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鉴定一种核孤儿受体(Ear2)作为肾素基因转录的负调节因子。

Identification of a nuclear orphan receptor (Ear2) as a negative regulator of renin gene transcription.

作者信息

Liu Xuebo, Huang Xiaodong, Sigmund Curt D

机构信息

Department of Internal Medicine, University of Iowa, Iowa City, Iowa 52242, USA.

出版信息

Circ Res. 2003 May 16;92(9):1033-40. doi: 10.1161/01.RES.0000071355.82009.43. Epub 2003 Apr 10.

DOI:10.1161/01.RES.0000071355.82009.43
PMID:12690040
Abstract

A potent transcriptional enhancer was previously identified upstream of the mouse renin gene. Within the enhancer is a TGACCT direct-repeat motif, required for enhancer activity, that is the consensus sequence recognized by members of the thyroid hormone subfamily of steroid hormone receptors. We previously reported that RAR/RXR bind to this sequence and mediate the induction of renin promoter activity by retinoids. However, gel mobility shift assays clearly show that other as yet unidentified factors also bind to this motif. In order to identify some of these TGACCT binding factors, we screened a yeast one-hybrid cDNA library derived from mouse As4.1 cells. One of these encoded the orphan nuclear receptor Ear2. Recombinant Ear2 was purified from Escherichia coli and an antipeptide antisera was generated. EMSA showed that purified recombinant Ear2 specifically binds the TGACCT direct-repeat motif. Transfection assays showed that Ear2 potently decreases both baseline and retinoid-induced mouse renin promoter activity in a dose-dependent, enhancer-dependent, and sequence-specific manner. Mutations in Ear2, which abolish its binding to the TGACCT motif, also abolish transcriptional repression. Ear2 was identified as a nuclear protein in As4.1 cells, is one of the proteins binding to the TGACCT repeat motif, and its overexpression can repress transcription of the endogenous renin gene in As4.1 cells. These data suggest that Ear2 is a negative modulator of renin gene transcription in As4.1 cells, and that the renin enhancer may actually encode a complex positive and negative regulator of transcription.

摘要

先前在小鼠肾素基因上游鉴定出一种强效转录增强子。该增强子内有一个TGACCT直接重复基序,它是增强子活性所必需的,是类固醇激素受体甲状腺激素亚家族成员识别的共有序列。我们先前报道,RAR/RXR结合该序列并介导类视黄醇对肾素启动子活性的诱导。然而,凝胶迁移率变动分析清楚地表明,其他尚未鉴定的因子也结合该基序。为了鉴定其中一些TGACCT结合因子,我们筛选了来自小鼠As4.1细胞的酵母单杂交cDNA文库。其中一个编码孤儿核受体Ear2。从大肠杆菌中纯化重组Ear2,并制备抗肽抗血清。电泳迁移率变动分析表明,纯化的重组Ear2特异性结合TGACCT直接重复基序。转染分析表明,Ear2以剂量依赖性、增强子依赖性和序列特异性方式强烈降低基线和类视黄醇诱导的小鼠肾素启动子活性。Ear2中消除其与TGACCT基序结合的突变也消除转录抑制。Ear2在As4.1细胞中被鉴定为核蛋白,是结合TGACCT重复基序的蛋白质之一,其过表达可抑制As4.1细胞中内源性肾素基因的转录。这些数据表明,Ear2是As4.1细胞中肾素基因转录的负调节因子,并且肾素增强子实际上可能编码一种复杂的转录正负调节因子。

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