Comparison of methods for quantification of global DNA methylation in human cells and tissues

Lisanti, Sofia; Omar, Wan A.W.; Tomaszewski, Bartlomiej; de Prins, Sofie; Jacobs, Griet; Koppen, Gudrun; Mathers, John C.; Langie, Sabine A. S.

doi:10.1371/JOURNAL.PONE.0079044

Title

Comparison of methods for quantification of global DNA methylation in human cells and tissues

Author

Lisanti, Sofia

Omar, Wan A.W.

Tomaszewski, Bartlomiej

de Prins, Sofie

Jacobs, Griet

Koppen, Gudrun

Mathers, John C.

Langie, Sabine A. S.

Abstract

DNA methylation is a key epigenetic modification which, in mammals, occurs mainly at CpG dinucleotides. Most of the CpG methylation in the genome is found in repetitive regions, rich in dormant transposons and endogenous retroviruses. Global DNA hypomethylation, which is a common feature of several conditions such as ageing and cancer, can cause the undesirable activation of dormant repeat elements and lead to altered expression of associated genes. DNA hypomethylation can cause genomic instability and may contribute to mutations and chromosomal recombinations. Various approaches for quantification of global DNA methylation are widely used. Several of these approaches measure a surrogate for total genomic methyl cytosine and there is uncertainty about the comparability of these methods. Here we have applied 3 different approaches (luminometric methylation assay, pyrosequencing of the methylation status of the Alu repeat element and of the LINE1 repeat element) for estimating global DNA methylation in the same human cell and tissue samples and have compared these estimates with the "gold standard'' of methyl cytosine quantification by HPLC. Next to HPLC, the LINE1 approach shows the smallest variation between samples, followed by Alu. Pearson correlations and Bland-Altman analyses confirmed that global DNA methylation estimates obtained via the LINE1 approach corresponded best with HPLC-based measurements. Although, we did not find compelling evidence that the gold standard measurement by HPLC could be substituted with confidence by any of the surrogate assays for detecting global DNA methylation investigated here, the LINE1 assay seems likely to be an acceptable surrogate in many cases.

Language

English

Source (journal)

PLoS ONE

Publication

2013

ISSN

1932-6203

DOI

10.1371/JOURNAL.PONE.0079044

Volume/pages

8 :11 (2013) , p. 1-11

Article Reference

e79044

ISI

000327308500021

Medium

E-only publicatie

Full text (Publisher's DOI)

https://doi.org/10.1371/JOURNAL.PONE.0079044

Full text (open access)

https://repository.uantwerpen.be/docman/irua/ccee19/6430.pdf

Faculty/Department				Faculty of Pharmaceutical, Biomedical and Veterinary Sciences . Biomedical Sciences

Research group
Publication type				A1 Journal article

Subject				Engineering sciences. Technology

Affiliation				Publications with a UAntwerp address

Web of Science

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Identifier

Creation

15.01.2014

Last edited

09.10.2023

To cite this reference

https://hdl.handle.net/10067/1128230151162165141