Pan-cancer genomic analysis links 3’UTR DNA methylation with increased gene expression in T cells

Michael H. McGuire; Shelley M. Herbrich; Santosh K. Dasari; Sherry Y. Wu; Ying Wang; Rajesha Rupaimoole; Gabriel Lopez-Berestein; Keith A. Baggerly; Anil K. Sood

doi:10.1016/j.ebiom.2019.04.045

Pan-cancer genomic analysis links 3’UTR DNA methylation with increased gene expression in T cells

Michael H. McGuire, Shelley M. Herbrich, Santosh K. Dasari, Sherry Y. Wu, Ying Wang, Rajesha Rupaimoole, Gabriel Lopez-Berestein, Keith A. Baggerly, Anil K. Sood

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

31 Scopus citations

Abstract

Background: Investigations into the function of non-promoter DNA methylation have yielded new insights into the epigenetic regulation of gene expression. However, integrated genome-wide non-promoter DNA methylation and gene expression analyses across a wide number of tumour types and corresponding normal tissues have not been performed. Methods: To investigate the impact of non-promoter DNA methylation on cancer pathogenesis, we performed a large-scale analysis of gene expression and DNA methylation profiles, finding enrichment in the 3’UTR DNA methylation positively correlated with gene expression. Filtering for genes in which 3’UTR DNA methylation strongly correlated with gene expression yielded a list of genes enriched for functions involving T cell activation. Findings: The important immune checkpoint gene Havcr2 showed a substantial increase in 3’UTR DNA methylation upon T cell activation and subsequent upregulation of gene expression in mice. Furthermore, this increase in Havcr2 gene expression was abrogated by treatment with decitabine. Interpretation: These findings indicate that the 3’UTR is a functionally relevant DNA methylation site. Additionally, we show a potential novel mechanism of HAVCR2 regulation in T cells, providing new insights for modulating immune checkpoint blockade.

Original language	English (US)
Pages (from-to)	127-137
Number of pages	11
Journal	EBioMedicine
Volume	43
DOIs	https://doi.org/10.1016/j.ebiom.2019.04.045
State	Published - May 2019

Keywords

3’UTR
Epigenetics
Immune checkpoint
Methylation

ASJC Scopus subject areas

General Biochemistry, Genetics and Molecular Biology

MD Anderson CCSG core facilities

Advanced Technology Genomics Core
Bioinformatics Shared Resource
Flow Cytometry and Cellular Imaging Facility
Epigenomics Profiling Core Facility

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10.1016/j.ebiom.2019.04.045

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@article{382329ff315c43c2a5b34417591b1b7e,

title = "Pan-cancer genomic analysis links 3{\textquoteright}UTR DNA methylation with increased gene expression in T cells",

abstract = "Background: Investigations into the function of non-promoter DNA methylation have yielded new insights into the epigenetic regulation of gene expression. However, integrated genome-wide non-promoter DNA methylation and gene expression analyses across a wide number of tumour types and corresponding normal tissues have not been performed. Methods: To investigate the impact of non-promoter DNA methylation on cancer pathogenesis, we performed a large-scale analysis of gene expression and DNA methylation profiles, finding enrichment in the 3{\textquoteright}UTR DNA methylation positively correlated with gene expression. Filtering for genes in which 3{\textquoteright}UTR DNA methylation strongly correlated with gene expression yielded a list of genes enriched for functions involving T cell activation. Findings: The important immune checkpoint gene Havcr2 showed a substantial increase in 3{\textquoteright}UTR DNA methylation upon T cell activation and subsequent upregulation of gene expression in mice. Furthermore, this increase in Havcr2 gene expression was abrogated by treatment with decitabine. Interpretation: These findings indicate that the 3{\textquoteright}UTR is a functionally relevant DNA methylation site. Additionally, we show a potential novel mechanism of HAVCR2 regulation in T cells, providing new insights for modulating immune checkpoint blockade.",

keywords = "3{\textquoteright}UTR, Epigenetics, Immune checkpoint, Methylation",

author = "McGuire, {Michael H.} and Herbrich, {Shelley M.} and Dasari, {Santosh K.} and Wu, {Sherry Y.} and Ying Wang and Rajesha Rupaimoole and Gabriel Lopez-Berestein and Baggerly, {Keith A.} and Sood, {Anil K.}",

