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TitleMolecular determinants for dsDNA translocation by the transcription-repair coupling and evolvability factor Mfd.
Journal, issue, pagesNat Commun, Vol. 11, Issue 1, Page 3740, Year 2020
Publish dateJul 27, 2020
AuthorsChristiane Brugger / Cheng Zhang / Margaret M Suhanovsky / David D Kim / Amy N Sinclair / Dmitry Lyumkis / Alexandra M Deaconescu /
PubMed AbstractMfd couples transcription to nucleotide excision repair, and acts on RNA polymerases when elongation is impeded. Depending on impediment severity, this action results in either transcription ...Mfd couples transcription to nucleotide excision repair, and acts on RNA polymerases when elongation is impeded. Depending on impediment severity, this action results in either transcription termination or elongation rescue, which rely on ATP-dependent Mfd translocation on DNA. Due to its role in antibiotic resistance, Mfd is also emerging as a prime target for developing anti-evolution drugs. Here we report the structure of DNA-bound Mfd, which reveals large DNA-induced structural changes that are linked to the active site via ATPase motif VI. These changes relieve autoinhibitory contacts between the N- and C-termini and unmask UvrA recognition determinants. We also demonstrate that translocation relies on a threonine in motif Ic, widely conserved in translocases, and a family-specific histidine near motif IVa, reminiscent of the "arginine clamp" of RNA helicases. Thus, Mfd employs a mode of DNA recognition that at its core is common to ss/ds translocases that act on DNA or RNA.
External linksNat Commun / PubMed:32719356 / PubMed Central
MethodsEM (single particle)
Resolution5.5 Å
Structure data

EMDB-22146, PDB-6xeo:
Structure of Mfd bound to dsDNA
Method: EM (single particle) / Resolution: 5.5 Å

Source
  • Escherichia coli (E. coli)
  • escherichia coli (strain k12) (bacteria)
  • synthetic construct (others)
KeywordsDNA BINDING PROTEIN / Hydrolase/DNA / DNA translocase / transcription-coupled DNA repair / helicase / ATPase / Hydrolase-DNA complex

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