AI Article Synopsis

  • DNA methylation at CpG sites is typically viewed as a stable epigenetic marker, but new research shows its inheritance is more complex than previously thought.
  • High-throughput bisulfite sequencing revealed that while methylation is generally stable at low and high levels, intermediate methylation does not maintain this stability consistently across the genome.
  • The study suggests that changes in intermediate methylation are likely influenced by the enzyme DNMT1 and challenges the conventional understanding of DNA methylation as a reliable marker for epigenetic inheritance, raising questions about its functional significance.

Article Abstract

DNA methylation at the CpG dinucleotide is considered a stable epigenetic mark due to its presumed long-term inheritance through clonal expansion. Here, we perform high-throughput bisulfite sequencing on clonally derived somatic cell lines to quantitatively measure methylation inheritance at the nucleotide level. We find that although DNA methylation is generally faithfully maintained at hypo- and hypermethylated sites, this is not the case at intermediately methylated CpGs. Low fidelity intermediate methylation is interspersed throughout the genome and within genes with no or low transcriptional activity, and is not coordinately maintained between neighbouring sites. We determine that the probabilistic changes that occur at intermediately methylated sites are likely due to DNMT1 rather than DNMT3A/3B activity. The observed lack of clonal inheritance at intermediately methylated sites challenges the current epigenetic inheritance model and has direct implications for both the functional relevance and general interpretability of DNA methylation as a stable epigenetic mark.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC10475082PMC
http://dx.doi.org/10.1038/s41467-023-40845-2DOI Listing

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