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A Novel SP1/SP3 Dependent Intronic Enhancer Governing Transcription of the UCP3 Gene in Brown Adipocytes

机译:一种新型的SP1 / SP3依赖性内含子增强子可控制棕色脂肪细胞中UCP3基因的转录。

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摘要

Uncoupling protein (UCP) 3 is a mitochondrial inner membrane protein implicated in lipid handling and metabolism of reactive oxygen species. Its transcription is mainly regulated by peroxisome proliferator-activated receptors (PPAR), a family of nuclear hormone receptors. Employing bandshift assays, RNA interference and reporter gene assays we examine an intronic region in the UCP3 gene harboring a cis-element essential for expression in brown adipocytes. We demonstrate binding of SP1 and SP3 to this element which is adjacent to a direct repeat 1 element mediating activation of UCP3 expression by PPARγ agonists. Transactivation mediated by these elements is interdependent and indispensable for UCP3 expression. Systematic deletion uncovered a third binding element, a putative NF1 site, in close proximity to the SP1/3 and PPARγ binding elements. Data mining demonstrated binding of MyoD and Myogenin to this third element in C2C12 cells, and, furthermore, revealed recruitment of p300. Taken together, this intronic region is the main enhancer driving UCP3 expression with SP1/3 and PPARγ as the core factors required for expression.
机译:解偶联蛋白(UCP)3是线粒体内膜蛋白,参与脂质的处理和活性氧的代谢。它的转录主要受过氧化物酶体增殖物激活受体(PPAR)(核激素受体家族)调节。使用带移分析,RNA干扰和报告基因分析,我们检查了UCP3基因中的一个内含子区域,该区域具有在棕色脂肪细胞中表达所必需的顺式元件。我们证明SP1和SP3对此元素的绑定,该元素与直接重复1元素介导通过PPARγ激动剂激活UCP3表达的元素相邻。这些元素介导的反式激活是相互依赖的,对于UCP3表达而言是必不可少的。系统性删除发现了第三个结合元件,一个假定的NF1位点,与SP1 / 3和PPARγ结合元件非常接近。数据挖掘证明了MyoD和Myogenin与C2C12细胞中的第三个元素结合,此外,还揭示了p300的募集。总体而言,该内含子区域是驱动UCP3表达的主要增强子,其中SP1 / 3和PPARγ是表达所需的核心因子。

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