Lead exposure during early human development and DNA methylation of imprinted gene regulatory elements in adulthood

Yue Li; Changchun Xie; Susan K. Murphy; David Skaar; Monica Nye; Adriana C. Vidal; Kim M. Cecil; Kim N. Dietrich; Alvaro Puga; Randy L. Jirtle; Cathrine Hoyo

doi:10.1289/ehp.1408577

Lead exposure during early human development and DNA methylation of imprinted gene regulatory elements in adulthood

Yue Li
, Changchun Xie
, Susan K. Murphy
, David Skaar
, Monica Nye
, Adriana C. Vidal
, Kim M. Cecil
, Kim N. Dietrich
, Alvaro Puga
, Randy L. Jirtle
, Cathrine Hoyo

Duke University
University of Cincinnati
North Carolina State University
University of North Carolina at Chapel Hill
University of Wisconsin-Madison

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

59 Citations (Scopus)

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Abstract

Background: Lead exposure during early development causes neurodevelopmental disorders by unknown mechanisms. Epidemiologic studies have focused recently on determining associations between lead exposure and global DNA methylation; however, such approaches preclude the identification of loci that may alter human disease risk. oBjectives: The objective of this study was to determine whether maternal, postnatal, and early childhood lead exposure can alter the differentially methylated regions (DMRs) that control the monoallelic expression of imprinted genes involved in metabolism, growth, and development. Methods: Questionnaire data and serial blood lead levels were obtained from 105 participants (64 females, 41 males) of the Cincinnati Lead Study from birth to 78 months. When participants were adults, we used Sequenom EpiTYPER assays to test peripheral blood DNA to quantify CpG methylation in peripheral blood leukocytes at DMRs of 22 human imprinted genes. Statistical analyses were conducted using linear regression. results: Mean blood lead concentration from birth to 78 months was associated with a significant decrease in PEG3 DMR methylation (β = –0.0014; 95% CI: –0.0023, –0.0005, p = 0.002), stronger in males (β = –0.0024; 95% CI: –0.0038, –0.0009, p = 0.003) than in females (β = –0.0009; 95% CI: –0.0020, 0.0003, p = 0.1). Elevated mean childhood blood lead concentration was also asso-ciated with a significant decrease in IGF2/H19 (β = –0.0013; 95% CI: –0.0023, –0.0003, p = 0.01) DMR methylation, but primarily in females, (β = –0.0017; 95% CI: –0.0029, –0.0006, p = 0.005) rather than in males, (β = –0.0004; 95% CI: –0.0023, 0.0015, p = 0.7). Elevated blood lead concen-tration during the neonatal period was associated with higher PLAGL1/HYMAI DMR methylation regardless of sex (β = 0.0075; 95% CI: 0.0018, 0.0132, p = 0.01). The magnitude of associations between cumulative lead exposure and CpG methylation remained unaltered from 30 to 78 months. conclusions: Our findings provide evidence that early childhood lead exposure results in sex-dependent and gene-specific DNA methylation differences in the DMRs of PEG3, IGF2/H19, and PLAGL1/HYMAI in adulthood.

Original language	English
Pages (from-to)	666-673
Number of pages	8
Journal	Environmental Health Perspectives
Volume	124
Issue number	5
DOIs	https://doi.org/10.1289/ehp.1408577
Publication status	Published - May 2016

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This output contributes to the following UN Sustainable Development Goals (SDGs)

SDG 3 Good Health and Well-being

ASJC Scopus subject areas

Public Health, Environmental and Occupational Health
Health, Toxicology and Mutagenesis

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ehp.1408577Final published version, 358 KBLicence: CC BY-NC-ND

