CHM13 PRO-seq Bowtie2 (-k 100) alignments to CHM13v1.1 and Meryl unique k-mer filtering (stranded & not stranded)
The PRO-seq experiment was done on CHM13 cells and sequenced for 75bp single-ended reads.
Reads were adapter trimmed, quality filtered and D. melanogaster spike-ins were removed.
Reads were mapped with Bowtie2 -k 100 and then filtered through unique genome-wide 21 or 51mers
Savannah Hoyt (PROseq library prep & sequencing; all mapping & filtering)
Rachel O'Neill
Arang Rhie (Meryl software for generation of unique kmers)