Abstract
Elongating DNA polymerases frequently encounter lesions or structures that impede progress and require repair before DNA replication can be completed. Therefore, directing repair factors to a blocked fork, without interfering with normal replication, is important for proper cell function, and it is a process that is not well understood. To study this process, we have employed the chain-terminating nucleoside analog, 3’ azidothymidine (AZT) and the E. coli genetic system, for which replication and repair factors have been well-defined. By using high-expression suppressor screens, we identified yoaA, encoding a putative helicase, and holC, encoding the Chi component of the replication clamp loader, as genes that promoted tolerance to AZT. YoaA is a putative Fe-S helicase in the XPD/RAD3 family for which orthologs can be found in most bacterial genomes; E. coli has a paralog to YoaA, DinG, which possesses 5’ to 3’ helicase activity and an Fe-S cluster essential to its activity. Mutants in yoaA are sensitive to AZT exposure; dinG mutations cause mild sensitivity to AZT and exacerbate the sensitivity of yoaA mutant strains. Suppression of AZT sensitivity by holC or yoaA was mutually codependent and we provide evidence here that YoaA and Chi physically interact. Interactions of Chi with single-strand DNA binding protein (SSB) and with Psi were required to aid AZT tolerance, as was the proofreading 3’ exonuclease, DnaQ. Our studies suggest that repair is coupled to blocked replication through these interactions. We hypothesize that SSB, through Chi, recruits the YoaA helicase to replication gaps and that unwinding of the nascent strand promotes repair and AZT excision. This recruitment prevents the toxicity of helicase activity and aids the handoff of repair with replication factors, ensuring timely repair and resumption of replication.
Highlights
All cells must balance ongoing DNA synthesis with repair reactions that are necessary to overcome problems in replication
Our study identifies a repair protein that is recruited to problem sites by interactions with the replication machinery
These interactions provide a means by which the cell can sense, respond to and repair damage that interferes with the completion of DNA replication
Summary
All cells must balance ongoing DNA synthesis with repair reactions that are necessary to overcome problems in replication. Recruitment of DNA processing enzymes including nucleases, helicases and topoisomerases to a persistent gap, signaled by the presence of single-strand DNA binding protein (SSB), may aid repair [5]. In E. coli, the genetic requirement for RecFOR is diagnostic for the formation of ssDNA gaps in adjoining duplex DNA and is distinct from single-strand DNA caused by resection of DSBs, which require RecBCD for processing and RecA loading (reviewed in [4]). E. coli cells can tolerate a certain level of AZT monophosphate incorporation, which appears to be excised from the 3’ nascent strain by Exonuclease III [6], a 3’ to 5’ exonuclease acting on duplex DNA from a nick or gap [7]. AZT appears to elicit recombination via the RecAFOR pathway and to produce DSBs at some level, which are repaired via the alternative RecABCD recombination pathway [6]
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