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Hi there guys!
I am using Subread v1.5.0-p1 to get tables of counts for RNAseq data I got from ENCODE (https://www.encodeproject.org/experiments/ENCSR000BYX/).
What I am trying to get are counts for genes (using reads assigned to exons) since I want to ultimately turn the numbers into FPKM or TPM.
However, I am getting around 13% of successfully assigned reads:
|| Total fragments : 72502756 ||
|| Successfully assigned fragments : 9324091 (12.9%) ||
|| Running time : 2.20 minutes ||
This doesn't sound right to me, I am used to getting 50-75% of reads assigned in RNAseq, using HTseq + DESeq2. I don't expect ENCODE data to be of poor quality so I think it's something on my side.
I tried all the combinations of fr-firststrand, fr-secondstrand, rf-firststrand, rf-secondstrand etc. Nothing gives me higher values than those 13%.
Using GENCODE M3 annotation gtf since the data was originally aligned to mm9.
This is a paired-end library from Illumina GAIIx sequencer.
Any tips ?
I am using Subread v1.5.0-p1 to get tables of counts for RNAseq data I got from ENCODE (https://www.encodeproject.org/experiments/ENCSR000BYX/).
What I am trying to get are counts for genes (using reads assigned to exons) since I want to ultimately turn the numbers into FPKM or TPM.
However, I am getting around 13% of successfully assigned reads:
|| Total fragments : 72502756 ||
|| Successfully assigned fragments : 9324091 (12.9%) ||
|| Running time : 2.20 minutes ||
This doesn't sound right to me, I am used to getting 50-75% of reads assigned in RNAseq, using HTseq + DESeq2. I don't expect ENCODE data to be of poor quality so I think it's something on my side.
I tried all the combinations of fr-firststrand, fr-secondstrand, rf-firststrand, rf-secondstrand etc. Nothing gives me higher values than those 13%.
Using GENCODE M3 annotation gtf since the data was originally aligned to mm9.
This is a paired-end library from Illumina GAIIx sequencer.
Any tips ?
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