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TATA 结合蛋白启动子结合因子的纯化与特性分析。tbp 基因的一种调控转录因子。

Purification and characterization of TATA-binding protein promoter binding factor. A regulatory transcription factor of the tbp gene.

作者信息

Liu F, Bateman E

机构信息

Department of Microbiology and Molecular Genetics, Markey Center for Molecular Genetics, University of Vermont, Burlington 05405.

出版信息

J Biol Chem. 1994 Jul 15;269(28):18541-8.

PMID:8034602
Abstract

Transcription of the Acanthamoeba tbp gene is stimulated by a cis-acting promoter element that is bound by an activator protein, TATA-binding protein promoter binding factor (TPBF). Here, we report the complete purification of TPBF and describe its transcription activating and DNA-binding properties. TPBF contains two polypeptides with molecular weights of 51,000 and 50,000, whereas the native molecular weight of TPBF suggests it is dimeric or trimeric in solution. Phosphatase treatment of TPBF converts the 51,000 molecular weight species to the 50,000 molecular weight form, demonstrating that TPBF is phosphorylated. Phosphorylation reduces DNA binding by TPBF, as assessed by electrophoretic mobility shift assays after phosphatase treatment. TPBF makes numerous contacts with the bases and phosphate backbone of its DNA recognition element, and the pattern of these contacts suggests that it is a novel type of DNA-binding protein. TPBF can bind to additional, low affinity sites within the TBP gene promoter, suggesting that, in addition to positive activation of tbp gene expression, TPBF could also inhibit transcription by competing for binding sites for other proteins within the TBP promoter.

摘要

棘阿米巴属tbp基因的转录受一个顺式作用启动子元件的刺激,该元件可被一种激活蛋白——TATA结合蛋白启动子结合因子(TPBF)所结合。在此,我们报告了TPBF的完全纯化,并描述了其转录激活和DNA结合特性。TPBF包含两条分子量分别为51,000和50,000的多肽,而TPBF的天然分子量表明它在溶液中是二聚体或三聚体。对TPBF进行磷酸酶处理会将分子量为51,000的蛋白转化为分子量为50,000的形式,这表明TPBF是磷酸化的。如磷酸酶处理后的电泳迁移率变动分析所评估的,磷酸化会降低TPBF与DNA的结合。TPBF与其DNA识别元件的碱基和磷酸骨架有大量接触,这些接触模式表明它是一种新型的DNA结合蛋白。TPBF可以结合到TBP基因启动子内的其他低亲和力位点,这表明,除了对tbp基因表达的正向激活作用外,TPBF还可能通过竞争TBP启动子内其他蛋白的结合位点来抑制转录。

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