AI Article Synopsis

  • DNA methylation at gene promoters is crucial for regulating gene expression, with the insulin promoter being particularly unmethylated in insulin-producing pancreatic β-cells.
  • Recent findings show that both insulin and glucagon gene promoters are demethylated in pancreatic islet cells, regardless of whether they express insulin, glucagon, or somatostatin.
  • This study indicates that the lack of methylation at these promoters supports the flexible identity of islet cell types and could have important implications for diabetes treatment and understanding β-cell health through circulating DNA methylation patterns.

Article Abstract

DNA methylation at promoters is an important determinant of gene expression. Earlier studies suggested that the insulin gene promoter is uniquely unmethylated in insulin-expressing pancreatic β-cells, providing a classic example of this paradigm. Here we show that islet cells expressing insulin, glucagon, or somatostatin share a lack of methylation at the promoters of the insulin and glucagon genes. This is achieved by rapid demethylation of the insulin and glucagon gene promoters during differentiation of Neurogenin3 embryonic endocrine progenitors, regardless of the specific endocrine cell-type chosen. Similar methylation dynamics were observed in transgenic mice containing a human insulin promoter fragment, pointing to the responsible cis element. Whole-methylome comparison of human α- and β-cells revealed generality of the findings: genes active in one cell type and silent in the other tend to share demethylated promoters, while methylation differences between α- and β-cells are concentrated in enhancers. These findings suggest an epigenetic basis for the observed plastic identity of islet cell types, and have implications for β-cell reprogramming in diabetes and diagnosis of β-cell death using methylation patterns of circulating DNA.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC5754795PMC
http://dx.doi.org/10.1073/pnas.1713736114DOI Listing

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