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酵母转录因子IIB的体内突变研究揭示了对基因激活很重要的功能表面。

Mutational studies of yeast transcription factor IIB in vivo reveal a functional surface important for gene activation.

作者信息

Shaw S P, Carson D J, Dorsey M J, Ma J

机构信息

Division of Developmental Biology, Children's Hospital Research Foundation, University of Cincinnati College of Medicine, OH 45229, USA.

出版信息

Proc Natl Acad Sci U S A. 1997 Mar 18;94(6):2427-32. doi: 10.1073/pnas.94.6.2427.

Abstract

Recent experiments in yeast (Saccharomyces cerevisiae) cells have identified a species-specific region of yeast transcription factor IIB (TFIIB) located at residues 144-157. According to the human TFIIB structure, this region is part of a solvent-exposed helix in the first repeat of the carboxyl-terminal core domain. In this report, we systematically analyze four positions in this region (Lys-147, Cys-149, Lys-151, and Glu-152) that together have been shown previously to be important for yeast TFIIB's function in vivo. Our experiments suggest that all of these four positions, and in particular positions 151, 149, and 152, are critical for yeast TFIIB's ability to support cell growth. In addition, we describe an intragenic suppressor screening experiment to identify mutations that reverse, or partially reverse, the temperature-sensitive phenotype of a yeast TFIIB derivative bearing amino acid changes at these four positions to human residues. The suppressor mutations reveal changes at positions 115, 117, and 182 that are located outside the species-specific region of yeast TFIIB, suggesting an extended surface available to interact with other proteins. Finally, we demonstrate that the suppressor mutations restore gene activation in vivo, further supporting the idea that one important function of yeast TFIIB in living cells is to mediate gene activation.

摘要

最近在酵母(酿酒酵母)细胞中进行的实验确定了酵母转录因子IIB(TFIIB)位于第144 - 157位残基的物种特异性区域。根据人类TFIIB的结构,该区域是羧基末端核心结构域第一个重复序列中一个溶剂暴露螺旋的一部分。在本报告中,我们系统地分析了该区域的四个位置(赖氨酸-147、半胱氨酸-149、赖氨酸-151和谷氨酸-152),先前已证明这些位置共同对酵母TFIIB在体内的功能很重要。我们的实验表明,这四个位置全部,尤其是151、149和152位,对于酵母TFIIB支持细胞生长的能力至关重要。此外,我们描述了一项基因内抑制子筛选实验,以鉴定能够逆转或部分逆转在这四个位置将氨基酸替换为人源残基的酵母TFIIB衍生物温度敏感表型的突变。这些抑制子突变揭示了位于酵母TFIIB物种特异性区域之外的115、117和182位的变化,表明存在一个可与其他蛋白质相互作用的扩展表面。最后,我们证明这些抑制子突变在体内恢复了基因激活,进一步支持了酵母TFIIB在活细胞中的一个重要功能是介导基因激活这一观点。

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本文引用的文献

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Mol Cell Biol. 1996 Jul;16(7):3651-7. doi: 10.1128/MCB.16.7.3651.
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