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grp (chk1) replication-checkpoint mutations and DNA damage trigger a Chk2-dependent block at the Drosophila midblastula transition

机译:grp(chk1)复制 - 检查点突变和DNa损伤在果蝇中胚轴转换中触发Chk2依赖性阻断

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摘要

The 13 syncytial cleavage divisions that initiate Drosophila embryogenesis are under maternal genetic control. The switch to zygotic regulation of development at the midblastula transition (MBT) follows mitosis 13, when the cleavage divisions terminate, transcription increases and the blastoderm cellularizes. Embryos mutant for grp, which encodes Checkpoint kinase 1 (Chk1), are DNA-replication-checkpoint defective and fail to cellularize, gastrulate or to initiate high-level zygotic transcription at the MBT. The mnk (also known as loki) gene encodes Checkpoint kinase 2 (Chk2), which functions in DNA-damage signal transduction. We show that mnk grp double-mutant embryos are replication-checkpoint defective but cellularize, gastrulate and activate high levels of zygotic gene expression. We also show that grp mutant embryos accumulate DNA double-strand breaks and that DNA-damaging agents induce a mnk-dependent block to cellularization and zygotic gene expression. We conclude that the DNA-replication checkpoint maintains genome integrity during the cleavage divisions, and that checkpoint mutations lead to DNA damage that induces a novel Chk2-dependent block at the MBT.
机译:启动果蝇胚胎发生的13个合胞体分裂分裂受母体遗传控制。当分裂分裂终止,转录增加并且胚盘细胞化时,在中胚层过渡期(MBT)上向合子调控的转变转变遵循有丝分裂13。 grp的胚胎突变体,编码Checkpoint激酶1(Chk1),是DNA复制Checkpoint缺陷,无法在MBT上进行细胞化,胃化或启动高水平的合子转录。 mnk(也称为loki)基因编码Checkpoint激酶2(Chk2),其在DNA损伤信号转导中起作用。我们表明,mnk grp双突变胚胎是复制检查点缺陷,但细胞化,消化和激活高水平的合子基因表达。我们还显示,grp突变体胚胎会积累DNA双链断裂,并且DNA破坏剂会诱导mnk依赖性阻滞细胞化和合子基因的表达。我们得出的结论是,DNA复制检查点在裂解分裂过程中保持了基因组的完整性,并且检查点突变导致DNA损伤,从而在MBT上诱导了一个新的Chk2依赖的阻滞。

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