PIP₃ distribution in chemotaxing neutrophils. (A) PIP₃ immunolocalization to leading edge is disrupted in Rac1 null neutrophils. Immunolocalization of PIP₃ was carried out and analyzed as described in “Materials and methods.” Representative images demonstrate the PIP₃ localization toward the leading edge in wild-type and Rac2 null neutrophils but not in Rac1 null cells. (B) Immunoblot analysis of phospho-Akt levels in neutrophils. Representative immunoblot of Akt and phospho-Akt levels in peritoneal neutrophils. Neutrophils were isolated from bone marrow as described. Blot is representative of 4 separate experiments that all demonstrate decreased phospho-Akt levels in Rac1 and Rac1/2 null neutrophils compared to wild-type and Rac2 null neutrophils. (C) Immunolocalization of phospho-Akt to the leading edge requires Rac1. Immunolocalization of phospho-Akt, was carried out and analyzed as described in “Materials and methods.” Representative images demonstrate phospho-Akt localization toward the leading edge in wild-type and Rac2 null neutrophils but not in Rac1 null cells. ^*Leading edge. (D) Quantification of mean phospho-Akt–related fluorescence intensity at the leading edge, in the cytoplasm, and in the tail was carried out as described in “Materials and methods.” These data clearly confirm that p-AKT levels are high at the leading edge in both wild-type and Rac2 null neutrophils but decreased in Rac1 null cells. (The leading edge of Rac1 was different from both wild-type and Rac2 null at the P < .05 level.) Scale bar equals 5 μm. Error bars represent standard error of the means.