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@article{c38d3cc32bb54d088746f15a24d9d0b0,

title = "Lead exposure during early human development and DNA methylation of imprinted gene regulatory elements in adulthood",

abstract = "Background: Lead exposure during early development causes neurodevelopmental disorders by unknown mechanisms. Epidemiologic studies have focused recently on determining associations between lead exposure and global DNA methylation; however, such approaches preclude the identification of loci that may alter human disease risk. oBjectives: The objective of this study was to determine whether maternal, postnatal, and early childhood lead exposure can alter the differentially methylated regions (DMRs) that control the monoallelic expression of imprinted genes involved in metabolism, growth, and development. Methods: Questionnaire data and serial blood lead levels were obtained from 105 participants (64 females, 41 males) of the Cincinnati Lead Study from birth to 78 months. When participants were adults, we used Sequenom EpiTYPER assays to test peripheral blood DNA to quantify CpG methylation in peripheral blood leukocytes at DMRs of 22 human imprinted genes. Statistical analyses were conducted using linear regression. results: Mean blood lead concentration from birth to 78 months was associated with a significant decrease in PEG3 DMR methylation (β = –0.0014; 95\% CI: –0.0023, –0.0005, p = 0.002), stronger in males (β = –0.0024; 95\% CI: –0.0038, –0.0009, p = 0.003) than in females (β = –0.0009; 95\% CI: –0.0020, 0.0003, p = 0.1). Elevated mean childhood blood lead concentration was also asso-ciated with a significant decrease in IGF2/H19 (β = –0.0013; 95\% CI: –0.0023, –0.0003, p = 0.01) DMR methylation, but primarily in females, (β = –0.0017; 95\% CI: –0.0029, –0.0006, p = 0.005) rather than in males, (β = –0.0004; 95\% CI: –0.0023, 0.0015, p = 0.7). Elevated blood lead concen-tration during the neonatal period was associated with higher PLAGL1/HYMAI DMR methylation regardless of sex (β = 0.0075; 95\% CI: 0.0018, 0.0132, p = 0.01). The magnitude of associations between cumulative lead exposure and CpG methylation remained unaltered from 30 to 78 months. conclusions: Our findings provide evidence that early childhood lead exposure results in sex-dependent and gene-specific DNA methylation differences in the DMRs of PEG3, IGF2/H19, and PLAGL1/HYMAI in adulthood.",

author = "Yue Li and Changchun Xie and Murphy, \{Susan K.\} and David Skaar and Monica Nye and Vidal, \{Adriana C.\} and Cecil, \{Kim M.\} and Dietrich, \{Kim N.\} and Alvaro Puga and Jirtle, \{Randy L.\} and Cathrine Hoyo",

year = "2016",

month = may,

doi = "10.1289/ehp.1408577",

language = "English",

volume = "124",

pages = "666--673",

journal = "Environmental Health Perspectives",

issn = "0091-6765",

publisher = "Public Health Services, US Dept of Health and Human Services",

number = "5",

}

TY - JOUR

T1 - Lead exposure during early human development and DNA methylation of imprinted gene regulatory elements in adulthood

AU - Li, Yue

AU - Xie, Changchun

AU - Murphy, Susan K.

AU - Skaar, David

AU - Nye, Monica

AU - Vidal, Adriana C.

AU - Cecil, Kim M.

AU - Dietrich, Kim N.

AU - Puga, Alvaro

AU - Jirtle, Randy L.

