Lumenal association of HTsol-GFP at Maurer's clefts. (A) Schematic representation of the infected erythrocyte (left) and its permeabilization (dotted lines) after treatment with tetanolysin (top) or saponin (bottom). Panels of fluorescent images show infected erythrocyte expressing HTsol-GFP, permeabilized with tetanolysin (top) or saponin (bottom), and probed with antibodies to GFP (green) and PfStomatin (red). Respective merged images are also shown. Dotted lines indicate erythrocyte periphery. Arrows show intraerythrocytic clefts. (B) 0° projections of an rHT-GFP–loaded erythrocyte ghost infected with 3D7 P falciparum (top) or a mock-loaded erythrocyte ghost infected with transgenic parasite expressing HTsol-GFP (bottom). Empty arrowhead, cleft structure not labeled with intraerythrocytic rHT-GFP; solid arrowhead, GFP labeled cleft. (C) Cells in panel B fixed, permeabilized, and probed with antibodies to GFP (green) and resident cleft protein PfSBP1 (red). Arrows show clefts. (D) Immunoelectron microscopy of cells in panel B showing distribution of GFP associated with Maurer's clefts (MC). Bar indicates 500 nm. (E) Bar graph showing the percentage colocalization between GFP and Maurer's cleft in indicated samples by fluorescence microscopy. (F) Quantitation for the number of gold particles (measuring GFP) associated with clefts by immunoelectron microscopy over 20 infected erythrocytes. In all fluorescence micrographs: p, parasite (nucleus stained with Hoechst 33342; blue); ec, erythrocyte cytosol; bar, 2 μm.