

机构信息

Department of Microbiology, College of Medicine, University of Iowa, Iowa City 52242.

出版信息

Proc Natl Acad Sci U S A. 1993 Jan 15;90(2):707-11. doi: 10.1073/pnas.90.2.707.

Abstract

In vivo, negative autoregulation of the strong major immediate early promoter (MIEP) of human cytomegalovirus requires the viral immediate early 2 protein (IE2) and a cis element located from position -13 through position -1 relative to the transcription start site. We have established an in vitro transcription system that reproduces the specificity of IE2-mediated negative autoregulation. The carboxyl-terminal 290-amino acid fragment of IE2 was purified as a bacterial fusion protein. Addition of this chimeric protein to the cell-free system specifically repressed transcription from the MIEP containing the wild-type cis-acting repressor element but not from a mutated template in which the cis element had been replaced by heterologous DNA. Control protein and a mutant IE2 fusion protein containing two specific amino acid substitutions in a putative zinc finger motif did not repress the MIEP in vitro. Using conditions defined by this functional assay, we demonstrated by mobility-shift experiments that IE2 binds directly and specifically to DNA bearing the cis-acting repressor element. In addition, IE2 bound to the MIEP in the in vitro transcription reaction mixture.

摘要

在体内,人巨细胞病毒强主要立即早期启动子(MIEP)的负向自动调节需要病毒立即早期2蛋白(IE2)和一个位于相对于转录起始位点-13至-1位置的顺式元件。我们建立了一个体外转录系统,该系统重现了IE2介导的负向自动调节的特异性。IE2的羧基末端290个氨基酸片段作为细菌融合蛋白被纯化。将这种嵌合蛋白添加到无细胞系统中,可特异性抑制来自含有野生型顺式作用阻遏元件的MIEP的转录,但不能抑制顺式元件已被异源DNA取代的突变模板的转录。对照蛋白和在假定的锌指基序中含有两个特定氨基酸取代的突变IE2融合蛋白在体外不抑制MIEP。利用该功能分析所确定的条件,我们通过迁移率变动实验证明IE2直接且特异性地结合到带有顺式作用阻遏元件的DNA上。此外,IE2在体外转录反应混合物中与MIEP结合。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/e869/45734/8adde9ffca29/pnas01100-0354-a.jpg

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