HI, I want to compare the differential expression (prokaryotic) in metatranscriptomics samlples form two different conditions. I used Prodigal to get the gff file and later used featurecount to get the raw counts of each predicted region. But from some of the blogs/articles it is mentioned that for Differential expression analysis we should use Exon count rather than CDS. Prodigal can predict just CDS region. Is it ok to use CDS regions for DE analysis? if not, how can i predict the related exons from my assembled fasta file?