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Endonuclease enrichment TAPS for cost-effective genome-wide base-resolution DNA methylation detection
Author(s) -
Jingfei Cheng,
Paulina Siejka-Zielińska,
Yibin Liu,
Anandhakumar Chandran,
Skirmantas Kriaučionis,
ChunXiao Song
Publication year - 2021
Publication title -
nucleic acids research
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 9.008
H-Index - 537
eISSN - 1362-4954
pISSN - 0305-1048
DOI - 10.1093/nar/gkab291
Subject(s) - biology , genome , dna methylation , endonuclease , cpg site , computational biology , dna sequencing , genetics , illumina methylation assay , bisulfite sequencing , illumina dye sequencing , hybrid genome assembly , restriction enzyme , deep sequencing , methylated dna immunoprecipitation , dna , gene , gene expression
Whole genome base-resolution methylome sequencing allows for the most comprehensive analysis of DNA methylation, however, the considerable sequencing cost often limits its applications. While reduced representation sequencing can be an affordable alternative, over 80% of CpGs in the genome are not covered. Building on our recently developed TET-assisted pyridine borane sequencing (TAPS) method, we here described endonuclease enrichment TAPS (eeTAPS), which utilizes dihydrouracil (DHU)-cleaving endonuclease digestion of TAPS-converted DNA to enrich methylated CpG sites (mCpGs). eeTAPS can accurately detect 87% of mCpGs in the mouse genome with a sequencing depth equivalent to 4× whole genome sequencing. In comparison, reduced representation TAPS (rrTAPS) detected less than 4% of mCpGs with 2.5× sequencing depth. Our results demonstrate eeTAPS to be a new strategy for cost-effective genome-wide methylation analysis at single-CpG resolution that can fill the gap between whole-genome and reduced representation sequencing.

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