Hi everyone,

I want to run GSEA with my RNA-seq data using fgsea Bioconductor package (http://www.bioconductor.org/packages/release/bioc/vignettes/fgsea/inst/doc/fgsea-tutorial.html). What metric for gene ranking should I use? Should it be absolute log fold changes or not? In the example, provided by fgsea, they use not absolute log fold changes, however, I am not sure, if it makes sense, since gene sets (pathways and GO terms) usually don't have direction.

Thank you

To perform GSEA analysis we typically use the log2-fold change NOT THE ABSOLUTE FOLD CHANGE with a pre-ranked GSEA. Pre-ranked GSEA will give you an output for enriched genes in the positive direction (upregulated) and enriched genes in the negative direction (downregulated). By using the absolute fold change you're losing that directional data, and will get erroneous results.

For example, if you have a gene set of interest and half of the genes are upregulated and half are downregulated there should be no enrichment for this gene set. However, if you rank based on the absolute fold change, a strong upregulation and enrichment will be reported.

GSEA uses a ranked list of genes (ranking by any suitable metric like fold-change). For RNA-seq data, you need to run GSEAPreranked instead of GSEA and it has been very well explained in the FAQ

https://software.broadinstitute.org/cancer/software/gsea/wiki/index.php/FAQ#Can_I_use_GSEA_to_analyze_SNP.2C_SAGE.2C_ChIP-Seq_or_RNA-Seq_data.3F