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肝细胞核因子4的DNA结合与转录激活特异性

DNA binding and transcription activation specificity of hepatocyte nuclear factor 4.

作者信息

Fraser J D, Martinez V, Straney R, Briggs M R

机构信息

Ligand Pharmaceuticals Inc., 10255 Science Center Drive, San Diego, CA 92121, USA.

出版信息

Nucleic Acids Res. 1998 Jun 1;26(11):2702-7. doi: 10.1093/nar/26.11.2702.

Abstract

Hepatocyte nuclear factor 4 (HNF-4) is an orphan intracellular receptor that appears to be a key factor in the regulation of energy metabolism. In order to gain greater understanding of the binding and activation requirements of HNF-4, we performed genetic analysis of the apoCIII promoter, a promoter that has previously been shown to be highly sensitive to HNF-4-induced transcription. We identified two elements within the apoCIII promoter that bind HNF-4, either of which are sufficient to confer promoter induction in response to HNF-4. These two elements are both direct repeat-like in nature, but they differ significantly in motif sequence and the repeats are separated by either 1 or 2 nt. Therefore, to better define the DNA sequence recognition requirements of HNF-4, we utilized PCR-based binding site selection. HNF-4 selected for direct repeat-like elements with either 1 or 2 nt between the repeats. Surprisingly, the strongest selection was for a core motif that included the nucleotides between the repeats. Mutation of the nucleotide between the repeats resulted in a 6-fold reduction in affinity, indicating that the interaction between HNF-4 and the intervening nucleotide(s) is critical for high affinity binding.

摘要

肝细胞核因子4(HNF-4)是一种孤儿细胞内受体,似乎是能量代谢调节中的关键因子。为了更深入了解HNF-4的结合和激活要求,我们对载脂蛋白CIII启动子进行了基因分析,该启动子先前已被证明对HNF-4诱导的转录高度敏感。我们在载脂蛋白CIII启动子中鉴定出两个与HNF-4结合的元件,其中任何一个都足以赋予启动子对HNF-4的诱导反应。这两个元件本质上都是类似直接重复的,但它们在基序序列上有显著差异,并且重复序列之间相隔1或2个核苷酸。因此,为了更好地定义HNF-4的DNA序列识别要求,我们利用了基于PCR的结合位点选择。HNF-4选择了重复序列之间间隔1或2个核苷酸的类似直接重复的元件。令人惊讶的是,最强的选择是针对包含重复序列之间核苷酸的核心基序。重复序列之间核苷酸的突变导致亲和力降低6倍,表明HNF-4与中间核苷酸之间的相互作用对于高亲和力结合至关重要。

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