Communication between DNA and nucleotide binding sites facilitates stepping by the RecBCD helicase

Author:

Gaydar Vera1,Zananiri Rani1,Saied Layla1,Dvir Or1,Kaplan Ariel1ORCID,Henn Arnon1ORCID

Affiliation:

1. Faculty of Biology, Technion - Israel Institute of Technology , Haifa  3200003 , Israel

Abstract

Abstract Double-strand DNA breaks are the severest type of genomic damage, requiring rapid response to ensure survival. RecBCD helicase in prokaryotes initiates processive and rapid DNA unzipping, essential for break repair. The energetics of RecBCD during translocation along the DNA track are quantitatively not defined. Specifically, it's essential to understand the mechanism by which RecBCD switches between its binding states to enable its translocation. Here, we determine, by systematic affinity measurements, the degree of coupling between DNA and nucleotide binding to RecBCD. In the presence of ADP, RecBCD binds weakly to DNA that harbors a double overhang mimicking an unwinding intermediate. Consistently, RecBCD binds weakly to ADP in the presence of the same DNA. We did not observe coupling between DNA and nucleotide binding for DNA molecules having only a single overhang, suggesting that RecBCD subunits must both bind DNA to ‘sense’ the nucleotide state. On the contrary, AMPpNp shows weak coupling as RecBCD remains strongly bound to DNA in its presence. Detailed thermodynamic analysis of the RecBCD reaction mechanism suggests an ‘energetic compensation’ between RecB and RecD, which may be essential for rapid unwinding. Our findings provide the basis for a plausible stepping mechanism’ during the processive translocation of RecBCD.

Funder

Israel Science Foundation

Marie Curie Career Integration Award

Publisher

Oxford University Press (OUP)

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