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小鼠中父本甲基化印记建立的时间。

Timing of establishment of paternal methylation imprints in the mouse.

作者信息

Li Jing-Yu, Lees-Murdock Diane J, Xu Guo-Liang, Walsh Colum P

机构信息

Laboratory for Molecular Biology, Institute of Biochemistry and Cell Biology, Chinese Academy of Sciences, 320 Yueyang Road, Shanghai 200031, China.

出版信息

Genomics. 2004 Dec;84(6):952-60. doi: 10.1016/j.ygeno.2004.08.012.

DOI:10.1016/j.ygeno.2004.08.012
PMID:15533712
Abstract

Imprinted genes are characterized by predominant expression from one parental allele and differential DNA methylation. Few imprinted genes have been found to acquire a methylation mark in the male germ line, however, and only one of these, H19, has been studied in detail. We examined methylation of the Rasgrf1 and Gtl2 differentially methylated regions (DMR) to determine whether methylation is erased in male germ cells at e12.5 and when the paternal allele acquires methylation. We also compared their methylation dynamics with those of H19 and the maternally methylated gene Snrpn. Our results show that methylation is erased on Rasgrf1, H19, and Snrpn at e12.5, but that Gtl2 retains substantial methylation at this stage. Erasure of methylation marks on Gtl2 appears to occur later in female germ cells to give the unmethylated profile seen in mature MII oocytes. In the male germ line, de novo methylation of Rasgrf1, Gtl2, and H19 occurs in parallel between e12.5 and e17.5, but the DMR are not completely methylated until the mature sperm stage, suggesting a methylation dynamic different from that of IAP, L1, and minor satellite sequences, which have been shown to become fully methylated by e17.5 in male germ cells. This study also indicates important differences between different imprinted DMR in timing and extent of methylation in the germ cells.

摘要

印记基因的特征是一个亲本等位基因的优势表达和差异DNA甲基化。然而,很少有印记基因在雄性生殖系中获得甲基化标记,其中只有H19这一个基因得到了详细研究。我们检测了Rasgrf1和Gtl2差异甲基化区域(DMR)的甲基化情况,以确定在胚胎发育12.5天时雄性生殖细胞中的甲基化是否被消除,以及父本等位基因何时获得甲基化。我们还将它们的甲基化动态与H19和母源甲基化基因Snrpn的甲基化动态进行了比较。我们的结果表明,在胚胎发育12.5天时,Rasgrf1、H19和Snrpn上的甲基化被消除,但Gtl2在这个阶段仍保留大量甲基化。Gtl2上甲基化标记的消除似乎在雌性生殖细胞中发生得较晚,从而在成熟的MII期卵母细胞中呈现出未甲基化的状态。在雄性生殖系中,Rasgrf1、Gtl2和H19的从头甲基化在胚胎发育12.5天至17.5天之间同时发生,但直到成熟精子阶段DMR才完全甲基化,这表明其甲基化动态与IAP、L1和小卫星序列不同,后者已被证明在雄性生殖细胞中到胚胎发育17.5天时会完全甲基化。这项研究还表明,不同的印记DMR在生殖细胞甲基化的时间和程度上存在重要差异。

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