Hello, I am working on a "simple" lettuce RNAseq experiment comparing one situation to a control.
I did a topGO enrichment of all my differentially expressed genes.
Then, for some pathways my lab is interested in, I am trying to get back the list of the associated genes and then see how they are regulated (UP or DOWN) in the initial DGE table (fold change).
Clearly, this approach sounds true. (Especially since lettuce is not a genetic model.)
Or am I doing it the wrong way?
Note , I have allready read this post: Question: GO analysis- analyze upregulated and downregulated genes separately? and I agree to :
the fact that a gene is upregulated or downregulated does not mean that the process, function or component that the gene is annotated to is also respectively directionally regulated
Just because some genes are up or down-regulators.
I have also read this post and the associated article of Guini Hong. It seems that one could not be convinced...
I understand that GO enrichment is a hot topic, so it is hard to know If a way of analyis is really the good one...
Thanks in advance for your expertise.
I am not sure I understand what your problem is. You're interested in a pathway, you know which genes belong to this pathway and you have data that tell you whether these genes are up and down regulated. There's no problem there. So what is your question ? Is it about how to draw conclusions from this ? This is probably going to be pathway-specific because one can imagine that pathways with both positive and negative regulators would see those regulated in different ways, e.g. positive regulators could be down-regulated when negative regulators are up-regulated.
Is there a question here? Yes, having a bunch of up-regulated genes in a pathway doesn't mean that the pathway is more active (it could be less active due to increased expression of inhibitory elements). If directionality is important then you need to think of that yourself.
Sorry for the confusion, simply, my question was: What is the better way ? - Make the GO enrichment on a mixed list of up- and down-regulated genes? - Make the Go enrichment on up-regulated genes and then on down-regulated genes separately? I did the first way with topGO / R. But I know that the both approaches are used. Anyway, thanks all for your answers. I will have a look on the technics you suggested.