Inhibition assay to define the spatial relationship between the peptide-specific epitopes and the rituximab antigen-combining site. (A) Fifty microliters of a PBS solution containing 2-fold serial dilutions of Rp1-L (♦), Rp5-L (▴), Rp15-C (○), Rp3-C (▵), mRp3-C (□), and RpCD20-L (▪) was mixed with an equal volume of an appropriate dilution of biotinylated rituximab. After 2-hour incubation at 4 °C, the mixture was added to target Raji cells (7 × 10⁵ cells/well) and their binding to rituximab was detected with HRP-avidin. Binding of rituximab in the presence of unlabeled rituximab (+), infliximab (•), and peptide Qp1a (×) were included as specificity controls. Results are expressed as percentage inhibition of binding compared with binding in the absence of inhibitor. (B) One microliter of PBS solution containing 10-fold serial dilution of Rp1-L (♦), Rp5-L (▴), and Rp15-C (○; starting concentration 1 mg/mL) was mixed with 9 μL PBS solution containing rituximab (500 ng/mL). After 1-hour incubation at 4°C, the mixture was added to Raji cells (1 × 10⁴ cells/well). Following 30-minute incubation at 25°C, an appropriate dilution of rabbit complement was added to each well and the assay was continued as described in “CDC assay.” Lysis mediated by rituximab in the presence of infliximab F(ab′)₂ (•) and mAb HC-10-specific peptide Qp1a (□) was included as negative control. Lysis mediated by rituximab in the presence of rituximab F(ab′)₂ (+) was used as positive control.