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克隆的人TATA结合蛋白的功能结构域及上游激活特性

Functional domains and upstream activation properties of cloned human TATA binding protein.

作者信息

Peterson M G, Tanese N, Pugh B F, Tjian R

机构信息

Howard Hughes Medical Institute, Department of Molecular and Cell Biology, University of California, Berkeley 94720.

出版信息

Science. 1990 Jun 29;248(4963):1625-30. doi: 10.1126/science.2363050.

Abstract

The TATA binding protein, TFIID, plays a central role in the initiation of eukaryotic mRNA synthesis. Here, we present a human cDNA clone for this factor. Comparison of its predicted protein sequence with those from Drosophila and yeast reveals a highly conserved carboxyl-terminal 180 amino acids. By contrast, the amino-terminal region of TFIID has diverged in both sequence and length. A striking feature of the human protein is a stretch of 38 glutamine residues in the NH2-terminal region. Expression of human TFIID in both Escherichia coli and HeLa cells produces a protein that binds specifically to a TATA box and promotes basal transcription; the conserved COOH-terminal portion of the protein is sufficient for both of these activities. Recombinant TFIID forms a stable complex on a TATA box either alone or in combination with either of the general transcription factors, TFIIA or TFIIB. Full-length recombinant TFIID is able to support Sp1 activated transcription in a TFIID-depleted nuclear extract, while a deletion of the NH2-terminal half of the protein is not. These results indicate the importance of the NH2-terminal region for upstream activation functions and suggest that additional factors (co-activators) are required for mediating interactions with specific regulators.

摘要

TATA 结合蛋白(TFIID)在真核生物 mRNA 合成起始过程中发挥核心作用。在此,我们展示了该因子的一个人类 cDNA 克隆。将其预测的蛋白质序列与果蝇和酵母的序列进行比较,发现其羧基末端 180 个氨基酸高度保守。相比之下,TFIID 的氨基末端区域在序列和长度上都有所不同。人类蛋白质的一个显著特征是在氨基末端区域有一段 38 个谷氨酰胺残基的序列。在大肠杆菌和 HeLa 细胞中表达人类 TFIID 均产生一种能特异性结合 TATA 框并促进基础转录的蛋白质;该蛋白质保守的羧基末端部分对于这两种活性而言已足够。重组 TFIID 单独或与通用转录因子 TFIIA 或 TFIIB 结合,均可在 TATA 框上形成稳定复合物。全长重组 TFIID 能够在 TFIID 缺失的核提取物中支持 Sp1 激活的转录,而蛋白质氨基末端一半区域缺失的情况则不能。这些结果表明氨基末端区域对于上游激活功能很重要,并提示介导与特定调节因子相互作用还需要其他因子(共激活因子)。

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