A longitudinal and transancestral analysis of DNA methylation patterns and disease activity in lupus patients
Patrick Coit, … , Kathleen Maksimowicz-McKinnon, Amr H. Sawalha
Patrick Coit, … , Kathleen Maksimowicz-McKinnon, Amr H. Sawalha
Published October 27, 2020
Citation Information: JCI Insight. 2020;5(22):e143654. https://doi.org/10.1172/jci.insight.143654.
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Research Article

A longitudinal and transancestral analysis of DNA methylation patterns and disease activity in lupus patients

Abstract

Epigenetic dysregulation is implicated in the pathogenesis of lupus. We performed a longitudinal analysis to assess changes in DNA methylation in lupus neutrophils over 4 years of follow-up and across disease activity levels using 229 patient samples. We demonstrate that DNA methylation profiles in lupus are partly determined by ancestry-associated genetic variations and are highly stable over time. DNA methylation levels in 2 CpG sites correlated significantly with changes in lupus disease activity. Progressive demethylation in SNX18 was observed with increasing disease activity in African American patients. Importantly, demethylation of a CpG site located within GALNT18 was associated with the development of active lupus nephritis. Differentially methylated genes between African American and European American lupus patients include type I IFN–response genes such as IRF7 and IFI44, and genes related to the NF-κB pathway. TREML4, which plays a vital role in TLR signaling, was hypomethylated in African American patients and demonstrated a strong cis–methylation quantitative trait loci (cis-meQTL) effect among 8855 cis-meQTL associations identified in our study.

Authors

Patrick Coit, Lourdes Ortiz-Fernandez, Emily E. Lewis, W. Joseph McCune, Kathleen Maksimowicz-McKinnon, Amr H. Sawalha

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Figure 1

The relationship between DNA methylation changes, disease activity, and the development of lupus nephritis in a longitudinal cohort of lupus patients.

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The relationship between DNA methylation changes, disease activity, and ...
(A) A Manhattan plot depicting the significance of correlation between methylation levels of CpG sites and disease activity as measured using SLEDAI scores in African American lupus patients (n = 93 samples). The red dots are CpG sites that meet the threshold for significance of FDR-adjusted P < 0.05 (bold line), and the blue dots are CpG sites that meet the suggestive threshold of FDR-adjusted P < 0.10 (dashed line). (B and C) Methylation status of cg26104306 (B) and cg06708913 (C) across SLEDAI scores for African American (n = 93 samples; red dots/line) and European American (n = 136 samples; blue dots/line) lupus patients. (D) Ideogram of chromosome 11 showing the location of 11p15.5 and 11p15.4 cytobands. Cg16204559 (black line) is within the body of GALNT18 located in the 11p15.4 region (green box). Methylation profiles for n = 11 lupus patients (red dots; n = 7 African American and n = 4 European American) at a time point with active nephritis and the nearest preceding or receding time point without nephritis were compared after adjusting for medications, age, and ancestry group using a linear mixed effects model. Cg16204559 (GALNT18) was significantly demethylated (FDR-adjusted P = 0.048) with the occurrence of nephritis. Mean β nephritis was 78.4% (25th percentile, 80.9%; 75th percentile, 82.0%) and mean β nonnephritis was 81.2% (25th percentile, 77.7%; 75th percentile, 79.5%). Whiskers extend to the maximum value within 1.5 times the IQR on either end of the group. Points beyond the whiskers are outliers.