Fig. 4

Correlation between duplicate reads, spike-ins and the sequencing platforms. a, b Plots showing the frequency of distribution of duplicate reads for two cell line DNA samples during down sampling of the raw reads from HiSeq X Ten to the number of raw reads obtained from HiSeq 2500. c Box plot showing the difference in duplicate percentage when the same set of ten bisulphite libraries were spiked with 25% of 250 pM genomic library and 25% of 300 pM PhiX library