The ligation of pol β mismatch insertion products governs the formation of promutagenic base excision DNA repair intermediates.

Nucleic Acids Research
Melike Çağlayan

Abstract

DNA ligase I and DNA ligase III/XRCC1 complex catalyze the ultimate ligation step following DNA polymerase (pol) β nucleotide insertion during base excision repair (BER). Pol β Asn279 and Arg283 are the critical active site residues for the differentiation of an incoming nucleotide and a template base and the N-terminal domain of DNA ligase I mediates its interaction with pol β. Here, we show inefficient ligation of pol β insertion products with mismatched or damaged nucleotides, with the exception of a Watson-Crick-like dGTP insertion opposite T, using BER DNA ligases in vitro. Moreover, pol β N279A and R283A mutants deter the ligation of the promutagenic repair intermediates and the presence of N-terminal domain of DNA ligase I in a coupled reaction governs the channeling of the pol β insertion products. Our results demonstrate that the BER DNA ligases are compromised by subtle changes in all 12 possible noncanonical base pairs at the 3'-end of the nicked repair intermediate. These findings contribute to understanding of how the identity of the mismatch affects the substrate channeling of the repair pathway and the mechanism underlying the coordination between pol β and DNA ligase at the final ligation step to maintain the BE...Continue Reading

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Citations

Jun 18, 2020·Frontiers in Immunology·Maria StratigopoulouJeroen E J Guikema

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Methods Mentioned

BETA
gel-filtration
nucleotide insertion
electrophoresis
coimmunoprecipitation
X-ray

Software Mentioned

ImageQuant

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