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酵母和人类TATA结合蛋白的保守与非保守功能

Conserved and nonconserved functions of the yeast and human TATA-binding proteins.

作者信息

Cormack B P, Strubin M, Stargell L A, Struhl K

机构信息

Department of Biological Chemistry and Molecular Pharmacology, Harvard Medical School, Boston, Massachusetts 02115.

出版信息

Genes Dev. 1994 Jun 1;8(11):1335-43. doi: 10.1101/gad.8.11.1335.

DOI:10.1101/gad.8.11.1335
PMID:7926734
Abstract

Although the TATA-binding protein (TBP) is highly conserved throughout the eukaryotic kingdom, human TBP cannot functionally replace yeast TBP for cell viability. To investigate the basis of this species specificity, we examine the in vivo transcriptional activity of human TBP at different classes of yeast promoters. Consistent with previous results, analysis of yeast/human hybrid TBPs indicates that growth defects are not correlated with the ability to promote TATA-dependent polymerase II (Pol II) transcription or to respond to acidic activator proteins. Human TBP partially complements the growth defects of a yeast TBP mutant with altered TATA element-binding specificity, suggesting that it carries out sufficient Pol II function to support viability. However, human TBP does not complement the defects of yeast TBP mutants that are specifically defective in transcription by RNA polymerase III. Three independently isolated derivatives of human TBP that permit yeast cell growth replace arginine 231 with lysine; the corresponding amino acid in yeast TBP (lysine 133) has been implicated in RNA polymerase III transcription. Transcriptional analysis indicates that human TBP functions poorly at promoters recognized by RNA polymerases I and III and at RNA Pol II promoters lacking a conventional TATA element. These observations suggest that species specificity of TBP primarily reflects evolutionarily diverged interactions with TBP-associated factors (TAFs) that are necessary for recruitment to promoters lacking TATA elements.

摘要

尽管TATA结合蛋白(TBP)在整个真核生物界高度保守,但人类TBP在功能上无法替代酵母TBP以维持细胞活力。为了探究这种物种特异性的基础,我们检测了人类TBP在不同类型酵母启动子上的体内转录活性。与先前的结果一致,对酵母/人类杂交TBP的分析表明,生长缺陷与促进TATA依赖的聚合酶II(Pol II)转录或对酸性激活蛋白作出反应的能力无关。人类TBP部分弥补了具有改变的TATA元件结合特异性的酵母TBP突变体的生长缺陷,这表明它执行了足够的Pol II功能来维持细胞活力。然而,人类TBP不能弥补在RNA聚合酶III转录中存在特异性缺陷的酵母TBP突变体的缺陷。三种独立分离的允许酵母细胞生长的人类TBP衍生物将精氨酸231替换为赖氨酸;酵母TBP中的相应氨基酸(赖氨酸133)与RNA聚合酶III转录有关。转录分析表明,人类TBP在RNA聚合酶I和III识别的启动子以及缺乏常规TATA元件的RNA Pol II启动子上功能不佳。这些观察结果表明,TBP的物种特异性主要反映了与TBP相关因子(TAF)在进化上不同的相互作用,这些相互作用对于募集到缺乏TATA元件的启动子是必需的。

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