Peripheral blood DNA methylation signatures and response to tofacitinib in moderate-to-severe ulcerative colitis

Vincent Joustra; Andrew Y F Li Yim; Sara van Gennep; Ishtu Hageman; T de Waard; Evgeni Levin; Peter Lauffer; Wouter J de Jonge; Peter Henneman; Mark Löwenberg; Geert R D'Haens

doi:https://doi.org/10.1093/ecco-jcc/jjad129

Peripheral blood DNA methylation signatures and response to tofacitinib in moderate-to-severe ulcerative colitis

Vincent Joustra, Andrew Y F Li Yim, Sara van Gennep, Ishtu Hageman, T de Waard, Evgeni Levin, Peter Lauffer, Wouter J de Jonge, Peter Henneman, Mark Löwenberg, Geert R D'Haens

Research output: Contribution to journal › Article › Academic › peer-review

Abstract

INTRODUCTION: Predictive biomarkers for treatment efficacy of ulcerative colitis (UC) treatments are lacking. Here, we performed a longitudinal study investigating the association and potential predictive power of genome-wide peripheral blood (PB) DNA methylation signatures and response to tofacitinib treatment in UC.

METHODS: We recruited moderate-to-severe UC patients starting tofacitinib treatment and measured PB DNA methylation profiles at baseline (T1), after 8 weeks (T2), and in a subset (n=8), after a median of 20 weeks (T3) using the Illumina Infinium HumanMethylation EPIC BeadChip. After 8 weeks, we categorized responders (R) from non-responders (NR) based on a centrally read endoscopic response (decrease in endoscopic mayo score ≥1 or UCEIS ≥2) combined with corticosteroid-free clinical- and/or biochemical response. T1 PB samples were used for biomarker identification, while T2 and publicly available intra-class correlation (ICC) data were used for stability analyses. RNA-sequencing was performed to understand the downstream effects of the predictor CpG loci.

RESULTS: In total, 16 R and 15 NR patients with a median disease duration of 7 (4-12) years and overall comparable patient characteristics at baseline were analyzed. We identified a panel of 53 differentially methylated positions (DMPs) associated with response to tofacitinib (AUROC 0.74). Most DMPs (77%) demonstrated both short- and long-term hyper stability (ICC ≥0.90), irrespective of inflammatory status. Gene expression analysis showed lower FGFR2 (pBH=0.011) and LRPAP1 (pBH=0.020), and higher OR2L13 (pBH=0.016) expression at T1 in R compared to NR.

CONCLUSION: Our observations demonstrate the utility of genome-wide PB DNA methylation signatures to predict response to tofacitinib.

Original language	English
Journal	Journal of Crohn's & Colitis
DOIs	https://doi.org/10.1093/ecco-jcc/jjad129
Publication status	E-pub ahead of print - 1 Aug 2023

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https://doi.org/10.1093/ecco-jcc/jjad129

Cite this

Joustra, V., Li Yim, A. Y. F., van Gennep, S., Hageman, I., de Waard, T., Levin, E., Lauffer, P., de Jonge, W. J., Henneman, P., Löwenberg, M., & D'Haens, G. R. (2023). Peripheral blood DNA methylation signatures and response to tofacitinib in moderate-to-severe ulcerative colitis. Journal of Crohn's & Colitis. Advance online publication. https://doi.org/10.1093/ecco-jcc/jjad129

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title = "Peripheral blood DNA methylation signatures and response to tofacitinib in moderate-to-severe ulcerative colitis",

abstract = "INTRODUCTION: Predictive biomarkers for treatment efficacy of ulcerative colitis (UC) treatments are lacking. Here, we performed a longitudinal study investigating the association and potential predictive power of genome-wide peripheral blood (PB) DNA methylation signatures and response to tofacitinib treatment in UC.METHODS: We recruited moderate-to-severe UC patients starting tofacitinib treatment and measured PB DNA methylation profiles at baseline (T1), after 8 weeks (T2), and in a subset (n=8), after a median of 20 weeks (T3) using the Illumina Infinium HumanMethylation EPIC BeadChip. After 8 weeks, we categorized responders (R) from non-responders (NR) based on a centrally read endoscopic response (decrease in endoscopic mayo score ≥1 or UCEIS ≥2) combined with corticosteroid-free clinical- and/or biochemical response. T1 PB samples were used for biomarker identification, while T2 and publicly available intra-class correlation (ICC) data were used for stability analyses. RNA-sequencing was performed to understand the downstream effects of the predictor CpG loci.RESULTS: In total, 16 R and 15 NR patients with a median disease duration of 7 (4-12) years and overall comparable patient characteristics at baseline were analyzed. We identified a panel of 53 differentially methylated positions (DMPs) associated with response to tofacitinib (AUROC 0.74). Most DMPs (77%) demonstrated both short- and long-term hyper stability (ICC ≥0.90), irrespective of inflammatory status. Gene expression analysis showed lower FGFR2 (pBH=0.011) and LRPAP1 (pBH=0.020), and higher OR2L13 (pBH=0.016) expression at T1 in R compared to NR.CONCLUSION: Our observations demonstrate the utility of genome-wide PB DNA methylation signatures to predict response to tofacitinib.",

