Hi,

I have around 500 RNA-Seq datasets, all analyzed using DESeq. As I studied similar questions and posts here, specialists recommend to use Stat column values as ranking metric for genes. However, the stat column is not included in the the DE analysis results. I have Log2FC, p-value, and adjusted p-value, and standard deviation for each group. I am not sure what metric should I pick now. I have tried once with fold-change and another time with absolute fold change. Which one is valid? I am getting two different set of significant pathways using each.

I have tried once with fold-change and another time with absolute fold change. Which one is valid? I am getting two different set of significant pathways using each.

It depends on what changes you are looking for. Ranking genes by logFC will prioritize pathways that are predominantly up- or down- regulated, while absolute logFC ranking will prioritize pathways that have many changing genes (independent of direction, e.g. a pathway that have 50% genes going up and 50% genes going down will be highly significant). Normally, people are looking for directed change, so signed ranking is proffered. But there can be situations when absolute ranking is also meaningful. Just make sure to use scoreType="pos" option to run a one-tailed test.

As for selecting the best signed metric - currently there is no proper consensus and people use different ones. In general, the results should be pretty similar. That said, if the logFC represent DESEq2-shrinked logFC estimates, it should be a pretty good metric. You can also try signed logPval, that is log(pvalue) * sign(logFC).