Coordination between nucleotide excision repair and specialized polymerase DnaE2 action enables DNA damage survival in non-replicating bacteria

Translesion synthesis (TLS) is a highly conserved mutagenic DNA lesion tolerance pathway, which employs specialized, low-fidelity DNA polymerases to synthesize across lesions. Current models suggest that activity of these polymerases is predominantly associated with ongoing replication, functioning either at or behind the replication fork. Here we provide evidence for DNA damage-dependent function of a specialized polymerase, DnaE2, in replicationindependent conditions. We develop an assay to follow lesion repair in non-replicating Caulobacter and observe that components of the replication machinery localize on DNA in response to damage. These localizations persist in the absence of DnaE2 or if catalytic activity of this polymerase is mutated. Single-stranded DNA gaps for SSB binding and low-fidelity polymerase-mediated synthesis are generated by nucleotide excision repair (NER), as replisome components fail to localize in the absence of NER. This mechanism of gap-filling facilitates cell cycle restoration when cells are released into replication-permissive conditions. Thus, such cross-talk (between activity of NER and specialized polymerases in subsequent gap-filling) helps preserve genome integrity and enhances survival in a replication-independent manner.

Automated summary

Translesion synthesis (TLS) is a crucial mutagenic DNA lesion tolerance pathway that utilizes specialized low-fidelity DNA polymerases, such as DnaE2, to synthesize across lesions. In replication-independent conditions, DnaE2 plays a DNA damage-dependent role in facilitating lesion repair, contributing to genome integrity. The interplay between nucleotide excision repair (NER) and specialized polymerases in gap-filling mechanisms helps enhance cell survival and maintain genome integrity in a replication-independent manner.