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基于单细胞限制酶的植入前小鼠胚胎基因组印记区域甲基化分析。

Single Cell Restriction Enzyme-Based Analysis of Methylation at Genomic Imprinted Regions in Preimplantation Mouse Embryos.

作者信息

Ling Ka Yi, Cheow Lih Feng, Quake Stephen R, Burkholder William F, Messerschmidt Daniel M

机构信息

Developmental Epigenetics and Disease Laboratory, Institute of Molecular and Cell Biology, Agency for Science, Technology and Research (A*STAR), Singapore, Singapore.

Microfluidics Systems Biology Laboratory, Institute of Molecular and Cell Biology, Agency for Science, Technology and Research (A*STAR), Singapore, Singapore.

出版信息

Methods Mol Biol. 2017;1605:171-189. doi: 10.1007/978-1-4939-6988-3_12.

Abstract

The methylation of cytosines in DNA is a fundamental epigenetic regulatory mechanism. During preimplantation development, mammalian embryos undergo extensive epigenetic reprogramming, including the global erasure of germ cell-specific DNA methylation marks, to allow for the establishment of the pluripotent state of the epiblast. However, DNA methylation marks at specific regions, such as imprinted gene regions, escape this reprogramming process, as their inheritance from germline to soma is paramount for proper development. To study the dynamics of DNA methylation marks in single blastomeres of mouse preimplantation embryos, we devised a new approach-single cell restriction enzyme analysis of methylation (SCRAM). SCRAM allows for reliable, fast, and high-throughput analysis of DNA methylation states of multiple regions of interest from single cells. In the method described below, SCRAM is specifically used to address loss of DNA methylation at genomic imprints or other highly methylated regions of interest.

摘要

DNA中胞嘧啶的甲基化是一种基本的表观遗传调控机制。在植入前发育过程中,哺乳动物胚胎经历广泛的表观遗传重编程,包括生殖细胞特异性DNA甲基化标记的整体擦除,以允许上胚层多能状态的建立。然而,特定区域(如印记基因区域)的DNA甲基化标记会逃避这种重编程过程,因为它们从种系到体细胞的遗传对于正常发育至关重要。为了研究小鼠植入前胚胎单个卵裂球中DNA甲基化标记的动态变化,我们设计了一种新方法——单细胞甲基化限制酶分析(SCRAM)。SCRAM能够对来自单个细胞的多个感兴趣区域的DNA甲基化状态进行可靠、快速且高通量的分析。在以下所述方法中,SCRAM专门用于解决基因组印记或其他感兴趣的高度甲基化区域的DNA甲基化缺失问题。

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