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On the mechanism of recombination hotspot scanning during double-stranded DNA break resection.


ABSTRACT: Double-stranded DNA break repair by homologous recombination is initiated by resection of free DNA ends to produce a 3'-ssDNA overhang. In bacteria, this reaction is catalyzed by helicase-nuclease complexes such as AddAB in a manner regulated by specific recombination hotspot sequences called Crossover hotspot instigator (Chi). We have used magnetic tweezers to investigate the dynamics of AddAB translocation and hotspot scanning during double-stranded DNA break resection. AddAB was prone to stochastic pausing due to transient recognition of Chi-like sequences, unveiling an antagonistic relationship between DNA translocation and sequence-specific DNA recognition. Pauses at bona fide Chi sequences were longer, were nonexponentially distributed, and resulted in an altered velocity upon restart of translocation downstream of Chi. We propose a model for the recognition of Chi sequences to explain the origin of pausing during failed and successful hotspot recognition.

SUBMITTER: Carrasco C 

PROVIDER: S-EPMC3710824 | biostudies-other | 2013 Jul

REPOSITORIES: biostudies-other

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On the mechanism of recombination hotspot scanning during double-stranded DNA break resection.

Carrasco Carolina C   Gilhooly Neville S NS   Dillingham Mark S MS   Moreno-Herrero Fernando F  

Proceedings of the National Academy of Sciences of the United States of America 20130624 28


Double-stranded DNA break repair by homologous recombination is initiated by resection of free DNA ends to produce a 3'-ssDNA overhang. In bacteria, this reaction is catalyzed by helicase-nuclease complexes such as AddAB in a manner regulated by specific recombination hotspot sequences called Crossover hotspot instigator (Chi). We have used magnetic tweezers to investigate the dynamics of AddAB translocation and hotspot scanning during double-stranded DNA break resection. AddAB was prone to stoc  ...[more]

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