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转录因子IID复合体的一个组分对起始元件的直接识别。

Direct recognition of initiator elements by a component of the transcription factor IID complex.

作者信息

Kaufmann J, Smale S T

机构信息

Howard Hughes Medical Institute, University of California, Los Angeles School of Medicine 90024-1662.

出版信息

Genes Dev. 1994 Apr 1;8(7):821-9. doi: 10.1101/gad.8.7.821.

Abstract

A core promoter element called an initiator (Inr) overlaps the transcription start site of numerous mammalian protein-coding genes. In promoters that lack a TATA box, the Inr is functionally analogous to TATA, in that it is capable of directing basal transcription by RNA polymerase II and of determining the precise site of transcription initiation. In promoters that contain a TATA box, the Inr can greatly enhance promoter strength. Mammalian Inr consensus sequences have been defined through functional studies and sequence comparisons of the start site regions of protein-coding genes. Here, we show that, in a DNase I footprinting assay with synthetic promoters, the purified TATA-binding protein complex TFIID specifically contacted the Inr. The TFIID-Inr interaction relies on the precise nucleotides needed for Inr function. Detection of the interaction was dependent either on a TATA box or on Sp1 bound to upstream sites. Furthermore, recombinant TFIIB appeared to influence the TFIID-Inr interaction, whereas TFIIA stabilized the TFIID-TATA interaction. These results demonstrate that distinct components of TFIID interact with the TATA boxes and Inr elements of core promoters for RNA polymerase II.

摘要

一种称为起始子(Inr)的核心启动子元件与众多哺乳动物蛋白质编码基因的转录起始位点重叠。在缺乏TATA框的启动子中,Inr在功能上类似于TATA框,因为它能够指导RNA聚合酶II进行基础转录并确定转录起始的精确位点。在含有TATA框的启动子中,Inr可以极大地增强启动子强度。哺乳动物Inr共有序列已通过功能研究和蛋白质编码基因起始位点区域的序列比较得以确定。在此,我们表明,在使用合成启动子的DNase I足迹分析中,纯化的TATA结合蛋白复合物TFIID特异性地与Inr接触。TFIID与Inr的相互作用依赖于Inr功能所需的精确核苷酸。这种相互作用的检测要么依赖于TATA框,要么依赖于结合在上游位点的Sp1。此外,重组TFIIB似乎会影响TFIID与Inr的相互作用,而TFIIA则稳定TFIID与TATA的相互作用。这些结果表明,TFIID的不同组分与RNA聚合酶II核心启动子的TATA框和Inr元件相互作用。

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