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In vivo repair of methylation damage in Aag 3-methyladenine DNA glycosylase null mouse cells

机译:Aag 3-甲基腺嘌呤DNA糖基化酶无效小鼠细胞中甲基化损伤的体内修复

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3-Methyladenine (3MeA) DNA glycosylases initiate base excision repair by removing 3MeA. These glycosylases also remove a broad spectrum of spontaneous and environmentally induced base lesions in vitro. Mouse cells lacking the Aag 3MeA DNA glycosylase (also known as the Mpg, APNG or ANPG DNA glycosylase) are susceptible to 3MeA-induced S phase arrest, chromosome aberrations and apoptosis, but it is not known if Aag is solely responsible for repair of 3MeA in vivo. Here we show that in Aag~(-/-) cells, 3MeA lesions disappear from the genome slightly faster than would be expected by spontaneous depurination alone, suggesting that there may be residual repair of 3MeA. However, repair of 3MeA is at least 10 times slower in Aag~(-/-) cells than in Aag~(+/+) cells. Consequently, 24 h after exposure to [~3H]MNU, 30% of the original 3MeA burden is intact in Aag~(-/-) cells, while 3MeA is undetectable in Aag~(+/+) cells. Thus, Aag is the major DNA glycosylase for 3MeA repair. We also investigated the in vivo repair kinetics of another Aag substrate, 7-methylguanine. Surprisingly, 7-methylguanine is removed equally efficiently in Aag~(+/+) and Aag~(-/-) cells, suggesting that another DNA glycosylase acts on lesions previously thought to be repaired by Aag.
机译:3-甲基腺嘌呤(3MeA)DNA糖基化酶通过去除3MeA启动碱基切除修复。这些糖基化酶还可以在体外去除广谱的自发性和环境诱导的基础病变。缺少Aag 3MeA DNA糖基化酶(也称为Mpg,APNG或ANPG DNA糖基化酶)的小鼠细胞易受3MeA诱导的S期停滞,染色体畸变和细胞凋亡的影响,但尚不清楚Aag是否仅负责修复3MeA体内。在这里,我们显示在Aag〜(-/-)细胞中,3MeA损伤从基因组中消失的速度比单独进行自发净化所预期的快,这表明可能存在3MeA的残留修复。然而,在Aag _(-/-)细胞中3MeA的修复比在Aag _(+ / +)细胞中的修复至少慢10倍。因此,在暴露于[〜3H] MNU后24小时,原始的3MeA负担的30%在Aag _(-/-)细胞中是完整的,而3MeA在Aag _(+ / +)细胞中是不可检测的。因此,Aag是修复3MeA的主要DNA糖基化酶。我们还研究了另一种Aag底物7-甲基鸟嘌呤的体内修复动力学。令人惊讶地,在Aag-(+ / +)和Aag-(-/-)细胞中7-甲基鸟嘌呤被同样有效地去除,表明另一种DNA糖基化酶作用于先前认为由Aag修复的损伤。

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