Table 1.
Summary of derm A594 and ntx A594 affinity measurementsa
| Ligand | Assay | Affinity (nm) |
|---|---|---|
| derm A594 | Radioligand competition | 2.9 ± 0.8 (Ki) |
| +Na+, Mg2+, GTPγS | 120 ± 40 nm (Ki) | |
| Association kinetics | 111 (85–149) (Kd) | |
| Association kinetics after ME 2 h | 32 (24–42 (Kd) | |
| Steady-state imaging | 85 (50–142) (EC50) | |
| Steady-state after ME 2 h | 11.6 (8.4–16.2) (EC50) | |
| ntx A594 | Kinetics | 53 (44–65) (Kd) |
a [3H]Diprenorphine competition performed in crude membrane preparations in the presence and absence of Na+, Mg2+, and GTPγS (Ki ± SD; Fig. 2A) revealed low- and high-affinity states of derm A594 binding. Kinetic affinity measurements from live cells were calculated from initial apparent binding kinetics measured for a range of derm A594 concentrations performed in live cells untreated and pretreated with ME 2 h (Kd ± error range; Fig. 2C,D). Steady-state binding of derm A594 to live cells untreated and pretreated with ME 2 h (EC50 ± 95% CI; Figs. 2B, 3B) are shown demonstrating increased affinity after ME treatment. Affinity of ntx A594 was based on measurement of apparent on rate and off rate of ntx A594 (100 nm, 5 min) (Kd ± error range; Fig. 6B). ntx A594 shows similar affinity to derm A594 despite different kinetics.