Figure 5
Figure 5. Correlation of homotypic adhesion, actin reorganization, and lysosomal involvement to cell death evoked by the bispecific anti-CD20/CD74 HexAbs. (A) JeKo-1 cells were pretreated or not pretreated with the actin polymerization inhibitor, latrunculin B (1μM), for 2 hours followed by addition of HexAbs or both parental mAbs and evaluated for aggregation after 4 hours by light microscopy. (B) Apoptosis induced by HexAbs was reduced significantly (P < .025) in JeKo-1 with 1μM cytochalasin D (CsD), another inhibitor of actin polymerization. Error bars represent SD; n = 3. (C) Lysosomal V ATPase inhibitors, concanamycin A (Con A) and bafilomycin A1 (Bfa1), inhibited the apoptosis induced by HexAbs in JeKo-1 cells. (D) HexAbs induced changes in lysosomal volumes as determined by staining the cells with LysoTracker (75nM). The lysosomal compartmental volume changes were analyzed for JeKo-1 cells (top panel) and Granta-519 (bottom panel) by flow cytometry as enhanced binding and shift in the emission spectrum toward the right. (E) Immunofluorescence analysis of cathepsin B staining (red) 48 hours after treatment with select Abs. Nuclei were stained with DAPI (blue).

Correlation of homotypic adhesion, actin reorganization, and lysosomal involvement to cell death evoked by the bispecific anti-CD20/CD74 HexAbs. (A) JeKo-1 cells were pretreated or not pretreated with the actin polymerization inhibitor, latrunculin B (1μM), for 2 hours followed by addition of HexAbs or both parental mAbs and evaluated for aggregation after 4 hours by light microscopy. (B) Apoptosis induced by HexAbs was reduced significantly (P < .025) in JeKo-1 with 1μM cytochalasin D (CsD), another inhibitor of actin polymerization. Error bars represent SD; n = 3. (C) Lysosomal V ATPase inhibitors, concanamycin A (Con A) and bafilomycin A1 (Bfa1), inhibited the apoptosis induced by HexAbs in JeKo-1 cells. (D) HexAbs induced changes in lysosomal volumes as determined by staining the cells with LysoTracker (75nM). The lysosomal compartmental volume changes were analyzed for JeKo-1 cells (top panel) and Granta-519 (bottom panel) by flow cytometry as enhanced binding and shift in the emission spectrum toward the right. (E) Immunofluorescence analysis of cathepsin B staining (red) 48 hours after treatment with select Abs. Nuclei were stained with DAPI (blue).

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