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- Title
Quantitative DNA methylation analysis based on four-dye trace data from direct sequencing of PCR amplificates.
- Authors
Lewin, Jörn; Schmitt, Armin O; Adorján, Péter; Hildmann, Thomas; Piepenbrock, Christian
- Abstract
Methylation of cytosines in DNA plays an important role in the regulation of gene expression, and the analysis of methylation patterns is fundamental for the understanding of cell differentiation, aging processes, diseases and cancer development. Such analysis has been limited, because technologies for detailed and efficient high-throughput studies have not been available. We have developed a novel quantitative methylation analysis algorithm and workflow based on direct DNA sequencing of PCR products from bisulfite-treated DNA with high-throughput sequencing machines. This technology is a prerequisite for success of the Human Epigenome Project, the first large genome-wide sequencing study for DNA methylation in many different tissues. Methylation in tissue samples which are compositions of different cells is a quantitative information represented by cytosine/thymine proportions after bisulfite conversion of unmethylated cytosines to uracil and PCR. Calculation of quantitative methylation information from base proportions represented by different dye signals in four-dye sequencing trace files needs a specific algorithm handling imbalanced and overscaled signals, incomplete conversion, quality problems and basecaller artifacts.
- Publication
Bioinformatics (Oxford, England), 2004, Vol 20, Issue 17, p3005
- ISSN
1367-4803
- Publication type
Journal Article
- DOI
10.1093/bioinformatics/bth346