author = "Vincent Joustra and {Li Yim}, {Andrew Y F} and {van Gennep}, Sara and Ishtu Hageman and {de Waard}, T and Evgeni Levin and Peter Lauffer and {de Jonge}, {Wouter J} and Peter Henneman and Mark L{\"o}wenberg and D'Haens, {Geert R}",

note = "{\textcopyright} The Author(s) 2023. Published by Oxford University Press on behalf of European Crohn{\textquoteright}s and Colitis Organisation.",

year = "2023",

month = aug,

day = "1",

doi = "https://doi.org/10.1093/ecco-jcc/jjad129",

language = "English",

journal = "Journal of Crohn's & Colitis",

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TY - JOUR

T1 - Peripheral blood DNA methylation signatures and response to tofacitinib in moderate-to-severe ulcerative colitis

AU - Joustra, Vincent

AU - Li Yim, Andrew Y F

AU - van Gennep, Sara

AU - Hageman, Ishtu

AU - de Waard, T

AU - Levin, Evgeni

AU - Lauffer, Peter

AU - de Jonge, Wouter J

AU - Henneman, Peter

AU - Löwenberg, Mark

AU - D'Haens, Geert R

PY - 2023/8/1

Y1 - 2023/8/1

N2 - INTRODUCTION: Predictive biomarkers for treatment efficacy of ulcerative colitis (UC) treatments are lacking. Here, we performed a longitudinal study investigating the association and potential predictive power of genome-wide peripheral blood (PB) DNA methylation signatures and response to tofacitinib treatment in UC.METHODS: We recruited moderate-to-severe UC patients starting tofacitinib treatment and measured PB DNA methylation profiles at baseline (T1), after 8 weeks (T2), and in a subset (n=8), after a median of 20 weeks (T3) using the Illumina Infinium HumanMethylation EPIC BeadChip. After 8 weeks, we categorized responders (R) from non-responders (NR) based on a centrally read endoscopic response (decrease in endoscopic mayo score ≥1 or UCEIS ≥2) combined with corticosteroid-free clinical- and/or biochemical response. T1 PB samples were used for biomarker identification, while T2 and publicly available intra-class correlation (ICC) data were used for stability analyses. RNA-sequencing was performed to understand the downstream effects of the predictor CpG loci.RESULTS: In total, 16 R and 15 NR patients with a median disease duration of 7 (4-12) years and overall comparable patient characteristics at baseline were analyzed. We identified a panel of 53 differentially methylated positions (DMPs) associated with response to tofacitinib (AUROC 0.74). Most DMPs (77%) demonstrated both short- and long-term hyper stability (ICC ≥0.90), irrespective of inflammatory status. Gene expression analysis showed lower FGFR2 (pBH=0.011) and LRPAP1 (pBH=0.020), and higher OR2L13 (pBH=0.016) expression at T1 in R compared to NR.CONCLUSION: Our observations demonstrate the utility of genome-wide PB DNA methylation signatures to predict response to tofacitinib.

AB - INTRODUCTION: Predictive biomarkers for treatment efficacy of ulcerative colitis (UC) treatments are lacking. Here, we performed a longitudinal study investigating the association and potential predictive power of genome-wide peripheral blood (PB) DNA methylation signatures and response to tofacitinib treatment in UC.METHODS: We recruited moderate-to-severe UC patients starting tofacitinib treatment and measured PB DNA methylation profiles at baseline (T1), after 8 weeks (T2), and in a subset (n=8), after a median of 20 weeks (T3) using the Illumina Infinium HumanMethylation EPIC BeadChip. After 8 weeks, we categorized responders (R) from non-responders (NR) based on a centrally read endoscopic response (decrease in endoscopic mayo score ≥1 or UCEIS ≥2) combined with corticosteroid-free clinical- and/or biochemical response. T1 PB samples were used for biomarker identification, while T2 and publicly available intra-class correlation (ICC) data were used for stability analyses. RNA-sequencing was performed to understand the downstream effects of the predictor CpG loci.RESULTS: In total, 16 R and 15 NR patients with a median disease duration of 7 (4-12) years and overall comparable patient characteristics at baseline were analyzed. We identified a panel of 53 differentially methylated positions (DMPs) associated with response to tofacitinib (AUROC 0.74). Most DMPs (77%) demonstrated both short- and long-term hyper stability (ICC ≥0.90), irrespective of inflammatory status. Gene expression analysis showed lower FGFR2 (pBH=0.011) and LRPAP1 (pBH=0.020), and higher OR2L13 (pBH=0.016) expression at T1 in R compared to NR.CONCLUSION: Our observations demonstrate the utility of genome-wide PB DNA methylation signatures to predict response to tofacitinib.

U2 - https://doi.org/10.1093/ecco-jcc/jjad129

DO - https://doi.org/10.1093/ecco-jcc/jjad129

M3 - Article

C2 - 37526299

SN - 1873-9946

JO - Journal of Crohn's & Colitis

JF - Journal of Crohn's & Colitis

ER -