Selective chemical tracking of Dnmt1 catalytic activity in live cells
- PMID: 35245449
- PMCID: PMC8901439
- DOI: 10.1016/j.molcel.2022.02.008
Selective chemical tracking of Dnmt1 catalytic activity in live cells
Abstract
Enzymatic methylation of cytosine to 5-methylcytosine in DNA is a fundamental epigenetic mechanism involved in mammalian development and disease. DNA methylation is brought about by collective action of three AdoMet-dependent DNA methyltransferases, whose catalytic interactions and temporal interplay are poorly understood. We used structure-guided engineering of the Dnmt1 methyltransferase to enable catalytic transfer of azide tags onto DNA from a synthetic cofactor analog, Ado-6-azide, in vitro. We then CRISPR-edited the Dnmt1 locus in mouse embryonic stem cells to install the engineered codon, which, following pulse internalization of the Ado-6-azide cofactor by electroporation, permitted selective azide tagging of Dnmt1-specific genomic targets in cellulo. The deposited covalent tags were exploited as "click" handles for reading adjoining sequences and precise genomic mapping of the methylation sites. The proposed approach, Dnmt-TOP-seq, enables high-resolution temporal tracking of the Dnmt1 catalysis in mammalian cells, paving the way to selective studies of other methylation pathways in eukaryotic systems.
Keywords: 5-methylcytosine; DNA methyltransferase; cofactor selectivity; electroporation of AdoMet analogs; embryonic stem cells; enzyme engineering; epigenetic regulation; in cellulo labeling.
Copyright © 2022 The Author(s). Published by Elsevier Inc. All rights reserved.
Conflict of interest statement
Declaration of interests S.K. is an inventor on patents related to mTAG labeling and TOP-seq mapping.
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Comment in
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Meet the author: Vaidotas Stankevičius, Giedrius Vilkaitis, and Saulius Klimašauskas.Mol Cell. 2022 Mar 3;82(5):879-881. doi: 10.1016/j.molcel.2022.02.019. Mol Cell. 2022. PMID: 35245451
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