AU - Hoyo, Cathrine

PY - 2016/5

Y1 - 2016/5

N2 - Background: Lead exposure during early development causes neurodevelopmental disorders by unknown mechanisms. Epidemiologic studies have focused recently on determining associations between lead exposure and global DNA methylation; however, such approaches preclude the identification of loci that may alter human disease risk. oBjectives: The objective of this study was to determine whether maternal, postnatal, and early childhood lead exposure can alter the differentially methylated regions (DMRs) that control the monoallelic expression of imprinted genes involved in metabolism, growth, and development. Methods: Questionnaire data and serial blood lead levels were obtained from 105 participants (64 females, 41 males) of the Cincinnati Lead Study from birth to 78 months. When participants were adults, we used Sequenom EpiTYPER assays to test peripheral blood DNA to quantify CpG methylation in peripheral blood leukocytes at DMRs of 22 human imprinted genes. Statistical analyses were conducted using linear regression. results: Mean blood lead concentration from birth to 78 months was associated with a significant decrease in PEG3 DMR methylation (β = –0.0014; 95% CI: –0.0023, –0.0005, p = 0.002), stronger in males (β = –0.0024; 95% CI: –0.0038, –0.0009, p = 0.003) than in females (β = –0.0009; 95% CI: –0.0020, 0.0003, p = 0.1). Elevated mean childhood blood lead concentration was also asso-ciated with a significant decrease in IGF2/H19 (β = –0.0013; 95% CI: –0.0023, –0.0003, p = 0.01) DMR methylation, but primarily in females, (β = –0.0017; 95% CI: –0.0029, –0.0006, p = 0.005) rather than in males, (β = –0.0004; 95% CI: –0.0023, 0.0015, p = 0.7). Elevated blood lead concen-tration during the neonatal period was associated with higher PLAGL1/HYMAI DMR methylation regardless of sex (β = 0.0075; 95% CI: 0.0018, 0.0132, p = 0.01). The magnitude of associations between cumulative lead exposure and CpG methylation remained unaltered from 30 to 78 months. conclusions: Our findings provide evidence that early childhood lead exposure results in sex-dependent and gene-specific DNA methylation differences in the DMRs of PEG3, IGF2/H19, and PLAGL1/HYMAI in adulthood.

AB - Background: Lead exposure during early development causes neurodevelopmental disorders by unknown mechanisms. Epidemiologic studies have focused recently on determining associations between lead exposure and global DNA methylation; however, such approaches preclude the identification of loci that may alter human disease risk. oBjectives: The objective of this study was to determine whether maternal, postnatal, and early childhood lead exposure can alter the differentially methylated regions (DMRs) that control the monoallelic expression of imprinted genes involved in metabolism, growth, and development. Methods: Questionnaire data and serial blood lead levels were obtained from 105 participants (64 females, 41 males) of the Cincinnati Lead Study from birth to 78 months. When participants were adults, we used Sequenom EpiTYPER assays to test peripheral blood DNA to quantify CpG methylation in peripheral blood leukocytes at DMRs of 22 human imprinted genes. Statistical analyses were conducted using linear regression. results: Mean blood lead concentration from birth to 78 months was associated with a significant decrease in PEG3 DMR methylation (β = –0.0014; 95% CI: –0.0023, –0.0005, p = 0.002), stronger in males (β = –0.0024; 95% CI: –0.0038, –0.0009, p = 0.003) than in females (β = –0.0009; 95% CI: –0.0020, 0.0003, p = 0.1). Elevated mean childhood blood lead concentration was also asso-ciated with a significant decrease in IGF2/H19 (β = –0.0013; 95% CI: –0.0023, –0.0003, p = 0.01) DMR methylation, but primarily in females, (β = –0.0017; 95% CI: –0.0029, –0.0006, p = 0.005) rather than in males, (β = –0.0004; 95% CI: –0.0023, 0.0015, p = 0.7). Elevated blood lead concen-tration during the neonatal period was associated with higher PLAGL1/HYMAI DMR methylation regardless of sex (β = 0.0075; 95% CI: 0.0018, 0.0132, p = 0.01). The magnitude of associations between cumulative lead exposure and CpG methylation remained unaltered from 30 to 78 months. conclusions: Our findings provide evidence that early childhood lead exposure results in sex-dependent and gene-specific DNA methylation differences in the DMRs of PEG3, IGF2/H19, and PLAGL1/HYMAI in adulthood.

UR - https://www.scopus.com/pages/publications/84964844973

U2 - 10.1289/ehp.1408577

DO - 10.1289/ehp.1408577

M3 - Article

C2 - 26115033

AN - SCOPUS:84964844973

SN - 0091-6765

VL - 124

SP - 666

EP - 673

JO - Environmental Health Perspectives

JF - Environmental Health Perspectives

IS - 5

ER -

Lead exposure during early human development and DNA methylation of imprinted gene regulatory elements in adulthood

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