(A) Graphic of the agonistic effect induced by anti-DCIR mAbs. (B and C) WT and huDCIR transfected HEK293 cells were treated with anti-DCIR mAbs (10 μg/mL) for 30 minutes, followed by immunoprecipitation assay (IP) with anti-phosphorylated tyrosine (B) or anti-SHP2 (C) antibodies. DCIR levels were analyzed by WB and quantitated by densitometry. Representative data from 2 independent studies are shown. (D) Illustration of the huDCIR agonistic effect reporter cell generation. HEK293 cell was cotransfected with a huDCIR vector containing an ITAM motif cloned from Dectin-1 and a luciferase reporter vector with NF-кB response element. (E) Reporter cells as described in D were treated with 10 μg/mL anti-DCIR mAbs or isotype control for 30 minutes, followed by luciferase assay analysis. Agonistic effects induced by the antibodies were quantitated by the luminescent signal. (F) Reporter cells as described in D were treated with a serial dilution of agonistic or nonagonistic anti-DCIR antibodies or isotype control for 30 minutes, followed by luciferase assay analysis. Dose-dependent induction of agonistic signaling was quantitated by the luminescent signal. (G and H) DCIR ligands, mannose and asialo-biantennary N-glycan (NA2-glycan), were conjugated with BSA and immobilized on culture plates. Dose-dependent agonistic effects of mannose-BSA and NA2 glycan-BSA were determined by the reporter system as described in D. (I) In total, 50 μg/mL of mannose-BSA and NA2 glycan-BSA were coated on the cell culture plate and cultured with HEK293 cells contain the huDCIR-agonist reporter for 6 hours. Agonistic effects induced by anti-DCIR antibody (9D9) were determined by luciferase assay after overnight culture. (E–I) Representative data from 2 independent studies are shown. Means ± SEM from triplicates are shown.