The 2B subdomain of Rep helicase links translocation along DNA with protein displacement

Jan-Gert Bruning, Jamieson Anthony Leyland Howard, Kamila Katarzyna Myka, Mark S. Dillingham, Peter McGlynn

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Helicases catalyse DNA and RNA strand separation. Proteins bound to the nucleic
acid must also be displaced in order to unwind DNA. This is exemplified by accessory helicases that clear protein barriers from DNA ahead of advancing replication forks. How helicases catalyse DNA unwinding is increasingly well understood but how protein displacement is achieved is unclear. E. coli Rep accessory replicative helicase lacking one of its four subdomains, 2B, has been shown to be hyperactivated for DNA unwinding in vitro but we show here that Rep∆2B is, in contrast, deficient in displacing proteins from DNA. This defect correlates with an inability to promote replication of protein-bound DNA in vitro and lack of accessory helicase function in vivo. Defective protein displacement is manifested on double-stranded and single-stranded DNA. Thus binding and distortion of duplex DNA by the 2B subdomain ahead of the helicase is not the missing function responsible for this deficiency. These data demonstrate that protein displacement from DNA is not simply achieved by helicase translocation alone. They also imply that helicases may have evolved different specific features to optimise DNA unwinding and protein displacement, both of which are now recognised as key functions in all aspects of nucleic acid metabolism.
Original languageEnglish
JournalNucleic Acids Research
Early online date28 Jul 2018
Publication statusPublished - 28 Sept 2018

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© The Author(s) 2018.

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