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Associations Between Maternal Tobacco Smoke Exposure and the Cord Blood CD4(+) DNA Methylome

Environmental Health Perspectives(2019)

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摘要
BACKGROUND: Maternal tobacco smoke exposure has been associated with altered DNA methylation. However, previous studies largely used methylation arrays, which cover a small fraction of CpGs, and focused on whole cord blood. OBJECTIVES: The current study examined the impact of in utero exposure to maternal tobacco smoke on the cord blood CD4(+) DNA methylome. METHODS: The methylomes of 20 Hispanic white newborns (n = 10 exposed to any maternal tobacco smoke in pregnancy; n = 10 unexposed) from the Maternal and Child Health Study (MACHS) were profiled by whole-genome bisulfite sequencing (median coverage: 6.5 x ). Statistical analyses were conducted using the Regression Analysis of Differential Methylation (RADMeth) program because it performs well on low-coverage data (minimizes false positives and negatives). RESULTS: We found that 10,381 CpGs were differentially methylated by tobacco smoke exposure [neighbor-adjusted p-values that are additionally corrected for multiple testing based on the Benjamini-Hochberg method for controlling the false discovery rate (FDR) (P-FDR ) <0.05]. From these CpGs, RADMeth identified 557 differentially methylated regions (DMRs) that were overrepresented (p <0.05) in important regulatory regions, including enhancers. Of nine DMRs that could be queried in a reduced representation bisulfite sequencing (RRBS) study of adult CD4(+) cells (n = 9 smokers; n =10 nonsmokers), four replicated (p <0.05). Additionally, a CpG in the promoter of SLC7A8 (percent methylation difference: -9.4% comparing exposed to unexposed) replicated (p <0.05) in an EPIC (Illumina) array study of cord blood CD4(+) cells (n = 14 exposed to sustained maternal tobacco smoke; n = 16 unexposed) and in a study of adult CD4(+) cells across two platforms (EPIC: n =9 smokers; n =11 nonsmokers; 450K: n =59 smokers; n =72 nonsmokers). CONCLUSIONS: Maternal tobacco smoke exposure in pregnancy is associated with cord blood CD4(+) DNA methylation in key regulatory regions, including enhancers. While we used a method that performs well on low-coverage data, we cannot exclude the possibility that some results may be false positives. However, we identified a differentially methylated CpG in amino acid transporter SLC7A8 that is highly reproducible, which may be sensitive to cigarette smoke in both cord blood and adult CD4(+) cells.
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DNA Methylation
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