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DNA甲基化模式反映了牛胚胎中的表观遗传重编程。

DNA methylation patterns reflect epigenetic reprogramming in bovine embryos.

作者信息

Niemann Heiner, Carnwath Joseph W, Herrmann Doris, Wieczorek Georg, Lemme Erika, Lucas-Hahn Andrea, Olek Sven

机构信息

Institute of Farm Animal Genetics (FLI), Mariensee, Neustadt, Germany.

出版信息

Cell Reprogram. 2010 Feb;12(1):33-42. doi: 10.1089/cell.2009.0063.

DOI:10.1089/cell.2009.0063
PMID:20132011
Abstract

To understand the epigenetic alterations associated with assisted reproduction technology (ART) and the reprogramming of gene expression that follows somatic cell nuclear transfer (SCNT), we screened a panel of 41 amplicons representing 25 developmentally important genes on 15 different chromosomes (a total of 1079 CpG sites). Methylation analysis was performed on DNA from pools of 80 blastocysts representing three classes of embryos. This revealed a subset of amplicons that distinguish between embryos developing in vivo, produced in vitro, or reconstructed by SCNT. Following SCNT, we observed massive epigenetic reprogramming evidenced by reduced levels of methylation in the resultant embryos. Analysis of data from the 28 most informative amplicons (hotspot loci), representing more than 523 individual CpG sites, we discovered subsets of amplicons with methylation patterns that were unique to each class of embryo and may indicate metastable epialleles. Analysis of eight genes with respect to mRNA expression did not reveal a direct correlation with DNA methylation levels. In conclusion, this approach revealed a subset of amplicons that can be used to evaluate blastocyst quality and reprogramming following SCNT, and can also be employed for the localization of the epigenetic control regions within individual genes and for more general studies of stem cell differentiation.

摘要

为了解与辅助生殖技术(ART)相关的表观遗传改变以及体细胞核移植(SCNT)后随之而来的基因表达重编程,我们在15条不同染色体上筛选了一组代表25个对发育重要基因的41个扩增子(总共1079个CpG位点)。对来自代表三类胚胎的80个囊胚池的DNA进行甲基化分析。这揭示了一组扩增子,可区分体内发育、体外产生或通过SCNT重建的胚胎。在SCNT之后,我们观察到大量的表观遗传重编程,表现为所得胚胎中甲基化水平降低。对来自28个信息最丰富的扩增子(热点位点)的数据进行分析,这些扩增子代表了超过523个个体CpG位点,我们发现了具有独特甲基化模式的扩增子子集,每种胚胎类型都有其独特的甲基化模式,这可能表明存在亚稳定的表观等位基因。对八个基因的mRNA表达分析未发现与DNA甲基化水平有直接相关性。总之,这种方法揭示了一组扩增子,可用于评估SCNT后的囊胚质量和重编程,还可用于单个基因内表观遗传控制区域的定位以及更广泛的干细胞分化研究。

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