From methylation to myelination: epigenomic and transcriptomic profiling of chronic inactive demyelinated multiple sclerosis lesions

Assia Tiane; Melissa Schepers; Rick A. Reijnders; Lieve van Veggel; Sarah Chenine; Ben Rombaut; Emma Dempster; Catherine Verfaillie; Kobi Wasner; Anne Gruenewald; Jos Prickaerts; Ehsan Pishva; Niels Hellings; Daniel van den Hove; Tim Vanmierlo

doi:10.1007/s00401-023-02596-8

From methylation to myelination: epigenomic and transcriptomic profiling of chronic inactive demyelinated multiple sclerosis lesions

Assia Tiane, Melissa Schepers, Rick A. Reijnders, Lieve van Veggel, Sarah Chenine, Ben Rombaut, Emma Dempster, Catherine Verfaillie, Kobi Wasner, Anne Gruenewald, Jos Prickaerts, Ehsan Pishva, Niels Hellings, Daniel van den Hove, Tim Vanmierlo^*

^*Corresponding author for this work

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

Abstract

In the progressive phase of multiple sclerosis (MS), the hampered differentiation capacity of oligodendrocyte precursor cells (OPCs) eventually results in remyelination failure. We have previously shown that DNA methylation of Id2/Id4 is highly involved in OPC differentiation and remyelination. In this study, we took an unbiased approach by determining genome-wide DNA methylation patterns within chronically demyelinated MS lesions and investigated how certain epigenetic signatures relate to OPC differentiation capacity. We compared genome-wide DNA methylation and transcriptional profiles between chronically demyelinated MS lesions and matched normal-appearing white matter (NAWM), making use of post-mortem brain tissue (n = 9/group). DNA methylation differences that inversely correlated with mRNA expression of their corresponding genes were validated for their cell-type specificity in laser-captured OPCs using pyrosequencing. The CRISPR-dCas9-DNMT3a/TET1 system was used to epigenetically edit human-iPSC-derived oligodendrocytes to assess the effect on cellular differentiation. Our data show hypermethylation of CpGs within genes that cluster in gene ontologies related to myelination and axon ensheathment. Cell type-specific validation indicates a region-dependent hypermethylation of MBP, encoding for myelin basic protein, in OPCs obtained from white matter lesions compared to NAWM-derived OPCs. By altering the DNA methylation state of specific CpGs within the promotor region of MBP, using epigenetic editing, we show that cellular differentiation and myelination can be bidirectionally manipulated using the CRISPR-dCas9-DNMT3a/TET1 system in vitro. Our data indicate that OPCs within chronically demyelinated MS lesions acquire an inhibitory phenotype, which translates into hypermethylation of crucial myelination-related genes. Altering the epigenetic status of MBP can restore the differentiation capacity of OPCs and possibly boost (re)myelination.

Original language	English
Pages (from-to)	283-299
Number of pages	17
Journal	Acta Neuropathologica
Volume	146
Issue number	2
Early online date	1 Jun 2023
DOIs	https://doi.org/10.1007/s00401-023-02596-8
Publication status	Published - Aug 2023

Keywords

Epigenetics
Oligodendrocyte
Progressive MS
Epigenetic editing
BASIC-PROTEIN
DNA METHYLATION
OLIGODENDROCYTES
DIFFERENTIATION
REMYELINATION
PACKAGE
BINDING
CNS

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Cite this

Tiane, A., Schepers, M., Reijnders, R. A., van Veggel, L., Chenine, S., Rombaut, B., Dempster, E., Verfaillie, C., Wasner, K., Gruenewald, A., Prickaerts, J., Pishva, E., Hellings, N., van den Hove, D., & Vanmierlo, T. (2023). From methylation to myelination: epigenomic and transcriptomic profiling of chronic inactive demyelinated multiple sclerosis lesions. Acta Neuropathologica, 146(2), 283-299. https://doi.org/10.1007/s00401-023-02596-8

