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The haploid male germ cell- and oocyte-specific Mbd3l1 and Mbd3l2 genes are dispensable for early development fertility and zygotic DNA demethylation in the mouse

机译:单倍体雄性生殖细胞和卵母细胞特异性Mbd3l1和Mbd3l2基因对于小鼠的早期发育繁殖力和合子DNA去甲基化是必不可少的

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摘要

Genome-wide erasure of CpG methylation occurs along the paternal pronucleus in fertilized oocytes. This process involves an active, replication-independent enzymatic step, which has remained enigmatic. MBD3L1 and MBD3L2 are two mammalian homologues of the methyl-CpG-binding protein genes MBD2 and MBD3 that arose from recent gene duplication events. Expression of Mbd3l1 occurs specifically in haploid male germ cells. Mbd3l2 expression is restricted to metaphase II oocytes and zygotes making both proteins candidates for the zygotic demethylation process. Neither of these genes was able to promote reactivation of a methylation-silenced reporter gene. We created Mbd3l1 and Mbd3l2 knockout mice, which were viable and fertile. We show that demethylation of the paternal pronucleus in Mbd3l1−/− and Mbd3l2−/− mice is identical to that in wildtype controls. These data suggest that Mbd3l1 and Mbd3l2 are not involved in genome-wide demethylation of paternal genomes in mouse zygotes and are dispensable for normal development.
机译:CpG甲基化的全基因组擦除沿受精卵母细胞的父核发生。这个过程涉及一个活跃的,不依赖复制的酶促步骤,至今仍是一个谜。 MBD3L1和MBD3L2是甲基CpG结合蛋白基因MBD2和MBD3的两个哺乳动物同源物,它们起源于最近的基因复制事件。 Mbd3l1的表达特别发生在单倍体雄性生殖细胞中。 Mbd3l2的表达仅限于中期II卵母细胞和受精卵,使这两种蛋白均成为合子脱甲基化过程的候选蛋白。这些基因均不能促进甲基化沉默的报告基因的再激活。我们创建了Mbd3l1和Mbd3l2敲除小鼠,它们是活的和肥沃的。我们显示,Mbd3l1 -/-和Mbd3l2 -/-小鼠中父本核的去甲基化与野生型对照相同。这些数据表明,Mbd3l1和Mbd3l2不参与小鼠受精卵中父本基因组的全基因组去甲基化,并且对于正常发育是必不可少的。

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