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According to Iso-Seq Docs, 'Lima will orient sequences to 5’ → 3’ orientation according to the asymmetry of the primers.'. This is definitely not happening with my data and I have no idea why. Any help will be greatly appreciated.
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Both lima runs are able to trim the primers (IsoSeqX_bc03_5p and IsoSeqX_3p) really well. I also manually inspect this with: Can anyone share with me their results for the amount of polyt reads after lima? Why is this not working for me? |
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You ended up in the wrong GitHub repo. To file a bug against the bioconda software try the https://github.com/PacificBiosciences/pbbioconda issue tracker. |
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You ended up in the wrong GitHub repo. To file a bug against the bioconda software try the https://github.com/PacificBiosciences/pbbioconda issue tracker.