[BioC] RSEM for transcript and gene level read count and edgeR differential expression analysis
Steve Lianoglou
lianoglou.steve at gene.com
Mon Aug 19 22:44:04 CEST 2013
Hi,
On Mon, Aug 19, 2013 at 11:17 AM, Alan Smith <alan.sm310 at gmail.com> wrote:
> Hello,
>
> I used RSEM to extract gene and transcript level read count information for
> our single end read libraries. Then rounded off the expected read counts to
> use for differential expression analysis using edgeR at both transcript and
> gene level. However, I found that the number of DE transcripts were almost
> 10 times less than those of genes.
>
> Is this expected or should I be following other package to analyze
> transcript level DE analysis.
If you take a minute to take a walk down memory lane and browse
through the list archives searching for "RSEM":
http://search.gmane.org/?query=rsem&author=&group=gmane.science.biology.informatics.conductor&sort=date&DEFAULTOP=and&xP=Zrsem&xFILTERS=Gscience.biology.informatics.conductor---A/
You'll find that RSEM output doesn't play well with edgeR and DESeq.
These methods explicitly require *count* data -- not any old number
that has been then rounded to an integer.
I recall a thread about how voom would likely work well with RSEM
output, but I can't seem to dig it up right now -- I'm only finding
other people mentioning that thread ;-)
HTH,
-steve
--
Steve Lianoglou
Computational Biologist
Bioinformatics and Computational Biology
Genentech
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