(A) Light microscopy images of May-Grünwald–stained untreated or IM-treated K562 cells. Cells were cultured for 36 hours in the absence or presence of 2 μM IM and processed for May-Grünwald staining. Original magnification, ×40. (B and C) Reduced size of IM-treated K562 cells. The size of K562 cells treated with zVAD, IM, or IM and zVAD was analyzed using a cytofluorimeter. Representative dot plots of physical parameters forward light scatter-height/side light scatter-height (FSC-H/SSC-H) are shown. The yellow arrows indicate a subpopulation of smaller and denser cells in IM/zVAD-treated cultures, while the black arrow shows dying cells after treatment with IM only. Large boxes indicate viable cells; small box indicates denser cells appearing upon IM/zVAD treatment. (C) Representative histograms of the forward light scatter-height parameter are shown. (D) Accumulation of autophagosome-associated LC3-II in IM-treated K562 cells. The Western blot shows endogenous LC3-I and LC3-II levels (upper panel) or ectopic EGFP–LC3-I and EGFP–LC3-II expression (lower panel) in extracts from untreated (control) or IM-treated cells (at 6 and 12 hours). The asterisk indicates that bands are not specific for LC3 (lower panel). Actin was measured as loading control. (E) Formation of LC3-positive vesicles in IM-treated EGFP-LC3–transduced K562 cells. EGFP-LC3 K562 cells were cultured in the presence or absence of IM and stained with anti-LC3 antibody (red). Nuclei were counterstained with DAPI. Scale bar: 10 μm.