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Hi everyone,
Is there a standard approach to addressing transcript length bias in gene expression? I have come across the window approach provided by Oshlack & Wakefield (2012), but not much else.
I have run Bowtie2 with insert restrictions, ignoring discordant alignments, and removed reads that are not uniquely aligned afterwards (resulting in a uniquely aligned, concordant SAM file). Following this, I ran the SAM file through htseq-count and DESeq. The following graph shows the significant relationship between scaffold length and the BaseMean Expression provided by DESeq (the p-value is very low, but the R2 is also very low). Any thoughts? Thanks for any input!
Is there a standard approach to addressing transcript length bias in gene expression? I have come across the window approach provided by Oshlack & Wakefield (2012), but not much else.
I have run Bowtie2 with insert restrictions, ignoring discordant alignments, and removed reads that are not uniquely aligned afterwards (resulting in a uniquely aligned, concordant SAM file). Following this, I ran the SAM file through htseq-count and DESeq. The following graph shows the significant relationship between scaffold length and the BaseMean Expression provided by DESeq (the p-value is very low, but the R2 is also very low). Any thoughts? Thanks for any input!
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