Literature DB >> 24487959

Sustained active site rigidity during synthesis by human DNA polymerase μ.

Andrea F Moon1, John M Pryor2, Dale A Ramsden2, Thomas A Kunkel3, Katarzyna Bebenek3, Lars C Pedersen1.   

Abstract

DNA polymerase μ (Pol μ) is the only template-dependent human DNA polymerase capable of repairing double-strand DNA breaks (DSBs) with unpaired 3' ends in nonhomologous end joining (NHEJ). To probe this function, we structurally characterized Pol μ's catalytic cycle for single-nucleotide incorporation. These structures indicate that, unlike other template-dependent DNA polymerases, Pol μ shows no large-scale conformational changes in protein subdomains, amino acid side chains or DNA upon dNTP binding or catalysis. Instead, the only major conformational change is seen earlier in the catalytic cycle, when the flexible loop 1 region repositions upon DNA binding. Pol μ variants with changes in loop 1 have altered catalytic properties and are partially defective in NHEJ. The results indicate that specific loop 1 residues contribute to Pol μ's unique ability to catalyze template-dependent NHEJ of DSBs with unpaired 3' ends.

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Year:  2014        PMID: 24487959      PMCID: PMC4164209          DOI: 10.1038/nsmb.2766

Source DB:  PubMed          Journal:  Nat Struct Mol Biol        ISSN: 1545-9985            Impact factor:   15.369


  57 in total

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  34 in total

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Authors:  Andrea F Moon; Rajendrakumar A Gosavi; Thomas A Kunkel; Lars C Pedersen; Katarzyna Bebenek
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2.  Structural evidence for an in trans base selection mechanism involving Loop1 in polymerase μ at an NHEJ double-strand break junction.

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Review 7.  Main steps in DNA double-strand break repair: an introduction to homologous recombination and related processes.

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Review 8.  Interplay between DNA Polymerases and DNA Ligases: Influence on Substrate Channeling and the Fidelity of DNA Ligation.

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Review 9.  Non-homologous DNA end joining and alternative pathways to double-strand break repair.

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