PLoS Genetics (May 2017)

A new role for Rrm3 in repair of replication-born DNA breakage by sister chromatid recombination.

  • Sandra Muñoz-Galván,
  • María García-Rubio,
  • Pedro Ortega,
  • Jose F Ruiz,
  • Sonia Jimeno,
  • Benjamin Pardo,
  • Belén Gómez-González,
  • Andrés Aguilera

DOI
https://doi.org/10.1371/journal.pgen.1006781
Journal volume & issue
Vol. 13, no. 5
p. e1006781

Abstract

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Replication forks stall at different DNA obstacles such as those originated by transcription. Fork stalling can lead to DNA double-strand breaks (DSBs) that will be preferentially repaired by homologous recombination when the sister chromatid is available. The Rrm3 helicase is a replisome component that promotes replication upon fork stalling, accumulates at highly transcribed regions and prevents not only transcription-induced replication fork stalling but also transcription-associated hyper-recombination. This led us to explore the possible role of Rrm3 in the repair of DSBs when originating at the passage of the replication fork. Using a mini-HO system that induces mainly single-stranded DNA breaks, we show that rrm3Δ cells are defective in DSB repair. The defect is clearly seen in sister chromatid recombination, the major repair pathway of replication-born DSBs. Our results indicate that Rrm3 recruitment to replication-born DSBs is crucial for viability, uncovering a new role for Rrm3 in the repair of broken replication forks.