note = "Funding Information: Portions of the research reported in this publication were supported by the NIH (P30 CA016672, P50 CA217685, P50 CA098258, U01 CA2 13759, and R35 CA209904). Additional portions of this work were also funded by the Blanton-Davis Ovarian Cancer Research Program, American Cancer Society Research Professor Award, and the Frank McGraw Memorial Chair in Cancer Research. SW was supported by CPRIT grant RP101502 and the Foundation for Women's Cancer.We thank Dr. Marcos Estecio and the MD Anderson DNA methylation core for performing the methylation assays. Cells were sorted by the MD Anderson Flow Cytometry and Cellular Imaging Core Facility before being used in this study (this facility is funded by NCI Cancer Center Support Grant P30 CA16672). Publisher Copyright: {\textcopyright} 2019 The Authors",

year = "2019",

month = may,

doi = "10.1016/j.ebiom.2019.04.045",

language = "English (US)",

volume = "43",

pages = "127--137",

journal = "EBioMedicine",

issn = "2352-3964",

publisher = "Elsevier BV",

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TY - JOUR

T1 - Pan-cancer genomic analysis links 3’UTR DNA methylation with increased gene expression in T cells

AU - McGuire, Michael H.

AU - Herbrich, Shelley M.

AU - Dasari, Santosh K.

AU - Wu, Sherry Y.

AU - Wang, Ying

AU - Rupaimoole, Rajesha

AU - Lopez-Berestein, Gabriel

AU - Baggerly, Keith A.

AU - Sood, Anil K.

N1 - Funding Information: Portions of the research reported in this publication were supported by the NIH (P30 CA016672, P50 CA217685, P50 CA098258, U01 CA2 13759, and R35 CA209904). Additional portions of this work were also funded by the Blanton-Davis Ovarian Cancer Research Program, American Cancer Society Research Professor Award, and the Frank McGraw Memorial Chair in Cancer Research. SW was supported by CPRIT grant RP101502 and the Foundation for Women's Cancer.We thank Dr. Marcos Estecio and the MD Anderson DNA methylation core for performing the methylation assays. Cells were sorted by the MD Anderson Flow Cytometry and Cellular Imaging Core Facility before being used in this study (this facility is funded by NCI Cancer Center Support Grant P30 CA16672). Publisher Copyright: © 2019 The Authors

PY - 2019/5

Y1 - 2019/5

N2 - Background: Investigations into the function of non-promoter DNA methylation have yielded new insights into the epigenetic regulation of gene expression. However, integrated genome-wide non-promoter DNA methylation and gene expression analyses across a wide number of tumour types and corresponding normal tissues have not been performed. Methods: To investigate the impact of non-promoter DNA methylation on cancer pathogenesis, we performed a large-scale analysis of gene expression and DNA methylation profiles, finding enrichment in the 3’UTR DNA methylation positively correlated with gene expression. Filtering for genes in which 3’UTR DNA methylation strongly correlated with gene expression yielded a list of genes enriched for functions involving T cell activation. Findings: The important immune checkpoint gene Havcr2 showed a substantial increase in 3’UTR DNA methylation upon T cell activation and subsequent upregulation of gene expression in mice. Furthermore, this increase in Havcr2 gene expression was abrogated by treatment with decitabine. Interpretation: These findings indicate that the 3’UTR is a functionally relevant DNA methylation site. Additionally, we show a potential novel mechanism of HAVCR2 regulation in T cells, providing new insights for modulating immune checkpoint blockade.

AB - Background: Investigations into the function of non-promoter DNA methylation have yielded new insights into the epigenetic regulation of gene expression. However, integrated genome-wide non-promoter DNA methylation and gene expression analyses across a wide number of tumour types and corresponding normal tissues have not been performed. Methods: To investigate the impact of non-promoter DNA methylation on cancer pathogenesis, we performed a large-scale analysis of gene expression and DNA methylation profiles, finding enrichment in the 3’UTR DNA methylation positively correlated with gene expression. Filtering for genes in which 3’UTR DNA methylation strongly correlated with gene expression yielded a list of genes enriched for functions involving T cell activation. Findings: The important immune checkpoint gene Havcr2 showed a substantial increase in 3’UTR DNA methylation upon T cell activation and subsequent upregulation of gene expression in mice. Furthermore, this increase in Havcr2 gene expression was abrogated by treatment with decitabine. Interpretation: These findings indicate that the 3’UTR is a functionally relevant DNA methylation site. Additionally, we show a potential novel mechanism of HAVCR2 regulation in T cells, providing new insights for modulating immune checkpoint blockade.

KW - 3’UTR

KW - Epigenetics

KW - Immune checkpoint

KW - Methylation

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M3 - Article

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AN - SCOPUS:85065041969

SN - 2352-3964

VL - 43

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EP - 137

JO - EBioMedicine

JF - EBioMedicine

ER -

Pan-cancer genomic analysis links 3’UTR DNA methylation with increased gene expression in T cells

Abstract

Keywords

ASJC Scopus subject areas

MD Anderson CCSG core facilities

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