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Hi,
I have some Illumina GAII paired end reads (bisulfite converted) taken from a previous study.
It seems that based on the FASTQC report that there are two sequence lengths 50BP and 76BP contained in my read.
I was just wondering how the quality scores are calculated as they drop off quite considerably after 50BP. E.g. is this a real drop off in qualities on the 76BP reads (and hence should be trimmed) or is it because it is taking the 50BP reads as having 0 quality above 50BP and hence producing an incorrect average quality score?
I attempted looking at the code but I don't know Java well enough to understand whats going on.
Many thanks for any help,
Rob
I have some Illumina GAII paired end reads (bisulfite converted) taken from a previous study.
It seems that based on the FASTQC report that there are two sequence lengths 50BP and 76BP contained in my read.
I was just wondering how the quality scores are calculated as they drop off quite considerably after 50BP. E.g. is this a real drop off in qualities on the 76BP reads (and hence should be trimmed) or is it because it is taking the 50BP reads as having 0 quality above 50BP and hence producing an incorrect average quality score?
I attempted looking at the code but I don't know Java well enough to understand whats going on.
Many thanks for any help,
Rob
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