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Hi All,
I have prepared some Truseq RNA-seq libraries and i have 2 peaks.
I have been reading some previous threads that it could be bead carry-over, but I do not really see any beads in my library and I think some of the libraries look a bit different. Do you have any suggestions to what the problem could be?
I used another protocol than usual to remove rRNA but I do not think it should be the problem (Epicentre - Ribo Zero : http://www.illumina.com/products/rib...-kit-faqs.html)
I have prepared some Truseq RNA-seq libraries and i have 2 peaks.
I have been reading some previous threads that it could be bead carry-over, but I do not really see any beads in my library and I think some of the libraries look a bit different. Do you have any suggestions to what the problem could be?
I used another protocol than usual to remove rRNA but I do not think it should be the problem (Epicentre - Ribo Zero : http://www.illumina.com/products/rib...-kit-faqs.html)
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