UvrD facilitates DNA repair by pulling RNA polymerase backwards
- PMID: 24402227
- PMCID: PMC4471481
- DOI: 10.1038/nature12928
UvrD facilitates DNA repair by pulling RNA polymerase backwards
Abstract
UvrD helicase is required for nucleotide excision repair, although its role in this process is not well defined. Here we show that Escherichia coli UvrD binds RNA polymerase during transcription elongation and, using its helicase/translocase activity, forces RNA polymerase to slide backward along DNA. By inducing backtracking, UvrD exposes DNA lesions shielded by blocked RNA polymerase, allowing nucleotide excision repair enzymes to gain access to sites of damage. Our results establish UvrD as a bona fide transcription elongation factor that contributes to genomic integrity by resolving conflicts between transcription and DNA repair complexes. Furthermore, we show that the elongation factor NusA cooperates with UvrD in coupling transcription to DNA repair by promoting backtracking and recruiting nucleotide excision repair enzymes to exposed lesions. Because backtracking is a shared feature of all cellular RNA polymerases, we propose that this mechanism enables RNA polymerases to function as global DNA damage scanners in bacteria and eukaryotes.
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Comment in
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Molecular biology: The tug of DNA repair.Nature. 2014 Jan 16;505(7483):298-9. doi: 10.1038/nature12850. Epub 2014 Jan 8. Nature. 2014. PMID: 24402229 No abstract available.
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UvrD helicase: the little engine that could.Cell Cycle. 2014;13(8):1213-5. doi: 10.4161/cc.28382. Epub 2014 Mar 4. Cell Cycle. 2014. PMID: 24621500 Free PMC article. No abstract available.
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