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Tracing Dynamic Changes of DNA Methylation at Single-Cell Resolution

机译:在单细胞分辨率下追踪DNA甲基化的动态变化

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摘要

Mammalian DNA methylation plays an essential role in development. To date, only snapshots of different mouse and human cell types have been generated, providing a static view on DNA methylation. To enable monitoring of methylation status as it changes over time, we establish a reporter of genomic methylation (RGM) that relies on a minimal imprinted gene promoter driving a fluorescent protein. We show that insertion of RGM proximal to promoter-associated CpG islands reports the gain or loss of DNA methylation. We further utilized RGM to report endogenous methylation dynamics of non-coding regulatory elements, such as the pluripotency-specific super enhancers of Sox2 and miR290. Loci-specific DNA methylation changes and their correlation with transcription were visualized during cell-state transition following differentiation of mouse embryonic stem cells and during reprogramming of somatic cells to pluripotency. RGM will allow the investigation of dynamic methylation changes during development and disease at single-cell resolution.
机译:哺乳动物的DNA甲基化在发育中起着至关重要的作用。迄今为止,仅生成了不同小鼠和人类细胞类型的快照,从而提供了DNA甲基化的静态视图。为了能够监测甲基化状态随时间变化的情况,我们建立了一个报告基因组甲基化(RGM)的报告者,该报告者依赖于驱动荧光蛋白的最小印迹基因启动子。我们显示,与启动子相关的CpG岛附近的RGM的插入报告DNA甲基化的获得或损失。我们进一步利用RGM来报告非编码调控元件(例如Sox2和miR290的多能特异性超级增强剂)的内源性甲基化动力学。在小鼠胚胎干细胞分化后的细胞状态转换过程中以及体细胞重编程为多能性过程中,可以观察到基因座特异性DNA甲基化变化及其与转录的相关性。 RGM将允许以单细胞分辨率研究发育和疾病期间动态甲基化的变化。

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