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来自痘苗病毒粒子的早期启动子结合因子。

Early promoter-binding factor from vaccinia virions.

作者信息

Yuen L, Davison A J, Moss B

出版信息

Proc Natl Acad Sci U S A. 1987 Sep;84(17):6069-73. doi: 10.1073/pnas.84.17.6069.

Abstract

A factor, present in transcriptionally active extracts prepared from purified vaccinia virus particles, binds to vaccinia early promoter sequences. The specificity of binding was demonstrated by electrophoretic mobility shift assays using the 5'-terminal segments of two early genes and related and unrelated competitor DNA fragments. DNase I "footprint" analysis indicated that the factor formed a complex with promoter regions of both genes and protected sequences of 10-15 nucleotides centered 21-24 nucleotides upstream of the RNA start sites. The lack of protection of a late regulatory sequence and of an early promoter with transcriptionally inactivating single-nucleotide substitutions suggested that the protein is an early transcription factor. When subjected to glycerol gradient centrifugation, the DNA-binding factor was resolved from RNA polymerase and sedimented as a 7.5S species with an estimated molecular weight of 130,000.

摘要

从纯化的痘苗病毒颗粒制备的转录活性提取物中存在一种因子,它能与痘苗早期启动子序列结合。通过使用两个早期基因的5'末端片段以及相关和不相关的竞争DNA片段进行电泳迁移率变动分析,证明了结合的特异性。DNase I “足迹” 分析表明,该因子与两个基因的启动子区域形成复合物,并保护RNA起始位点上游21 - 24个核苷酸处中心的10 - 15个核苷酸序列。晚期调控序列和具有转录失活单核苷酸取代的早期启动子缺乏保护,这表明该蛋白质是一种早期转录因子。当进行甘油梯度离心时,DNA结合因子与RNA聚合酶分离,并以7.5S的形式沉降,估计分子量为130,000。

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