4.3 Review

Active DNA demethylation by DNA repair: Facts and uncertainties

Journal

DNA REPAIR
Volume 44, Issue -, Pages 92-102

Publisher

ELSEVIER SCIENCE BV
DOI: 10.1016/j.dnarep.2016.05.013

Keywords

DNA methylation; Active DNA demethylation; DNA repair; Base excision repair; TET1; TET2; TET3; AID TDG; MBD4; UNG2; NEIL1-3; Gadd45a

Funding

  1. Swiss National Science Foundation [SNF_31003A-156467]

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Pathways that control and modulate DNA methylation patterning in mammalian cells were poorly understood for a long time, although their importance in establishing and maintaining cell type-specific gene expression was well recognized. The discovery of proteins capable of converting 5-methylcytosine (5mC) to putative substrates for DNA repair introduced a novel and exciting conceptual framework for the investigation and ultimate discovery of molecular mechanisms of DNA demethylation. Against the prevailing notion that DNA methylation is a static epigenetic mark, it turned out to be dynamic and distinct mechanisms appear to have evolved to effect global and locus-specific DNA demethylation. There is compelling evidence that DNA repair, in particular base excision repair, contributes significantly to the turnover of 5mC in cells. By actively demethylating DNA, DNA repair supports the developmental establishment as well as the maintenance of DNA methylation landscapes and gene expression patterns. Yet, while the biochemical pathways are relatively well-established and reviewed, the biological context, function and regulation of DNA repair-mediated active DNA demethylation remains uncertain. In this review, we will thus summarize and critically discuss the evidence that associates active DNA demethylation by DNA repair with specific functional contexts including the DNA methylation erasure in the early embryo, the control of pluripotency and cellular differentiation, the maintenance of cell identity, and the nuclear reprogramming. (C) 2016 Elsevier B.V. All rights reserved.

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