Table 2.
Most commonly used functional assays to monitor the impact of small molecule agents on PD-1 pathway.
| Type of assay | Source for PD-1 | Source for PD-L1 | Consequence of interfering in the PD-1:PD-L1 interaction by small molecules | Detection system | Comments |
|---|---|---|---|---|---|
| NFAT reporter | Jurkat (immortalized line of human T cells) overexpressing PD-1 and luciferase gene controlled by the NFAT-response element | CHO-K1 (Chinese hamster ovary cells) cell line overexpressing PD-L1 and T-cell receptor activator | Activation of TCR signaling leading to greater luciferase expression | Chemiluminescence | Engineered cell line as T cells in the assay. Assay commercially available |
| SHP-1 | Jurkat cells expressing PD-1 and SHP-1 each fused with different individually inactive fragments of the β-galactosidase | U-2 OS osteosarcoma cell line expressing PD-L1 | Decrease in SHP-1 recruitment leading to lower β-galactosidase activity due to reduced enzyme fragment complementation | Chemiluminescence | Engineered cell line as T cells in the assay. Assay commercially available |
| PBMC | T cells activated by anti-CD3/anti-CD28 | Recombinant protein | Activation of TCR signaling leading to the rescue of proliferation or cytokine release | FACS or ELISA | Primary T cells in the assay—closer to physiological context |
| PBMC/whole blood | T cells activated by staphylococcal enterotoxin B (SEB) or CMV antigen | Other cells in PBMCs or blood; not controlled likely leading to greater variability in the assay | Activation of TCR signaling leading to the rescue of proliferation or cytokine release | FACS or ELISA | Primary T cells in the assay—closer to physiological context |