Leukocyte β2 integrins and CD44 are involved in interaction with SS RBCs. (A,B) Inhibition of PBMC interaction with epi-treated SS RBCs was performed as described in “Inhibition assays.” Results are presented as percentage of adherent PBMCs at a shear stress of 1 dyne/cm2. (A) PBMC adhesion was measured after preincubation of PBMCs with anti-β2 integrin antibody followed by exposure to epi-treated SS RBCs. Error bars show SEM of 3 different experiments. *P < .001 compared with unstimulated PBMCs; **P < .001 compared with PBMCs preincubated with P3. (B) PBMC adhesion was measured after exposure to epi-treated SS RBCs, or epi-treated SS RBCs preincubated with sCD44 or sLW. Error bars show SEM of 4 different experiments. *P < .001 compared with unstimulated PBMCs; **P < .001 compared with PBMCs coincubated with SS RBCs preincubated with sLW, then treated with epi. (C) Phosphorylation of leukocyte CD44. Inorganic 32P radiolabeled intact PBMCs were coincubated or not with sham-treated SS RBCs for 15 minutes or 30 minutes, or with epi-treated SS RBCs for 15 minutes or 30 minutes. Leukocyte CD44 was immunoprecipitated (IP) with anti-CD44 antibody or P3 as a control, as indicated. RBC CD44 was IP from sham-treated SS RBCs with anti-CD44 antibody. The cpm shown are quantitative data of the radioactive band at 85 kDa. One representative experiment is shown (n = 3). (D) Total immunoprecipitates (lanes 1-8) obtained using the same conditions as described in panel C but immunostained with A3D8 mAb against CD44.