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End-Joining Repair of Double-Strand Breaks in Drosophila melanogaster Is Largely DNA Ligase IV Independent

机译:果蝇双链断裂的末端连接修复在很大程度上与DNA Ligase IV无关。

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摘要

Repair of DNA double-strand breaks can occur by either nonhomologous end joining or homologous recombination. Most nonhomologous end joining requires a specialized ligase, DNA ligase IV (Lig4). In Drosophila melanogaster, double-strand breaks created by excision of a P element are usually repaired by a homologous recombination pathway called synthesis-dependent strand annealing (SDSA). SDSA requires strand invasion mediated by DmRad51, the product of the spn-A gene. In spn-A mutants, repair proceeds through a nonconservative pathway involving the annealing of microhomologies found within the 17-nt overhangs produced by P excision. We report here that end joining of P-element breaks in the absence of DmRad51 does not require Drosophila LIG4. In wild-type flies, SDSA is sometimes incomplete, and repair is finished by an end-joining pathway that also appears to be independent of LIG4. Loss of LIG4 does not increase sensitivity to ionizing radiation in late-stage larvae, but lig4 spn-A double mutants do show heightened sensitivity relative to spn-A single mutants. Together, our results suggest that a LIG4-independent end-joining pathway is responsible for the majority of double-strand break repair in the absence of homologous recombination in flies.
机译:DNA双链断裂的修复可通过非同源末端连接或同源重组进行。大多数非同源末端连接都需要特殊的连接酶,即DNA连接酶IV(Lig4)。在果蝇中,通常通过称为合成依赖链退火(SDSA)的同源重组途径修复由P元素切除产生的双链断裂。 SDSA需要由spn-A基因的产物DmRad51介导的链入侵。在spn-A突变体中,修复通过非保守途径进行,该途径涉及P切除产生的17-nt突出端中发现的微观同源性的退火。我们在这里报告,在没有DmRad51的情况下P元素断裂的末端连接不需要果蝇LIG4。在野生型果蝇中,SDSA有时是不完整的,并且修复过程通过似乎也独立于LIG4的末端连接途径完成。 LIG4的丢失不会增加后期幼虫对电离辐射的敏感性,但是lig4 spn-A双突变体确实显示出比spn-A单突变体更高的敏感性。在一起,我们的结果表明,在果蝇中没有同源重组的情况下,独立于LIG4的末端连接途径是大多数双链断裂修复的原因。

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