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孤儿核受体Nurr1与视黄酸X受体之间异源二聚化的要求。

Requirements for heterodimerization between the orphan nuclear receptor Nurr1 and retinoid X receptors.

作者信息

Sacchetti Paola, Dwornik Hélène, Formstecher Pierre, Rachez Christophe, Lefebvre Philippe

机构信息

INSERM Unité 459, Faculté de Medecine Henri Warembourg, 1 Place de Verdun, Lille 59045, France.

出版信息

J Biol Chem. 2002 Sep 20;277(38):35088-96. doi: 10.1074/jbc.M205816200. Epub 2002 Jul 16.

Abstract

The nuclear receptor nurr1 is a transcription factor involved in the development and maintenance of neurons synthesizing the neurotransmitter dopamine. Although the lack of nurr1 expression has dramatic consequences for these cells either in terms of differentiation or survival, the mechanisms by which nurr1 controls gene transcription still remain unclear. In the intent to understand better the modalities of action of this nuclear receptor, we have undertaken a systematic analysis of the transcriptional effects and DNA binding properties of nurr1 as a monomer or when forming dimers with the different isotypes of the retinoic X receptor (RXR). Here, we show that nurr1 acts as a gene activator independently of RXR and through an AF2-independent mechanism. In addition, heterodimerization with RXR is isotype-specific, involves multiple domains in the C-terminal region of nurr1, and requires RXR binding to DNA. RXR(alpha)-nurr1 and RXRgamma-nurr1 heterodimers bind direct repeat response elements and display no specific requirements with respect to half-site spacing. However, the retinoid responsiveness of DNA-bound heterodimers requires the reiteration of at least three nurr1 binding sites, thereby limiting retinoid-induced nurr1 transcriptional activity to specific direct response elements.

摘要

核受体Nurr1是一种转录因子,参与合成神经递质多巴胺的神经元的发育和维持。尽管Nurr1表达的缺失对这些细胞的分化或存活都有显著影响,但其控制基因转录的机制仍不清楚。为了更好地理解这种核受体的作用方式,我们对Nurr1作为单体或与视黄酸X受体(RXR)的不同亚型形成二聚体时的转录效应和DNA结合特性进行了系统分析。在此,我们表明Nurr1作为一种基因激活剂,独立于RXR并通过一种不依赖AF2的机制发挥作用。此外,与RXR的异源二聚化具有亚型特异性,涉及Nurr1 C端区域的多个结构域,并且需要RXR与DNA结合。RXR(α)-Nurr1和RXRγ-Nurr1异源二聚体结合直接重复反应元件,并且对半位点间距没有特定要求。然而,DNA结合的异源二聚体的类视黄醇反应性需要至少三个Nurr1结合位点的重复,从而将类视黄醇诱导的Nurr1转录活性限制在特定的直接反应元件上。

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