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着床前发育过程中基因组甲基化模式的维持需要DNA甲基转移酶1的体细胞形式。

Maintenance of genomic methylation patterns during preimplantation development requires the somatic form of DNA methyltransferase 1.

作者信息

Kurihara Yukiko, Kawamura Yumiko, Uchijima Yasunobu, Amamo Tomokazu, Kobayashi Hiroshi, Asano Tomoichiro, Kurihara Hiroki

机构信息

Department of Physiological Chemistry and Metabolism, Graduate School of Medicine, The University of Tokyo, 7-3-1 Hongo, Bunkyo-ku, Tokyo 113-0033, Japan.

出版信息

Dev Biol. 2008 Jan 1;313(1):335-46. doi: 10.1016/j.ydbio.2007.10.033. Epub 2007 Oct 30.

DOI:10.1016/j.ydbio.2007.10.033
PMID:18048024
Abstract

DNA methylation at cytosine residues in CpG dinucleotides is a component of epigenetic marks crucial to mammalian development. In preimplantation stage embryos, a large part of genomic DNA is extensively demethylated, whereas the methylation patterns are faithfully maintained in certain regions. To date, no enzymes responsible for the maintenance of DNA methylation during preimplantation development have been identified except for the oocyte form of DNA (cytosine-5)-methyltransferase 1 (Dnmt1o) at the 8-cell stage. Herein, we demonstrate that the somatic form of Dnmt1 (Dnmt1s) is present in association with chromatin in MII-stage oocytes as well as in the nucleus throughout preimplantation development. At the early one-cell stage, Dnmt1s is asymmetrically localized in the maternal pronuclei. Thereafter, Dnmt1s is recruited to the paternal genome during pronuclear maturation. During the first two cell cycles after fertilization, Dnmt1s is exported from the nucleus in the G2 phase in a CRM1/exportin-dependent manner. Antibody microinjection and small interfering RNA-mediated knock-down decreases methylated CpG dinucleotides in repetitive intracisternal A-type particle (IAP) sequences and the imprinted gene H19. These results indicate that Dnmt1s is responsible for the maintenance methylation of particular genomic regions whose methylation patterns must be faithfully maintained during preimplantation development.

摘要

CpG二核苷酸中胞嘧啶残基的DNA甲基化是对哺乳动物发育至关重要的表观遗传标记的一个组成部分。在植入前阶段的胚胎中,大部分基因组DNA被广泛去甲基化,而甲基化模式在某些区域被忠实地维持。迄今为止,除了8细胞期卵母细胞形式的DNA(胞嘧啶-5)-甲基转移酶1(Dnmt1o)外,尚未发现负责植入前发育过程中DNA甲基化维持的酶。在此,我们证明体细胞形式的Dnmt1(Dnmt1s)在MII期卵母细胞中与染色质相关联,并且在整个植入前发育过程中存在于细胞核中。在单细胞早期阶段,Dnmt1s不对称地定位于母源原核中。此后,Dnmt1s在原核成熟过程中被招募到父源基因组。在受精后的前两个细胞周期中,Dnmt1s在G2期以CRM1/输出蛋白依赖性方式从细胞核中输出。抗体显微注射和小干扰RNA介导的敲低减少了重复性脑内A 型颗粒(IAP)序列和印记基因H19中的甲基化CpG二核苷酸。这些结果表明,Dnmt1s负责特定基因组区域的维持甲基化,其甲基化模式在植入前发育过程中必须被忠实地维持。

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