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English: Epigenomics and the spectrum of single-cell sequencing technologies. The diagram outlines the single-cell sequencing technologies currently available. A single cell is first isolated by means of droplet encapsulation, manual manipulation, fluorescence-activated cell sorting (FACS) or microfluidic processing. The first examples of single-cell multi-omic technologies have used parallel amplification or physical separation to measure gene expression (scRNA-seq) and DNA sequence (scDNA-seq) from the same cell. Note that single-cell bisulfite conversion followed by sequencing (scBS-seq) is not compatible with parallel amplification of RNA and DNA, as DNA methylation is not conserved during in vitro amplification. Single-cell epigenomics approaches utilize chemical treatment of DNA (bisulfite conversion), immunoprecipitation or enzymatic digest (e.g., by DNaseI) to study DNA modifications (scBS-seq and scRRBS), histone modifications (scChIP-seq), DNA accessibility (scATAC-seq, scDNase-seq), chromatin conformation (scDamID, scHiC)
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Source https://genomebiology.biomedcentral.com/articles/10.1186/s13059-016-0944-x
Author Stephen J. Clark, Heather J. Lee, Sébastien A. Smallwood, Gavin Kelsey and Wolf Reik
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current14:44, 23 July 2017Thumbnail for version as of 14:44, 23 July 2017778 × 774 (117 KB)Kierano (talk | contribs)Transferred from http://media.springernature.com/full/springer-static/image/art%3A10.1186%2Fs13059-016-0944-x/MediaObjects/13059_2016_944_Fig1_HTML.gif

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