Comparison of enzymatic and bisulfite conversion of circulating cell-free tumor DNA for DNA methylation analyses

Stine H Kresse; Evy Marie Thorkildsen; Sara Brandt-Winge; Heidi Pharo; Hege Marie Vedeld; Guro E Lind

doi:10.1186/s13148-025-01901-4

Comparison of enzymatic and bisulfite conversion of circulating cell-free tumor DNA for DNA methylation analyses

Clin Epigenetics. 2025 Jun 4;17(1):93. doi: 10.1186/s13148-025-01901-4.

Authors

Stine H Kresse¹, Evy Marie Thorkildsen¹, Sara Brandt-Winge¹, Heidi Pharo¹, Hege Marie Vedeld¹, Guro E Lind^{2

3}

Affiliations

¹ Department of Molecular Oncology, Institute for Cancer Research, Norwegian Radium Hospital, Oslo University Hospital, Oslo, Montebello, 0379, Norway.
² Department of Molecular Oncology, Institute for Cancer Research, Norwegian Radium Hospital, Oslo University Hospital, Oslo, Montebello, 0379, Norway. guroli@uio.no.
³ Department of Biosciences, Faculty of Mathematics and Natural Sciences, University of Oslo, Oslo, Norway. guroli@uio.no.

Abstract

Background: Detection of DNA methylation biomarkers in circulating cell-free DNA (cfDNA) has great clinical potential for cancer management, but there is a high need for method optimization and standardization. Bisulfite conversion of DNA is the gold-standard pre-treatment method for DNA methylation analyses, but causes also DNA fragmentation and loss. Enzymatic conversion of DNA represents a promising alternative due to the more gentle treatment minimizing damage to DNA. The aim of this study was to evaluate and compare enzymatic and bisulfite conversion to identify the best pre-treatment method for detecting DNA methylation biomarkers in cfDNA from plasma using droplet digital PCR (ddPCR).

Results: The performance of the NEBNext Enzymatic Methyl-seq Kit (both the full kit intended for sequencing and the sub-component NEBNext Enzymatic Methyl-seq Conversion Module) and the EpiTect Plus DNA Bisulfite Kit was evaluated and compared using normal cfDNA and tumor cfDNA samples from colorectal cancer patients. The cytosine conversion efficiency was 99-100% for both enzymatic and bisulfite conversion. Enzymatic conversion resulted in longer DNA fragments with higher peak fragment sizes compared to bisulfite conversion, but the DNA recovery was considerably lower after enzymatic conversion (34-47%) compared to bisulfite conversion (61-81%). For enzymatic conversion, the full kit gave slightly better DNA recovery than the conversion module. A comparison of five magnetic bead brands, as well as several different magnetic bead-to-sample ratios revealed no major improvements in DNA recovery for the enzymatic conversion. DNA methylation of the biomarker BCAT1 was detected at similar rates in parallel tumor cfDNA samples pre-treated with either enzymatic or bisulfite conversion. However, enzymatic conversion resulted in lower number of positive droplets for both target and control ddPCR assays, in line with the lower DNA recovery after conversion.

Conclusions: Based on a thorough evaluation of enzymatic and bisulfite conversion of cfDNA using ddPCR, bisulfite conversion emerges as the best pre-treatment method due to higher DNA recovery after conversion and higher number of positive droplets in the ddPCR reactions.

Keywords: Bisulfite conversion; Circulating cell-free tumor DNA; Colorectal cancer; DNA methylation; Enzymatic Methyl-seq; Enzymatic conversion; Liquid biopsy; Magnetic beads; Plasma; cfDNA; ctDNA; ddPCR.

Publication types

Comparative Study

MeSH terms

Biomarkers, Tumor / blood
Biomarkers, Tumor / genetics
Circulating Tumor DNA* / analysis
Circulating Tumor DNA* / blood
Circulating Tumor DNA* / genetics
Colorectal Neoplasms* / blood
Colorectal Neoplasms* / genetics
DNA Methylation*
Female
Humans
Polymerase Chain Reaction / methods
Sequence Analysis, DNA / methods
Sulfites* / chemistry

Substances

Sulfites
hydrogen sulfite
Circulating Tumor DNA
Biomarkers, Tumor

Abstract

Publication types

MeSH terms

Substances

Grants and funding