Xu Ping-Long, Liu Yun-Qing, Shan Shi-Fang, Kong Yu-Ying, Zhou Qing, Li Mei, Ding Jian-Ping, Xie You-Hua, Wang Yuan
State Key Laboratory of Molecular Biology, Institute of Biochemistry and Cell Biology, Shanghai Institutes for Biological Sciences, Chinese Academy of Sciences, Shanghai 200031, China.
Mol Endocrinol. 2004 Aug;18(8):1887-905. doi: 10.1210/me.2003-0334. Epub 2004 May 13.
The liver receptor homolog 1 (LRH-1) belongs to the Fushi tarazu factor 1 nuclear receptor subfamily, and its biological functions are just being unveiled. The molecular mechanism for the transcriptional regulation by LRH-1 is not clear yet. In this report, we use mutagenesis and reporter gene assays to carry out a detailed analysis on the hinge region and the proximal ligand binding domain (LBD) of human (h) LRH-1 that possess important regulatory functions. Our results indicate that helix 1 of the LBD is essential for the activity of hLRH-1 and that the steroid receptor coactivator (SRC)-1 interacts directly with the LBD of hLRH-1 and significantly potentiates the transcriptional activity of hLRH-1. Cotransfection assays demonstrate that overexpressed SRC-1 potentiates hLRH-1 mediated activation of the cholesterol 7-alpha-hydroxylase promoter and increases the transcription of the endogenous cholesterol 7-alpha-hydroxylase in Huh7 cells. The interaction between SRC-1 and hLRH-1 assumes a unique pattern that involves primarily a region containing the glutamine-rich domain of SRC-1, and helix 1 and activation function-2 of hLRH-1 LBD. Mutagenesis and molecular modeling studies indicate that, similar to mouse LRH-1, the coactivator-binding cleft of hLRH-1 LBD is not optimized. An interaction between helix 1 of hLRH-1 LBD and a region containing the glutamine-rich domain of SRC-1 can provide an additional stabilizing force and enhances the recruitment of SRC-1. Similar interaction is observed between hLRH-1 and SRC-2/transcriptional intermediary factor 2 or SRC-3/acetyltransferase. Moreover, transcriptional intermediary factor 2 and acetyltransferase also potentiate the transcriptional activity of hLRH-1, suggesting a functional redundancy among SRC family members. These findings collectively demonstrate an important functional role of helix 1 in cofactor recruitment and reveal a novel molecular mechanism of transcriptional regulation and cofactor recruitment mediated by hLRH-1.
肝脏受体同源物1(LRH-1)属于无翅型基因相关因子1核受体亚家族,其生物学功能刚刚被揭示。LRH-1转录调控的分子机制尚不清楚。在本报告中,我们利用诱变和报告基因分析对具有重要调控功能的人(h)LRH-1的铰链区和近端配体结合结构域(LBD)进行了详细分析。我们的结果表明,LBD的螺旋1对hLRH-1的活性至关重要,类固醇受体共激活因子(SRC)-1直接与hLRH-1的LBD相互作用,并显著增强hLRH-1的转录活性。共转染分析表明,过表达的SRC-1增强了hLRH-1介导的胆固醇7-α-羟化酶启动子的激活,并增加了Huh7细胞中内源性胆固醇7-α-羟化酶的转录。SRC-1与hLRH-1之间的相互作用呈现出一种独特的模式,主要涉及包含SRC-1富含谷氨酰胺结构域的区域,以及hLRH-1 LBD的螺旋1和激活功能-2。诱变和分子建模研究表明,与小鼠LRH-1类似,hLRH-1 LBD的共激活因子结合裂隙未得到优化。hLRH-1 LBD的螺旋1与包含SRC-1富含谷氨酰胺结构域的区域之间的相互作用可以提供额外的稳定力,并增强SRC-1的募集。在hLRH-1与SRC-2/转录中介因子2或SRC-3/乙酰转移酶之间也观察到类似的相互作用。此外,转录中介因子2和乙酰转移酶也增强了hLRH-1的转录活性,表明SRC家族成员之间存在功能冗余。这些发现共同证明了螺旋1在辅因子募集中的重要功能作用,并揭示了hLRH-1介导的转录调控和辅因子募集的新分子机制。
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