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在体外,两种不同的转录因子与单纯疱疹病毒胸苷激酶启动子结合。

Two distinct transcription factors bind to the HSV thymidine kinase promoter in vitro.

作者信息

Jones K A, Yamamoto K R, Tjian R

出版信息

Cell. 1985 Sep;42(2):559-72. doi: 10.1016/0092-8674(85)90113-8.

Abstract

We have characterized an in vitro transcription system derived from uninfected HeLa cells that accurately initiates RNA synthesis at the herpes virus thymidine kinase (TK) promoter. Analysis of linker-scanning, single-site, and promoter-inversion mutants reveals that the TK upstream elements previously mapped in vivo are accurately recognized in vitro. A protein fraction required for TK transcription in reconstitution experiments was found to contain multiple protein species that bind specifically to the TK promoter. DNAase I footprint experiments with wild-type and mutant promoters reveal that the TK upstream elements contain three distinctive protein binding sites, two of which appear to be recognized by the Sp1 transcription factor and one which interacts with a cellular protein that binds to "CCAAT" sequences. Optimal expression of the thymidine kinase gene appears to require the coordinate interaction of these two types of transcription factors with the three upstream elements of the promoter.

摘要

我们已经对一种源自未感染的HeLa细胞的体外转录系统进行了特性分析,该系统能在疱疹病毒胸苷激酶(TK)启动子处准确起始RNA合成。对连接子扫描、单位点和启动子倒置突变体的分析表明,先前在体内定位的TK上游元件在体外能被准确识别。在重组实验中发现,TK转录所需的一种蛋白质组分含有多种能特异性结合TK启动子的蛋白质。用野生型和突变型启动子进行的DNA酶I足迹实验表明,TK上游元件含有三个独特的蛋白质结合位点,其中两个似乎能被Sp1转录因子识别,另一个则与一种结合“CCAAT”序列的细胞蛋白相互作用。胸苷激酶基因的最佳表达似乎需要这两种转录因子与启动子的三个上游元件协同相互作用。

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