Pooled CRISPR screening in primary T cells faces several technical challenges including efficient Cas9 delivery and sgRNA library transduction. For this reason, screens are often performed in cell line models, such as Jurkats, which are known to poorly represent primary T cell biology. We have adapted the SLICE protocol for genome-wide CRISPR screening in primary T cells and show that this method is applicable and adaptable across major T cell sub-populations. We determined that cell age is a key indicator of transducibility allowing us to forecast viral requirements based on cell age. We have evolved this method further to now be able to integrate biologically relevant genetic modifications into the process, in order to utilise this platform to support the target/drug discovery and development process across the AZ and CRUK communities.