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Literature DB >> 31262215

Global modulation in DNA epigenetics during pro-inflammatory macrophage activation.

Nikhil Jain¹, Tamar Shahal^2,3, Tslil Gabrieli³, Noa Gilat³, Dmitry Torchinsky³, Yael Michaeli³, Viola Vogel¹, Yuval Ebenstein³.

Abstract

DNA methylation patterns create distinct gene-expression profiles. These patterns are maintained after cell division, thus enabling the differentiation and maintenance of multiple cell types from the same genome sequence. The advantage of this mechanism for transcriptional control is that chemical-encoding allows to rapidly establish new epigenetic patterns 'on-demand' through enzymatic methylation and demethylation of DNA. Here we show that this feature is associated with the fast response of macrophages during their pro-inflammatory activation. By using a combination of mass spectroscopy and single-molecule imaging to quantify global epigenetic changes in the genomes of primary macrophages, we followed three distinct DNA marks (methylated, hydroxymethylated and unmethylated), involved in establishing new DNA methylation patterns during pro-inflammatory activation. The observed epigenetic modulation together with gene-expression data generated for the involved enzymatic machinery may suggest that de-methylation upon LPS-activation starts with oxidation of methylated CpGs, followed by excision-repair of these oxidized bases and their replacement with unmodified cytosine.

Entities: Chemical

Keywords: DNA methylation; Macrophage activation; RNA sequencing; mass spectroscopy; single-molecule imaging

Mesh：

Year: 2019 PMID： 31262215 PMCID： PMC6791700 DOI： 10.1080/15592294.2019.1638700

Source DB: PubMed Journal: Epigenetics ISSN： 1559-2294 Impact factor: 4.528

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10. Identification of DNMT3B2 as the Predominant Isoform of DNMT3B in Porcine Alveolar Macrophages and Its Involvement in LPS-Stimulated TNF-α Expression.

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