4.3 Article

ESC4/RTT107 and the control of recombination during replication

Journal

DNA REPAIR
Volume 5, Issue 5, Pages 618-628

Publisher

ELSEVIER
DOI: 10.1016/j.dnarep.2006.02.005

Keywords

ESC4; RTT107; DNA damage; DNA recombination; Rad55

Funding

  1. NCI NIH HHS [R01 CA92276, R01 CA092276-03, R01 CA092276] Funding Source: Medline
  2. NIGMS NIH HHS [R01 GM068569-03, R01 GM068569] Funding Source: Medline

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When replication forks stall during DNA synthesis, cells respond by assembling multiprotein complexes to control the various pathways that stabilize the replication machinery repair the replication fork, and facilitate the reinitiation of processive DNA synthesis. Increasing evidence suggests that cells have evolved scaffolding proteins to orchestrate and control the assembly of these repair complexes, typified in mammalian cells by several BRCT-motif containing proteins, such as Brca1, Xrcc1, and 53BP1. In Saccharomyces cerevisiae, Esc4 contains six such BRCT domains and is required for the most efficient response to a variety of agents that damage DNA. We show that Esc4 interacts with several proteins involved in the repair and processing of stalled or collapsed replication forks, including the recombination protein Rad55. However, the function of Esc4 does not appear to be restricted to a Rad55-dependent process, as we observed an increase in sensitivity to the DNA alkylating agent methane methylsulfonate (MMS) in a esc4 Delta rad55 Delta mutant, as well as in double mutants of esc4A and other recombination genes, compared to the corresponding single mutants. In addition, we show that Esc4 forms multiple nuclear foci in response to treatment with MMS. Similar behavior is also observed in the absence of damage when either of the S-phase checkpoint proteins, Tof1 or Mrc1, is deleted. Thus, we propose that Esc4 associates with ssDNA of stalled forks and acts as a scaffolding protein to recruit and/or modulate the function of other proteins required to reinitiate DNA synthesis. (c) 2006 Elsevier B.V. All rights reserved.

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