Epigenetics (Oct 2022)

Comparison of EM-seq and PBAT methylome library methods for low-input DNA

  • Yanan Han,
  • Galina Yurevna Zheleznyakova,
  • Yanara Marincevic-Zuniga,
  • Majid Pahlevan Kakhki,
  • Amanda Raine,
  • Maria Needhamsen,
  • Maja Jagodic

DOI
https://doi.org/10.1080/15592294.2021.1997406
Journal volume & issue
Vol. 17, no. 10
pp. 1195 – 1204

Abstract

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DNA methylation is the most studied epigenetic mark involved in regulation of gene expression. For low input samples, a limited number of methods for quantifying DNA methylation genome-wide has been evaluated. Here, we compared a series of input DNA amounts (1–10ng) from two methylome library preparation protocols, enzymatic methyl-seq (EM-seq) and post-bisulfite adaptor tagging (PBAT) adapted from single-cell PBAT. EM-seq takes advantage of enzymatic activity while PBAT relies on conventional bisulfite conversion for detection of DNA methylation. We found that both methods accurately quantified DNA methylation genome-wide. They produced expected distribution patterns around genomic features, high C-T transition efficiency at non-CpG sites and high correlation between input amounts. However, EM-seq performed better in regard to library and sequencing quality, i.e. EM-seq produced larger insert sizes, higher alignment rates and higher library complexity with lower duplication rate compared to PBAT. Moreover, EM-seq demonstrated higher CpG coverage, better CpG site overlap and higher consistency between input series. In summary, our data suggests that EM-seq overall performed better than PBAT in whole-genome methylation quantification of low input samples.

Keywords