Figure 7
Figure 7. Dnmt1 affects genome-wide methylation, leading to loss of the Treg phenotype. (A) Genome-wide overview of fold change in scaled log2 ratios and peak scores of methylated genomic DNA from Dnmt1−/− and WT Treg. Heatmap scale optimized for visualization of −2 to +2.5–fold changes (>96.6% of data; range, −5.68 to +9.28). Hypomethylation shown indicated in blue, and hypermethylation is indicated in red. Results pooled from 3 independent experiments and visualized with the Broad Institute’s Integrative Genomics Viewer. (B) Methylation assessment of the IFN-γ enhancer region, as in Figure 5, confirmed greater than 4× increase in demethylation in Dnmt1−/− Treg. (C) Real-time PCR analysis (mean ± SD, n = 4 per group) of the effects of Dnmt1 loss on Treg expression of various cytokines, and signature Treg genes showed increased IFN-γ expression, consistent with enhancer demethylation. (D-E) Selection transcripts with greater than 2× differential expression; microarray data are shown after z-score transformation (n = 3 per group), data shown after z-score transformation. (D) Transcripts identified as differentially methylated in (A). (E) Treg-relevant genes. (F) Functional annotation enrichment of probes with greater than 5 higher raw scores in Dnmt1−/− versus WT Treg (P < .05). Gene ontology (GO), cellular component (CC), biological process (BP), molecular function (MF). Functional Annotation Clustering calculated using DAVID.50 (G) Loss of Dnmt1 disrupted the normal expression of genes associated with adenosine production (real-time PCR, mean ± SD, n = 4 per group).

Dnmt1 affects genome-wide methylation, leading to loss of the Treg phenotype. (A) Genome-wide overview of fold change in scaled log2 ratios and peak scores of methylated genomic DNA from Dnmt1−/− and WT Treg. Heatmap scale optimized for visualization of −2 to +2.5–fold changes (>96.6% of data; range, −5.68 to +9.28). Hypomethylation shown indicated in blue, and hypermethylation is indicated in red. Results pooled from 3 independent experiments and visualized with the Broad Institute’s Integrative Genomics Viewer. (B) Methylation assessment of the IFN-γ enhancer region, as in Figure 5, confirmed greater than 4× increase in demethylation in Dnmt1−/− Treg. (C) Real-time PCR analysis (mean ± SD, n = 4 per group) of the effects of Dnmt1 loss on Treg expression of various cytokines, and signature Treg genes showed increased IFN-γ expression, consistent with enhancer demethylation. (D-E) Selection transcripts with greater than 2× differential expression; microarray data are shown after z-score transformation (n = 3 per group), data shown after z-score transformation. (D) Transcripts identified as differentially methylated in (A). (E) Treg-relevant genes. (F) Functional annotation enrichment of probes with greater than 5 higher raw scores in Dnmt1−/− versus WT Treg (P < .05). Gene ontology (GO), cellular component (CC), biological process (BP), molecular function (MF). Functional Annotation Clustering calculated using DAVID.50  (G) Loss of Dnmt1 disrupted the normal expression of genes associated with adenosine production (real-time PCR, mean ± SD, n = 4 per group).

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