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Sensitive and quantitative method to evaluate DNA methylation of the positive regulatory domains (PRDI, PRDII) and cAMP response element (CRE) in human endothelial nitric oxide synthase promoter

机译:评估人内皮一氧化氮合酶启动子阳性调节结构域(PRDI,PRDII)和营养响应元素(CRE)的DNA甲基化的敏感和定量方法

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摘要

Nitric oxide plays a prominent role in the cardiovascular system and much attention has been devoted in the last years on deciphering the regulation of human endothelial nitric oxide synthase (eNOS) expression. Epigenetic based mechanisms have a key role in the eNOS expression and their pathologic perturbations may have profound effects on the steady state RNA levels in the endothelium. The human eNOS promoter lacks a canonical TATA box and it does not contain a proximal CpG island. A differentially DNA methylated region (DMR) in the native eNOS proximal promoter is involved in gene expression regulation. Here we describe a quantitative, sensitive and cost-effective method that, relying on a novel normalization strategy, allows the quantification of DNA methylation status of the positive regulatory domains (PRDI, PRDII) and cAMP response element (CRE) in human eNOS promoter. This technique will enable to explore the functional relevance of DNA methylation perturbations of eNOS promoter both under pathological and physiological conditions.
机译:一氧化氮在心血管系统中起着突出的作用,在过去几年中致力于解读人内皮一氧化氮合酶(ENOS)表达的调控中的许多关注。基于表观遗传学机制在eNOS表达中具有关键作用,其病理扰动可能对内皮中稳态RNA水平具有深远的影响。人类enos启动子缺乏规范塔塔盒,它不包含一个近端的CPG岛。天然eNOS近端启动子中的差异性DNA甲基化区域(DMR)参与基因表达调节。在这里,我们描述了一种定量,敏感和成本效益的方法,依赖于新颖的归一化策略,允许在人脑启动子中定量阳性调节结构域(PRDI,PRDII)和CAMP反应元素(CRE)的DNA甲基化状态。该技术将能够在病理和生理条件下探讨eNOS启动子DNA甲基化扰动的功能相关性。

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