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Unaltered imprinting establishment of key imprinted genes in mouse oocytes after in vitro follicle culture under variable follicle-stimulating hormone exposure.

机译:在可变卵泡刺激激素暴露条件下进行体外卵泡培养后,小鼠卵母细胞中关键印迹基因的不变印迹建立。

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摘要

Imprinted genes are differentially methylated during gametogenesis to allow parental-specific monoallelic expression of genes. During mouse oogenesis, DNA methylation at imprinted genes is established during the transition from primordial to antral follicle stages. Studies in human and mouse suggest aberrant imprinting in oocytes following in vitro maturation and after superovulation with high doses of gonadotrophines. The exact mechanisms leading to aberrant imprinting are unknown. We examined the methylation status of differentially methylated regions of key imprinted genes (by bisulphite sequencing) in mouse metaphase II oocytes, grown in a long-term pre-antral follicle culture system and matured in vitro, in the presence of a physiological (10 IU/L) and a high (100 IU/L) recombinant FSH dose. Our results showed a normal DNA methylation at the studied regulatory sequences of Snrpn, Igf2r and H19, demonstrating that 1) prolonged culture and in vitro maturation do not per se modify the establishment of imprinting in oocytes and 2) supraphysiological FSH doses do not induce aberrant DNA methylation at the studied regulatory sequences in this system.
机译:印迹的基因在配子发生过程中差异甲基化,以允许父母特定的单等位基因表达。在小鼠卵子发生过程中,从原始卵泡到肛门卵泡的过渡过程中,印迹基因的DNA甲基化被建立。在人类和小鼠中的研究表明,在体外成熟后和高剂量促性腺激素超排卵后,卵母细胞会出现异常印迹。导致异常烙印的确切机制尚不清楚。我们检查了小鼠中期II卵母细胞中关键印记基因的差异甲基化区域的甲基化状态(通过亚硫酸氢盐测序),该卵母细胞在长期的前肛门前卵泡培养系统中生长并在生理学存在下(10 IU)在体外成熟/ L)和高剂量(100 IU / L)的重组FSH。我们的结果表明,在研究的S​​nrpn,Igf2r和H19调控序列上存在正常的DNA甲基化,表明1)长时间的培养和体外成熟本身不会改变卵母细胞中印迹的建立,并且2)超生理学FSH剂量不会引起异常在该系统中研究的调节序列处的DNA甲基化。

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