(A) TCRγδ/CD3ε surface expression on LOUCY cells that were cultured in media or cocultured for 3 days on OP9-DL1 stromal cells, in the absence or presence of 10 μM of γ-secretase inhibitor DAPT visualized by flow cytometry (n = 3). (B) Transduced LOUCY cells containing a dox-inducible MEF2C-BFP overexpression construct (middle panels) or an IPTG-inducible MEF2C shRNA knockdown construct (bottom panels) were generated and compared with parental LOUCY cells (top panels). Blue fluorescence (BFP, blue-filled histograms), intracellular MEF2C levels (green-filled histograms), and surface CD3ε levels (red-filled histograms) were analyzed using flow cytometry in the absence (open histograms) or presence of dox or IPTG, respectively (filled histograms), as indicated. “Endog. MEF2C” refers to endogenous MEF2C expression levels in the MEF2C shRNA knockdown line. CD3ε expression after coculture on OP9 control or OP9-DL1 stromal cells (right columns). (C) Significantly enriched up- (red) or downregulated (blue) GO terms in MEF2C-induced LOUCY cells for 24 hours compared with noninduced LOUCY cells. (D) Heatmaps of significantly up- or downregulated probe sets (log₂ fold change >0.6, P < 0.05, FDR < 0.1) in triplicate gene expression analysis (Affymetrix GeneChip Human Genome U133 Plus 2.0) per condition for LOUCY_MEF2C-BFP cells with/without MEF2C induction for 24 hours (± dox). Downregulated or upregulated probe sets following MEF2C-induction are shown in blue or red, respectively. Three of the 4 MEF2C probe sets, designated with asterisks, lie outside the cloned MEF2C cDNA sequence and thus represent endogenous MEF2C levels, whereas the other MEF2C probe set (indicated by the arrow) also covers the cloned cDNA construct.