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title = "From methylation to myelination: epigenomic and transcriptomic profiling of chronic inactive demyelinated multiple sclerosis lesions",

abstract = "In the progressive phase of multiple sclerosis (MS), the hampered differentiation capacity of oligodendrocyte precursor cells (OPCs) eventually results in remyelination failure. We have previously shown that DNA methylation of Id2/Id4 is highly involved in OPC differentiation and remyelination. In this study, we took an unbiased approach by determining genome-wide DNA methylation patterns within chronically demyelinated MS lesions and investigated how certain epigenetic signatures relate to OPC differentiation capacity. We compared genome-wide DNA methylation and transcriptional profiles between chronically demyelinated MS lesions and matched normal-appearing white matter (NAWM), making use of post-mortem brain tissue (n = 9/group). DNA methylation differences that inversely correlated with mRNA expression of their corresponding genes were validated for their cell-type specificity in laser-captured OPCs using pyrosequencing. The CRISPR-dCas9-DNMT3a/TET1 system was used to epigenetically edit human-iPSC-derived oligodendrocytes to assess the effect on cellular differentiation. Our data show hypermethylation of CpGs within genes that cluster in gene ontologies related to myelination and axon ensheathment. Cell type-specific validation indicates a region-dependent hypermethylation of MBP, encoding for myelin basic protein, in OPCs obtained from white matter lesions compared to NAWM-derived OPCs. By altering the DNA methylation state of specific CpGs within the promotor region of MBP, using epigenetic editing, we show that cellular differentiation and myelination can be bidirectionally manipulated using the CRISPR-dCas9-DNMT3a/TET1 system in vitro. Our data indicate that OPCs within chronically demyelinated MS lesions acquire an inhibitory phenotype, which translates into hypermethylation of crucial myelination-related genes. Altering the epigenetic status of MBP can restore the differentiation capacity of OPCs and possibly boost (re)myelination.",

keywords = "Epigenetics, Oligodendrocyte, Progressive MS, Epigenetic editing, BASIC-PROTEIN, DNA METHYLATION, OLIGODENDROCYTES, DIFFERENTIATION, REMYELINATION, PACKAGE, BINDING, CNS",

author = "Assia Tiane and Melissa Schepers and Reijnders, {Rick A.} and {van Veggel}, Lieve and Sarah Chenine and Ben Rombaut and Emma Dempster and Catherine Verfaillie and Kobi Wasner and Anne Gruenewald and Jos Prickaerts and Ehsan Pishva and Niels Hellings and {van den Hove}, Daniel and Tim Vanmierlo",

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Tiane, A, Schepers, M, Reijnders, RA , van Veggel, L , Chenine, S , Rombaut, B, Dempster, E, Verfaillie, C, Wasner, K, Gruenewald, A, Prickaerts, J, Pishva, E, Hellings, N, van den Hove, D & Vanmierlo, T 2023, 'From methylation to myelination: epigenomic and transcriptomic profiling of chronic inactive demyelinated multiple sclerosis lesions', Acta Neuropathologica, vol. 146, no. 2, pp. 283-299. https://doi.org/10.1007/s00401-023-02596-8

TY - JOUR

T1 - From methylation to myelination

T2 - epigenomic and transcriptomic profiling of chronic inactive demyelinated multiple sclerosis lesions

AU - Tiane, Assia

AU - Schepers, Melissa

AU - Reijnders, Rick A.

