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位于小鼠甲基化中心的串联B1元件为从头DNA甲基化提供了一个靶点。

Tandem B1 elements located in a mouse methylation center provide a target for de novo DNA methylation.

作者信息

Yates P A, Burman R W, Mummaneni P, Krussel S, Turker M S

机构信息

Center for Research on Occupational and Environmental Toxicology, Oregon Health Sciences University, Portland, Oregon 97201, USA.

出版信息

J Biol Chem. 1999 Dec 17;274(51):36357-61. doi: 10.1074/jbc.274.51.36357.

Abstract

A cis-acting methylation center that signals de novo DNA methylation is located upstream of the mouse Aprt gene. In the current study, two approaches were taken to determine if tandem B1 repetitive elements found at the 3' end of the methylation center contribute to the methylation signal. First, bisulfite genomic sequencing demonstrated that CpG sites within the B1 elements were methylated at relative levels of 43% in embryonal stem cells deficient for the maintenance DNA methyltransferase when compared with wild type embryonal stem cells. Second, the ability of the B1 elements to signal de novo methylation upon stable transfection into mouse embryonal carcinoma cells was examined. This approach demonstrated that the B1 elements were methylated de novo to a high level in the embryonal carcinoma cells and that the B1 elements acted synergistically. The results from these experiments provide strong evidence that the tandem B1 repetitive elements provide a significant fraction of the methylation center signal. By extension, they also support the hypothesis that one role for DNA methylation in mammals is to protect the genome from expression and transposition of parasitic elements.

摘要

一个指示从头DNA甲基化的顺式作用甲基化中心位于小鼠Aprt基因的上游。在当前研究中,采用了两种方法来确定在甲基化中心3'端发现的串联B1重复元件是否对甲基化信号有贡献。首先,亚硫酸氢盐基因组测序表明,与野生型胚胎干细胞相比,在维持性DNA甲基转移酶缺陷的胚胎干细胞中,B1元件内的CpG位点甲基化相对水平为43%。其次,检测了B1元件在稳定转染到小鼠胚胎癌细胞后指示从头甲基化的能力。该方法表明,B1元件在胚胎癌细胞中从头甲基化至高水平,且B1元件具有协同作用。这些实验结果提供了有力证据,证明串联B1重复元件提供了很大一部分甲基化中心信号。由此推断,它们也支持了这样一种假说,即哺乳动物中DNA甲基化的一个作用是保护基因组免受寄生元件的表达和转座影响。

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