Hi guys,
we are currently analyzing RNA-seq libraries from tomato and used FastQC for this. Remarkably, comparing the duplication levels from the forward and reverse library of the same experiment we see a different pattern in duplication level.
The plots you can find attached show, that the reverse reads are a lot more duplicated than the forward reads.
Do any of you have an explanation for this phenomenom? We expected a similar pattern for forward and reverse library.
Thanks a lot!
we are currently analyzing RNA-seq libraries from tomato and used FastQC for this. Remarkably, comparing the duplication levels from the forward and reverse library of the same experiment we see a different pattern in duplication level.
The plots you can find attached show, that the reverse reads are a lot more duplicated than the forward reads.
Do any of you have an explanation for this phenomenom? We expected a similar pattern for forward and reverse library.
Thanks a lot!
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