Department of Biology, Northeastern University, Boston, MA 02115, USA.
Nucleic Acids Res. 2011 Apr;39(8):3156-65. doi: 10.1093/nar/gkq1142. Epub 2010 Dec 20.
DNA repair is required to maintain genome stability in stem cells and early embryos. At critical junctures, oxidative damage to DNA requires the base excision repair (BER) pathway. Since early zebrafish embryos lack the major polymerase in BER, DNA polymerase ß, repair proceeds via replicative polymerases, even though there is ample polb mRNA. Here, we report that Polb protein fails to appear at the appropriate time in development when AP endonuclease 1 (Apex), the upstream protein in BER, is knocked down. Because polb contains a Creb1 binding site, we examined whether knockdown of Apex affects creb1. Apex knockdown results in loss of Creb1 and Creb complex members but not Creb1 phosphorylation. This effect is independent of p53. Although both apex and creb1 mRNA rescue Creb1 and Polb after Apex knockdown, Apex is not a co-activator of creb1 transcription. This observation has broad significance, as similar results occur when Apex is inhibited in B cells from apex(+/-) mice. These results describe a novel regulatory circuit involving Apex, Creb1 and Polb and provide a mechanism for lethality of Apex loss in higher eukaryotes.
DNA 修复对于维持干细胞和早期胚胎中的基因组稳定性至关重要。在关键节点,DNA 的氧化损伤需要碱基切除修复 (BER) 途径。由于早期斑马鱼胚胎缺乏 BER 的主要聚合酶,DNA 聚合酶 β,修复通过复制聚合酶进行,尽管有足够的 polb mRNA。在这里,我们报告说,当 BER 的上游蛋白 AP 内切核酸酶 1 (Apex) 被敲低时,Polb 蛋白在发育的适当时间未能出现。由于 polb 含有 Creb1 结合位点,我们检查了 Apex 敲低是否会影响 creb1。Apex 敲低导致 Creb1 和 Creb 复合物成员的丧失,但不会导致 Creb1 磷酸化。这种效应不依赖于 p53。尽管 Apex 敲低后 apex 和 creb1 mRNA 都能挽救 Creb1 和 Polb,但 Apex 不是 creb1 转录的共激活因子。这一观察结果具有广泛的意义,因为当在 apex(+/-) 小鼠的 B 细胞中抑制 Apex 时,也会出现类似的结果。这些结果描述了一个涉及 Apex、Creb1 和 Polb 的新型调节回路,并为高等真核生物中 Apex 缺失的致死性提供了一种机制。
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