Literature DB >> 11123941

Ensuring productive resolution by the junction-resolving enzyme RuvC: large enhancement of the second-strand cleavage rate.

J M Fogg1, D M Lilley.   

Abstract

RuvC is the principal junction-resolving enzyme of Escherichia coli, cleaving four-way DNA junctions created in homologous recombination. It binds with structural specificity to DNA junctions as a dimer, whereupon each subunit cleaves a phosphodiester bond of diametrically disposed strands. To generate a productive resolution event, these cleavages must be symmetrically located with respect to the point of strand exchange, and in the context of a branch-migrating junction, this requires near-simultaneous cleavage by the two subunits. Using a supercoil-stabilized cruciform as a substrate, we have analyzed the kinetics of strand cleavage. Coordinated bilateral cleavage is not essential in RuvC action, because a heterodimer comprising active and inactive subunits is active in unilateral cleavage. However, in operational terms, fully active RuvC appears to introduce simultaneous cleavages of two strands, because the rate of second-strand cleavage is accelerated by a factor of almost 150 relative to the first. We suggest that relief of strain following the first cleavage could lead to acceleration of subsequent cleavage, and show that DNA junctions rendered more flexible by the presence of strand breaks or bulges are subject to faster cleavage by RuvC. Cleavage of one strand of a junction generated in situ by the action of RuvC can accelerate cleavage at an intrinsically poor site by a factor of 500. Very large rate enhancement of second-strand cleavage by RuvC is likely to be essential to ensure productive resolution of a junction that is being actively branch migrated by the RuvAB machinery.

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Year:  2000        PMID: 11123941     DOI: 10.1021/bi001886m

Source DB:  PubMed          Journal:  Biochemistry        ISSN: 0006-2960            Impact factor:   3.162


  27 in total

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Review 2.  GEN1/Yen1 and the SLX4 complex: Solutions to the problem of Holliday junction resolution.

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3.  Resolution of single and double Holliday junction recombination intermediates by GEN1.

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5.  Resolution of the Holliday junction recombination intermediate by human GEN1 at the single-molecule level.

Authors:  Mohamed A Sobhy; Amer Bralić; Vlad-Stefan Raducanu; Masateru Takahashi; Muhammad Tehseen; Fahad Rashid; Manal S Zaher; Samir M Hamdan
Journal:  Nucleic Acids Res       Date:  2019-02-28       Impact factor: 16.971

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7.  The complex between a four-way DNA junction and T7 endonuclease I.

Authors:  Anne-Cécile Déclais; Jonathan M Fogg; Alasdair D J Freeman; Franck Coste; Jonathan M Hadden; Simon E V Phillips; David M J Lilley
Journal:  EMBO J       Date:  2003-03-17       Impact factor: 11.598

Review 8.  Holliday junction resolvases.

Authors:  Haley D M Wyatt; Stephen C West
Journal:  Cold Spring Harb Perspect Biol       Date:  2014-09-02       Impact factor: 10.005

9.  A monovalent ion in the DNA binding interface of the eukaryotic junction-resolving enzyme GEN1.

Authors:  Yijin Liu; Alasdair Dj Freeman; Anne-Cécile Déclais; David M J Lilley
Journal:  Nucleic Acids Res       Date:  2018-11-16       Impact factor: 16.971

10.  Mechanism of Holliday junction resolution by the human GEN1 protein.

Authors:  Ulrich Rass; Sarah A Compton; Joao Matos; Martin R Singleton; Stephen C Y Ip; Miguel G Blanco; Jack D Griffith; Stephen C West
Journal:  Genes Dev       Date:  2010-07-15       Impact factor: 11.361

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