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Hi Maria,
Kind Regards, |
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I forgot to add descriptions of some options like --maxNH in README. I'll add them later. |
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Hi,
I have been using RiboTISH with QTI-seq public data (SRR1630828 and SRR1630830, also analyzed in RiboTISH paper) and I am a bit confused about the topics I mentioned in the subject. Hope you can shed some light here, specifically:
Is RiboTISH discarding the multi-mapper reads?
I find it confusing because in the related paper, according to methods, the parameter -outSAMmultNmax is set to 1 (so allow for multimapping, just one hit) but then in the RPF length distribution, only those RPFs uniquely mapped to annotated protein- coding genes are considered. I have obtained a huge number of multi-mapping reads and was wondering if they are really 'useless' or not.
Based on your experience about the TIS enrichment score, is there any minimum score value that we could consider to assume acceptable quality data?
Since it is QTI-seq data, we were expecting to have most of the reads accumulated around the translational start regions. However, we have seen multiple reads aligned to other gene exons. We would assume this profile with Ribo-seq data but not for QTI-seq.
Inspecting the results (without applying FDR q-value threshold), we have seen that TIS site with ATG codon is not listed or not significant in some genes (i.e. for TP53 gene) while alternate codons are significantly predicted. Honestly, we expected to obtain TISs with ATG for all genes (with data) and additionally, zero or more alternate codons, are we wrong? I mean, is it right to have only significant TIS with alternate start codons but not with the canonical?
And some minor question:
Many thanks in advance for any comment about this!!
Kind Regards,
Maria Maqueda
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