Research output per year
Research output per year
Tim Stuart, Sam Buckberry, Trung Viet Nguyen, Ryan Lister
Research output: Chapter in Book/Conference paper › Chapter › peer-review
DNA methylation is a covalent modification of DNA that plays important roles in processes such as the regulation of gene expression, transcription factor binding, and suppression of transposable elements. The use of whole-genome bisulfite sequencing (WGBS) enables the genome-wide identification and quantification of DNA methylation patterns at single-base resolution and is the gold standard for the analysis of DNA methylation. However, the computational analysis of WGBS data can be particularly challenging, as many computationally intensive steps are required. Here, we outline step-by-step an approach for the analysis and interpretation of WGBS data. First, sequencing reads must be trimmed, quality-checked, and aligned to the genome. Second, DNA methylation levels are estimated at each cytosine position using the aligned sequence reads of the bisulfite-treated DNA. Third, regions of differential cytosine methylation between samples can be identified. Finally, these data need to be visualized and interpreted in the context of the biological question at hand.
Original language | English |
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Title of host publication | Epigenome Editing |
Subtitle of host publication | Methods and Protocols |
Editors | Albert Jeltsch, Marianne G. Rots |
Publisher | Humana Press Inc. |
Pages | 391-403 |
Number of pages | 13 |
Edition | 2 |
ISBN (Electronic) | 978-1-0716-4051-7 |
ISBN (Print) | 978-1-0716-4050-0, 978-1-0716-4053-1 |
DOIs | |
Publication status | Published - 2024 |
Name | Methods in Molecular Biology |
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Volume | 2842 |
ISSN (Print) | 1064-3745 |
ISSN (Electronic) | 1940-6029 |
Research output: Chapter in Book/Conference paper › Chapter › peer-review