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Flp 切口酶切割的复制叉处的双向重组。

Two-ended recombination at a Flp-nickase-broken replication fork.

作者信息

Elango Rajula, Nilavar Namrata, Li Andrew G, Duffey Erin E, Jiang Yuning, Nguyen Daniel, Abakir Abdulkadir, Willis Nicholas A, Houseley Jonathan, Scully Ralph

出版信息

bioRxiv. 2024 Apr 10:2024.04.10.588130. doi: 10.1101/2024.04.10.588130.

Abstract

Collision of a replication fork with a DNA nick is thought to generate a one-ended break, fostering genomic instability. Collision of the opposing converging fork with the nick could, in principle, form a second DNA end, enabling conservative repair by homologous recombination (HR). To study mechanisms of nickase-induced HR, we developed the Flp recombinase "step arrest" nickase in mammalian cells. Flp-nickase-induced HR entails two-ended, BRCA2/RAD51-dependent short tract gene conversion (STGC), BRCA2/RAD51-independent long tract gene conversion, and discoordinated two-ended invasions. HR induced by a replication-independent break and by the Flp-nickase differ in their dependence on . To determine the origin of the second DNA end during Flp-nickase-induced STGC, we blocked the opposing fork using a site-specific Tus/ replication fork barrier. Flp-nickase-induced STGC remained robust and two-ended. Thus, collision of a single replication fork with a Flp-nick can trigger two-ended HR, possibly reflecting replicative bypass of lagging strand nicks. This response may limit genomic instability during replication of a nicked DNA template.

摘要

复制叉与DNA切口的碰撞被认为会产生一个单端断裂,从而加剧基因组不稳定性。原则上,相对的汇聚叉与切口的碰撞可能会形成第二个DNA末端,从而通过同源重组(HR)实现保守修复。为了研究切口酶诱导的HR机制,我们在哺乳动物细胞中开发了Flp重组酶“步进阻滞”切口酶。Flp切口酶诱导的HR需要双端、依赖BRCA2/RAD51的短片段基因转换(STGC)、不依赖BRCA2/RAD51的长片段基因转换以及不协调的双端侵入。由复制非依赖性断裂和Flp切口酶诱导的HR在对……的依赖性上有所不同。为了确定Flp切口酶诱导的STGC过程中第二个DNA末端的来源,我们使用位点特异性Tus/……复制叉屏障阻断相对的叉。Flp切口酶诱导的STGC仍然强劲且是双端的。因此,单个复制叉与Flp切口的碰撞可以触发双端HR,这可能反映了滞后链切口的复制性绕过。这种反应可能会限制有切口的DNA模板复制过程中的基因组不稳定性。

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