Introduction of a multiplex amplicon sequencing assay to quantify DNA methylation in target cytosine markers underlying four selected epigenetic clocks

Ewelina Pośpiech; Aleksandra Pisarek; Joanna Rudnicka; Rezvan Noroozi; Michał Boroń; Aleksander Masny; Bożena Wysocka; Kamila Migacz-Gruszka; Dagmara Lisman; Paulina Pruszkowska-Przybylska; Magdalena Kobus; Maria Szargut; Joanna Dowejko; Kamila Stanisz; Julia Zacharczuk; Piotr Zieliński; Aneta Sitek; Andrzej Ossowski; Magdalena Spólnicka; Wojciech Branicki

doi:10.1186/s13148-023-01545-2

Introduction of a multiplex amplicon sequencing assay to quantify DNA methylation in target cytosine markers underlying four selected epigenetic clocks

Clin Epigenetics. 2023 Aug 10;15(1):128. doi: 10.1186/s13148-023-01545-2.

Authors

Ewelina Pośpiech^#^{1

2}, Aleksandra Pisarek^#³, Joanna Rudnicka^#^{4

5}, Rezvan Noroozi^{4

5}, Michał Boroń⁶, Aleksander Masny⁶, Bożena Wysocka⁶, Kamila Migacz-Gruszka⁷, Dagmara Lisman⁸, Paulina Pruszkowska-Przybylska⁹, Magdalena Kobus¹⁰, Maria Szargut⁸, Joanna Dowejko⁸, Kamila Stanisz⁸, Julia Zacharczuk⁸, Piotr Zieliński¹¹, Aneta Sitek⁹, Andrzej Ossowski⁸, Magdalena Spólnicka¹², Wojciech Branicki^{3

13}

Affiliations

¹ Malopolska Centre of Biotechnology, Jagiellonian University, Krakow, Poland. ewelina.pospiech@uj.edu.pl.
² Department of Forensic Genetics, Pomeranian Medical University in Szczecin, Szczecin, Poland. ewelina.pospiech@uj.edu.pl.
³ Institute of Zoology and Biomedical Research, Faculty of Biology, Jagiellonian University, Krakow, Poland.
⁴ Malopolska Centre of Biotechnology, Jagiellonian University, Krakow, Poland.
⁵ Doctoral School of Exact and Natural Sciences, Jagiellonian University, Krakow, Poland.
⁶ Central Forensic Laboratory of the Police, Warsaw, Poland.
⁷ Department of Dermatology, Collegium Medicum of the Jagiellonian University, Krakow, Poland.
⁸ Department of Forensic Genetics, Pomeranian Medical University in Szczecin, Szczecin, Poland.
⁹ Department of Anthropology, Faculty of Biology and Environmental Protection, University of Łódź, Łódź, Poland.
¹⁰ Institute of Biological Sciences, Faculty of Biology and Environmental Sciences, Cardinal Stefan Wyszynski University in Warsaw, Warsaw, Poland.
¹¹ Institute of Environmental Sciences, Faculty of Biology, Jagiellonian University, Krakow, Poland.
¹² Center for Forensic Science, University of Warsaw, Warsaw, Poland.
¹³ Institute of Forensic Research, Krakow, Poland.

^# Contributed equally.

Abstract

Background: DNA methylation analysis has proven to be a powerful tool for age assessment. However, the implementation of epigenetic age prediction in diagnostics or routine forensic casework requires appropriate laboratory methods. In this study, we aimed to compare the performance of large-scale DNA methylation analysis protocols that show promise in terms of accuracy, throughput, multiplexing capacity, and high sensitivity.

Results: The protocols were designed to target a predefined panel of 161 genomic CG/CA sites from four known estimators of epigenetic age-related parameters, optimized and validated using artificially methylated controls or blood samples. We successfully targeted 96% of these loci using two enrichment protocols: Ion AmpliSeq™, an amplicon-based method integrated with Ion Torrent S5, and SureSelect^XT Methyl-Seq, a hybridization-based method followed by MiSeq FGx sequencing. Both protocols demonstrated high accuracy and robustness. Although hybridization assays have greater multiplexing capabilities, the best overall performance was observed for the amplicon-based protocol with the lowest variability in DNA methylation at 25 ng of starting DNA, mean observed marker coverage of ~ 6.7 k reads, and accuracy of methylation quantification with a mean absolute difference between observed and expected methylation beta value of 0.054. The Ion AmpliSeq method correlated strongly with genome-scale EPIC microarray data (R = 0.91) and showed superiority in terms of methylation measurement accuracy. Method-to-method bias was accounted for by the use of linear transformation, which provided a highly accurate prediction of calendar age with a mean absolute error of less than 5 years for the VISAGE and Hannum age clocks used. The pace of aging (PoAm) and the mortality risk score (MRS) estimators included in our panel represent next-generation clocks, were found to have low to moderate correlations with the VISAGE and Hannum models (R < 0.75), and thus may capture different aspects of epigenetic aging.

Conclusions: We propose a laboratory tool that allows the quantification of DNA methylation in cytosines underlying four different clocks, thus providing broad information on epigenetic aging while maintaining a reasonable number of CpG markers, opening the way to a wide range of applications in forensics, medicine, and healthcare.

Keywords: DNA methylation analysis methods; Epigenetic age estimation; High-throughput sequencing; Mortality risk score; Pace of aging; Target enrichment protocols.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Aging / genetics
Child, Preschool
CpG Islands
Cytosine*
DNA Methylation*
Epigenesis, Genetic
Genomics / methods
High-Throughput Nucleotide Sequencing / methods
Humans

Substances

Cytosine