Measurement of DNA Methylation and Nuclear Organization with Nanopore Sequencing

Methylated adenosine sequencing has applications in bacterial epigenetics as well as exogenous labeling in mammalian systems. In particular, the damID method uses a dam enzyme fused to a protein of interest, e.g. nuclear lamina, resulting in labeling DNA proximal to the protein. We are able to detect this N6-mA modification simultaneously with 5mC, providing two distinct epigenetic signatures along ~10kb single DNA molecules. To train our model distinguishing methylated from unmethylated adenosine, we sequenced both completely unmethylated, fully dam-methylated (N6-mA), and dam (N6-mA) and M.SssI (5-mC) methylated E. coli and human genomic DNA, where dam methylates adenine residues in a 5’-GATC-3’ context and M.SssI methylates cytosine residues in a 5’-CG-3’ context. We applied this model to mammalian cells treated by damID to characterize lamin-associated domains (LADs). LADs identified using microarray probes showed on average significantly higher methylation profiles than other regions in our pipeline. Applying this model we can simultaneously measure phased nuclear positioning information (LADs) with DNA cytosine methylation (5-mC) using long reads.