| Literature DB >> 33588693 |
Lauren Y M Middleton1,2, John Dou1, Jonah Fisher3, Jonathan A Heiss4, Vy K Nguyen2,5, Allan C Just4, Jessica Faul3, Erin B Ware3,6, Colter Mitchell3,6, Justin A Colacino2,7,8,9, Kelly M Bakulski1.
Abstract
Saliva is a widely used biological sample, especially in pediatric research, containing a heterogenous mixture of immune and epithelial cells. Associations of exposure or disease with saliva DNA methylation can be influenced by cell-type proportions. Here, we developed a saliva cell-type DNA methylation reference panel to estimate interindividual cell-type heterogeneity in whole saliva studies. Saliva was collected from 22 children (7-16 years) and sorted into immune and epithelial cells, using size exclusion filtration and magnetic bead sorting. DNA methylation was measured using the Illumina MethylationEPIC BeadChip. We assessed cell-type differences in DNA methylation profiles and tested for enriched biological pathways. Immune and epithelial cells differed at 181,577 (22.8%) DNA methylation sites (t-test p < 6.28 × 10-8). Immune cell hypomethylated sites are mapped to genes enriched for immune pathways (p < 3.2 × 10-5). Epithelial cell hypomethylated sites were enriched for cornification (p = 5.2 × 10-4), a key process for hard palette formation. Saliva immune and epithelial cells have distinct DNA methylation profiles which can drive whole-saliva DNA methylation measures. A primary saliva DNA methylation reference panel, easily implemented with an R package, will allow estimates of cell proportions from whole saliva samples and improve epigenetic epidemiology studies by accounting for measurement heterogeneity by cell-type proportions.Entities:
Keywords: DNA methylation; cell type reference; cellular heterogeneity; epigenetics; saliva
Mesh:
Year: 2021 PMID: 33588693 PMCID: PMC8865319 DOI: 10.1080/15592294.2021.1890874
Source DB: PubMed Journal: Epigenetics ISSN: 1559-2294 Impact factor: 4.528