Entering edit mode
6.9 years ago
Duff
▴
670
Hi
I have some Illumina RNA seq data, 75bp paired end reads. I've run FastQC & trimmomatic and then re-run FastQC. Both before and after trimmomatic quite a few of my sequences fail the per base sequence content with the %A content running low in read 1 (e.g. http://i.imgur.com/Cv4HXJq.png) and the %T running low in read 2 (e.g. http://i.imgur.com/ul7v55H.png). Read 2 tends to be a warning rather than a fail.
Per base quality is good across the board, per sequence GC content looks fine and the only other fails I get are duplicated sequences and kmer content (both of which I gather are common fails in mRNA seq data).
I've little experience with RNA seq QC - is this something to be concerned about?
Thanks for any advice.
Best,
Iain
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Ah - strand specific. So obvious now you've pointed that out. Thanks. Can't see any poly A or oligo T in the kmers.
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I was looking at a fungal genome once that seemed to consist of only 3 letters on each strand. IIRC, one strand was only A, C, and G and the other was only C, G, and T (at least, in the areas I looked at). So if as Harold suggests your data is strand-specific, that particular organism might show this kind of pattern, if one of the two strands was generally coding and the other wasn't.