Figure 2.
PRO-001 binds to WT and mutant FGFR3, competes with FGF for FGFR3 binding, and inhibits the growth of B9WT cells. PRO-001 binding to FGFR3 was determined by flow cytometric analysis using a PE-conjugated anti–human secondary antibody. (A) Competition of PRO-001 binding to cell-surface FGFR3 on B9WT cells. The filled histogram indicates parental B9 cells; dotted gray line, B9WT without FGF9; solid line, B9WT in the presence of FGF9. (B) PRO-001 binding to cell-surface WT and mutant FGFR3 on B9 cells. The filled histogram indicates parental cells; thick light gray line, B9Y373C; thick dark gray line, B9K650E; dotted gray line, B9G384D; dotted black line, B9WT; solid black line, B9807C. (C) B9 cells were stimulated with FGF and incubated with increasing concentrations of PRO-001 or 100 nM PD173074 for 48 hours, and cell viability was assessed by MTT-based assay. □ indicates unstimulated; ▪, FGF stimulated; ▧, FGF plus 1 μg/mL PRO-001; , FGF plus 3 μg/mL PRO-001; ▨, FGF plus 5 μg/mL PRO-001; ▨, FGF9 plus 100 nM PD173074. Proliferation index (PI) = (ODd2)/(ODd0), where ODd2 and ODd0 are the optical density (OD) at 48 hours and day 0, respectively. When PI = 1, cells did not proliferate after 48 hours in culture. Values represent mean ± SD of 4 independent experiments.