AU - van Veggel, Lieve

AU - Chenine, Sarah

AU - Rombaut, Ben

AU - Dempster, Emma

AU - Verfaillie, Catherine

AU - Wasner, Kobi

AU - Gruenewald, Anne

AU - Prickaerts, Jos

AU - Pishva, Ehsan

AU - Hellings, Niels

AU - van den Hove, Daniel

AU - Vanmierlo, Tim

PY - 2023/8

Y1 - 2023/8

N2 - In the progressive phase of multiple sclerosis (MS), the hampered differentiation capacity of oligodendrocyte precursor cells (OPCs) eventually results in remyelination failure. We have previously shown that DNA methylation of Id2/Id4 is highly involved in OPC differentiation and remyelination. In this study, we took an unbiased approach by determining genome-wide DNA methylation patterns within chronically demyelinated MS lesions and investigated how certain epigenetic signatures relate to OPC differentiation capacity. We compared genome-wide DNA methylation and transcriptional profiles between chronically demyelinated MS lesions and matched normal-appearing white matter (NAWM), making use of post-mortem brain tissue (n = 9/group). DNA methylation differences that inversely correlated with mRNA expression of their corresponding genes were validated for their cell-type specificity in laser-captured OPCs using pyrosequencing. The CRISPR-dCas9-DNMT3a/TET1 system was used to epigenetically edit human-iPSC-derived oligodendrocytes to assess the effect on cellular differentiation. Our data show hypermethylation of CpGs within genes that cluster in gene ontologies related to myelination and axon ensheathment. Cell type-specific validation indicates a region-dependent hypermethylation of MBP, encoding for myelin basic protein, in OPCs obtained from white matter lesions compared to NAWM-derived OPCs. By altering the DNA methylation state of specific CpGs within the promotor region of MBP, using epigenetic editing, we show that cellular differentiation and myelination can be bidirectionally manipulated using the CRISPR-dCas9-DNMT3a/TET1 system in vitro. Our data indicate that OPCs within chronically demyelinated MS lesions acquire an inhibitory phenotype, which translates into hypermethylation of crucial myelination-related genes. Altering the epigenetic status of MBP can restore the differentiation capacity of OPCs and possibly boost (re)myelination.

AB - In the progressive phase of multiple sclerosis (MS), the hampered differentiation capacity of oligodendrocyte precursor cells (OPCs) eventually results in remyelination failure. We have previously shown that DNA methylation of Id2/Id4 is highly involved in OPC differentiation and remyelination. In this study, we took an unbiased approach by determining genome-wide DNA methylation patterns within chronically demyelinated MS lesions and investigated how certain epigenetic signatures relate to OPC differentiation capacity. We compared genome-wide DNA methylation and transcriptional profiles between chronically demyelinated MS lesions and matched normal-appearing white matter (NAWM), making use of post-mortem brain tissue (n = 9/group). DNA methylation differences that inversely correlated with mRNA expression of their corresponding genes were validated for their cell-type specificity in laser-captured OPCs using pyrosequencing. The CRISPR-dCas9-DNMT3a/TET1 system was used to epigenetically edit human-iPSC-derived oligodendrocytes to assess the effect on cellular differentiation. Our data show hypermethylation of CpGs within genes that cluster in gene ontologies related to myelination and axon ensheathment. Cell type-specific validation indicates a region-dependent hypermethylation of MBP, encoding for myelin basic protein, in OPCs obtained from white matter lesions compared to NAWM-derived OPCs. By altering the DNA methylation state of specific CpGs within the promotor region of MBP, using epigenetic editing, we show that cellular differentiation and myelination can be bidirectionally manipulated using the CRISPR-dCas9-DNMT3a/TET1 system in vitro. Our data indicate that OPCs within chronically demyelinated MS lesions acquire an inhibitory phenotype, which translates into hypermethylation of crucial myelination-related genes. Altering the epigenetic status of MBP can restore the differentiation capacity of OPCs and possibly boost (re)myelination.

KW - Epigenetics

KW - Oligodendrocyte

KW - Progressive MS

KW - Epigenetic editing

KW - BASIC-PROTEIN

KW - DNA METHYLATION

KW - OLIGODENDROCYTES

KW - DIFFERENTIATION

KW - REMYELINATION

KW - PACKAGE

KW - BINDING

KW - CNS

U2 - 10.1007/s00401-023-02596-8

DO - 10.1007/s00401-023-02596-8

M3 - Article

C2 - 37286732

SN - 0001-6322

VL - 146

SP - 283

EP - 299

JO - Acta Neuropathologica

JF - Acta Neuropathologica

IS - 2

ER -