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首页> 外文期刊>Molecular and Cellular Biology >Role of negative regulation in promoter specificity of the homologous transcriptional activators Ace2p and Swi5p.
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Role of negative regulation in promoter specificity of the homologous transcriptional activators Ace2p and Swi5p.

机译:负调控在同源转录激活因子Ace2p和Swi5p启动子特异性中的作用。

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摘要

The Ace2p and Swi5p zinc finger proteins have nearly identical DNA-binding domains, yet in vivo they activate transcription of different genes, CTS1 and HO. We now demonstrate that Ace2p and Swi5p recognize sites in the CTS1 and HO promoters with the same affinities, raising the question of how promoter specificity is achieved by these proteins with similar DNA-binding domains. It has been previously shown that Swi5p binds to the HO promoter cooperatively with the Pho2p (Base2p/Grf10p) homeodomain protein, and we now show that Ace2p does not interact with Pho2p. Analysis of CTS1 promoter fragments inserted into a heterologous promoter identify a sequence 90 bp away from the Ace2p binding sites which is required to prevent activation by Swi5p through these binding sites. These results suggest that a regulatory protein bound to the CTS1 promoter is needed to prevent Swi5p from activating CT1S expression. A genetic screen was conducted to identify suppressor mutations which allow CTS1 expression in the absence of the Ace2p activator. The nce3 mutation suppresses the ace2 defect in CTS1 expression only if the strain contains a functional SWI5 gene, suggesting that NCE3 normally functions to prevent Swi5p from activating CTS1. The role of negative regulators such as NCE3, as well as the previously described SIN5 gene, in determining the promoter specificity of homologous activators is discussed.
机译:Ace2p和Swi5p锌指蛋白具有几乎相同的DNA结合结构域,但在体内却激活了不同基因CTS1和HO的转录。我们现在证明,Ace2p和Swi5p以相同的亲和力识别CTS1和HO启动子中的位点,提出了如何通过具有相似的DNA结合结构域的蛋白质实现启动子特异性的问题。以前已经证明Swi5p与Pho2p(Base2p / Grf10p)同源域蛋白协同结合到HO启动子,我们现在证明Ace2p不与Pho2p相互作用。插入异源启动子的CTS1启动子片段的分析确定了一个距离Ace2p结合位点90 bp的序列,这是防止Swi5p通过这些结合位点激活所必需的。这些结果表明,需要与CTS1启动子结合的调节蛋白来防止Swi5p激活CT1S表达。进行了遗传筛选以鉴定抑制突变,该突变允许在没有Ace2p激活剂的情况下表达CTS1。仅当菌株包含功能性SWI5基因时,nce3突变才能抑制CTS1表达中的ace2缺陷,这表明NCE3正常发挥功能来阻止Swi5p激活CTS1。讨论了诸如NCE3等负调节剂以及先前描述的SIN5基因在确定同源激活子启动子特异性中的作用。

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