Comprehensive evaluation of targeted multiplex bisulphite PCR sequencing for validation of DNA methylation biomarker panels

Dilys Lam; Phuc-Loi Luu; Jenny Z Song; Wenjia Qu; Gail P Risbridger; Mitchell G Lawrence; Jennifer Lu; Matt Trau; Darren Korbie; Susan J Clark; Ruth Pidsley; Clare Stirzaker

doi:10.1186/s13148-020-00880-y

Comprehensive evaluation of targeted multiplex bisulphite PCR sequencing for validation of DNA methylation biomarker panels

Clin Epigenetics. 2020 Jun 22;12(1):90. doi: 10.1186/s13148-020-00880-y.

Authors

Dilys Lam¹, Phuc-Loi Luu^{1

2}, Jenny Z Song¹, Wenjia Qu¹, Gail P Risbridger^{3

4

5}, Mitchell G Lawrence^{3

4

5}, Jennifer Lu⁶, Matt Trau⁶, Darren Korbie⁶, Susan J Clark^{1

2}, Ruth Pidsley^{7

8}, Clare Stirzaker^{9

10}

Affiliations

¹ Epigenetics Research Laboratory, Genomics and Epigenetics Division, Garvan Institute of Medical Research, Sydney, New South Wales, 2010, Australia.
² St Vincent's Clinical School, UNSW Sydney, Sydney, New South Wales, 2010, Australia.
³ Monash Partners Comprehensive Cancer Consortium, Monash Biomedicine Discovery Institute Cancer Program, Prostate Cancer Research Group, Department of Anatomy and Developmental Biology, Monash University, Clayton, VIC, 3800, Australia.
⁴ Cancer Research Division, Peter MacCallum Cancer Centre, Melbourne, VIC, 3000, Australia.
⁵ Sir Peter MacCallum Department of Oncology, The University of Melbourne, Parkville, VIC, 3010, Australia.
⁶ Centre for Personalised Nanomedicine, Australian Institute for Bioengineering and Nanotechnology (AIBN), The University of Queensland, St Lucia, Queensland, 4072, Australia.
⁷ Epigenetics Research Laboratory, Genomics and Epigenetics Division, Garvan Institute of Medical Research, Sydney, New South Wales, 2010, Australia. r.pidsley@garvan.org.au.
⁸ St Vincent's Clinical School, UNSW Sydney, Sydney, New South Wales, 2010, Australia. r.pidsley@garvan.org.au.
⁹ Epigenetics Research Laboratory, Genomics and Epigenetics Division, Garvan Institute of Medical Research, Sydney, New South Wales, 2010, Australia. c.stirzaker@garvan.org.au.
¹⁰ St Vincent's Clinical School, UNSW Sydney, Sydney, New South Wales, 2010, Australia. c.stirzaker@garvan.org.au.

Abstract

Background: DNA methylation is a well-studied epigenetic mark that is frequently altered in diseases such as cancer, where specific changes are known to reflect the type and severity of the disease. Therefore, there is a growing interest in assessing the clinical utility of DNA methylation as a biomarker for diagnosing disease and guiding treatment. The development of an accurate loci-specific methylation assay, suitable for use on low-input clinical material, is crucial for advancing DNA methylation biomarkers into a clinical setting. A targeted multiplex bisulphite PCR sequencing approach meets these needs by allowing multiple DNA methylated regions to be interrogated simultaneously in one experiment on limited clinical material.

Results: Here, we provide an updated protocol and recommendations for multiplex bisulphite PCR sequencing (MBPS) assays for target DNA methylation analysis. We describe additional steps to improve performance and reliability: (1) pre-sequencing PCR optimisation which includes assessing the optimal PCR cycling temperature and primer concentration and (2) post-sequencing PCR optimisation to achieve uniform coverage of each amplicon. We use a gradient of methylated controls to demonstrate how PCR bias can be assessed and corrected. Methylated controls also allow assessment of the sensitivity of methylation detection for each amplicon. Here, we show that the MBPS assay can amplify as little as 0.625 ng starting DNA and can detect methylation differences of 1% with a sequencing coverage of 1000 reads. Furthermore, the multiplex bisulphite PCR assay can comprehensively interrogate multiple regions on 1-5 ng of formalin-fixed paraffin-embedded DNA or circulating cell-free DNA.

Conclusions: The MBPS assay is a valuable approach for assessing methylated DNA regions in clinical samples with limited material. The optimisation and additional quality control steps described here improve the performance and reliability of this method, advancing it towards potential clinical applications in biomarker studies.

Keywords: Bisulphite amplicon sequencing; Clinical biomarkers; DNA methylation; Epigenetics; Methylome; Multiplex.

Publication types

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

MeSH terms

Cell Line, Tumor
CpG Islands
DNA Methylation*
Early Detection of Cancer
Epigenesis, Genetic
Genetic Markers
Humans
Male
Multiplex Polymerase Chain Reaction / methods*
Prostatic Neoplasms / diagnosis*
Prostatic Neoplasms / genetics
Sample Size
Sensitivity and Specificity
Whole Genome Sequencing / methods*

Substances

Genetic Markers