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首页> 外文期刊>Biochimica et Biophysica Acta. Molecular and cell biology of Lipids >Role of DNA methylation and methyl-DNA binding proteins in the repression of 5-lipoxygenase promoter activity.
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Role of DNA methylation and methyl-DNA binding proteins in the repression of 5-lipoxygenase promoter activity.

机译:DNA甲基化和甲基DNA结合蛋白在抑制5-脂氧合酶启动子活性中的作用。

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摘要

Human 5-lipoxygenase (5-LO) is the key enzyme in the formation of inflammatory leukotrienes. 5-LO gene expression is mainly restricted to B cells and cells of myeloid origin. It is known that basal 5-lipoxygenase promoter activity is regulated by DNA methylation. In this study we investigated the impact of the DNA methylation status of the 5-LO promoter on its activity and the role of methyl DNA binding proteins (MBDs) in transcriptional silencing of the 5-LO promoter. Using ChIP assays, we found that the methyl-DNA binding proteins MBD1, MBD2 and MeCP2 bind to the methylated 5-LO core promoter in U937 cells. Knock down of each of the MBDs upregulates 5-LO mRNA expression in U937 cells indicating that these proteins are involved in silencing of the 5-LO gene. In reporter gene assays with in vitro methylated 5-LO promoter constructs, the extent of 5-LO promoter methylation inversely correlated with its activity. Furthermore, we found that MBD1 overexpression repressed 5-LO promoter activity when the CpG sites at the Sp1 binding site close to the transcriptional start site (GC4) were methylated. Gel shift data indicate that recruitment of Sp1 to this binding site is prevented by methylation.
机译:人5-脂氧合酶(5-LO)是炎症白三烯形成中的关键酶。 5-LO基因表达主要限于B细胞和骨髓来源的细胞。已知基础5-脂氧合酶启动子的活性受DNA甲基化的调节。在这项研究中,我们调查了5-LO启动子的DNA甲基化状态对其活性的影响以及甲基DNA结合蛋白(MBD)在5-LO启动子转录沉默中的作用。使用ChIP分析,我们发现甲基DNA结合蛋白MBD1,MBD2和MeCP2与U937细胞中的甲基化5-LO核心启动子结合。敲除每个MBD会上调U937细胞中5-LO mRNA的表达,表明这些蛋白质与5-LO基因的沉默有关。在体外甲基化5-LO启动子构建体的报告基因检测中,5-LO启动子甲基化的程度与其活性成反比。此外,我们发现当Sp1结合位点靠近转录起始位点(GC4)的CpG位点被甲基化时,MBD1过表达会抑制5-LO启动子活性。胶凝位移数据表明,甲基化可防止Sp1募集到该结合位点。

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