Genetic reconstitution with wild-type AP3D1 restores expression and function of the AP3 complex. (A) Immunofluorescence analysis of patient PHA/IL-2 blasts reconstituted with either empty vector or wild-type AP3D1 using mouse anti-AP3δ (SA4). Cells are shown in one 3D stack picture of 28 slices. Cells successfully transduced with the vector are GFP-positive (white in the single stains and green in the merged picture), the nucleus is stained with Hoechst (blue), and AP3δ is stained with SA4 provided by A. Peden18 (white in the single stains and red in the merged picture). The variable GFP intensity of reconstituted cells is explained by the use of an IRES-GFP construct in which AP3D1 is placed before and GFP is placed after the IRES sequence. (B) Transduced T cells were rested in medium free of IL-2 for 24 hours and then incubated in medium or stimulated with 3 µg/mL plate-bound CD3 for 3 hours. Transduction efficiencies varied between 1% and 12%. (C) CD107a expression after incubation of transduced cells with medium or plate-bound anti-CD3. Plots are gated on successfully transduced GFP-positive CD8+ cells. The solid line indicates peak CD107a expression in patient cells transduced with the empty vector. (D) Overlay of CD107a expression of transduced T cells kept in medium (dotted line) and (E) stimulated with anti-CD3 (solid line). The difference in mean fluorescence intensity (ΔMFI) of CD107a expression between cells incubated in medium vs stimulated with plate-bound anti-CD3 is shown for patient (Pat) and control (ctr) GFP-positive CD8+ T cells transduced with the indicated vector. Results are shown from 2 independent experiments.