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从牛睾丸中纯化和鉴定一种与DNA聚合酶β启动子起始元件结合的转录因子。

Purification and characterization of a DNA polymerase beta promoter initiator element-binding transcription factor from bovine testis.

作者信息

He F, Narayan S, Wilson S H

机构信息

Sealy Center for Molecular Science, University of Texas Medical Branch, Galveston 77555-1068, USA.

出版信息

Biochemistry. 1996 Feb 13;35(6):1775-82. doi: 10.1021/bi9525987.

Abstract

A low-abundance DNA-binding protein for the DNA polymerase beta (beta-pol) promoter initiator element was purified from bovine testis. The transcriptional initiator element (Inr) of the mammalian beta-pol promoters characterized is highly conserved, and the bovine beta-pol promoter Inr has the sequence -11CAGAGGCGGCCATTGTT+6. The purified initiator element-binding protein (Inr-BP) binds with high affinity to an oligonucleotide corresponding to the beta-pol promoter Inr (Kd = 5 pM), and increasing ionic strength decreases stability of the protein-DNA complex. Mutational analysis of the Inr shows that the purified Inr-BP binds with sequence specificity to the sequence CCAT at -2 to +2 of the Inr, but that seven residues on the 5' side and three residues on the 3' side of the CCAT sequence are required also. Using an in vitro transcription assay with HeLa cell nuclear extract, we find that the endogenous Inr-BP is required for transcriptional activity of the beta-pol promoter; addition of purified Inr-BP restores activity to the nuclear extract depleted in Inr-BP by affinity chromatography. These results, based upon the sequence specificity for DNA binding, indicate that Inr-BP is a YY1-like protein and suggest that it is a required transcription factor in beta-pol gene expression.

摘要

从牛睾丸中纯化出一种与DNA聚合酶β(β-pol)启动子起始元件结合的低丰度DNA结合蛋白。已鉴定的哺乳动物β-pol启动子的转录起始元件(Inr)高度保守,牛β-pol启动子Inr的序列为-11CAGAGGCGGCCATTGTT+6。纯化的起始元件结合蛋白(Inr-BP)与对应于β-pol启动子Inr的寡核苷酸具有高亲和力结合(解离常数Kd = 5 pM),增加离子强度会降低蛋白质-DNA复合物的稳定性。对Inr的突变分析表明,纯化的Inr-BP与Inr的-2至+2位的CCAT序列具有序列特异性结合,但CCAT序列5'侧的七个残基和3'侧的三个残基也是必需的。使用HeLa细胞核提取物进行体外转录分析,我们发现内源性Inr-BP是β-pol启动子转录活性所必需的;添加纯化的Inr-BP可使通过亲和层析耗尽Inr-BP的核提取物恢复活性。基于DNA结合的序列特异性,这些结果表明Inr-BP是一种类似YY1的蛋白,并提示它是β-pol基因表达中必需的转录因子。

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