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First published online 6 September 2005
doi: 10.1242/jcs.02551

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The leading edge is a lipid diffusion barrier

¹ Max Planck Institute of Molecular Cell Biology and Genetics, Pfotenhauerstr. 107, 01307 Dresden, Germany
² Max Planck Institute of Biochemistry, Am Klopferspitz 18, 82152 Martinsried, Germany

View larger version (11K): [in a new window]   Fig. 1. Schematic diagram of focal labeling and observation of initial diffusion (FLOID). (a) The cell body is lightly touched by a micro-needle containing carbocyanine dye. (b) Epi-illumination shows dye spreading in both dorsal and ventral cell membranes. The shortest diffusion path from the labeling point to the leading edge is via the dorsal membrane. (C) TIRF illumination shows only the ventral cell membrane.

View larger version (37K): [in a new window]   Fig. 2. FLOID analysis of migrating keratocytes. TIRF images (a and b) show the location in which dye has spread from the dorsal to ventral cell surface; either at the back of the cell only (single peak, a and c) or both at the front and back (double peak, b and d). Undulations in the ventral cell surface have been shown previously using interference reflection microscopy (Anderson and Cross, 2000), and lead to variations in dye excitation according to the distance of the cell surface from the coverslip. White bars (a and b) show the position used for fluorescence intensity scans in c and d, respectively. Arrowhead (b) indicates a region of reduced protrusion at the leading edge, where dye has spread from the dorsal to ventral cell membrane. Comparison of sequentially acquired epi-fluorescent (f) and TIRF (g) images from the same cell, and the overlay (h). Note that TIRF proceeds epi-fluorescent illumination by 750 milliseconds. The white bar (h) shows the position used for fluorescence intensity scans in i. (i) The epi-fluorescence intensity scan (green line) indicates that dye has spread from the back of the cell toward the front, and begun to accumulate at the leading edge (arrowhead). The TIRF intensity scan (red line) also shows that dye has spread from the back of the cell toward the front, but not yet reached the leading edge. Note that accumulated dye in the dorsal membrane has not spread around the leading edge to the ventral surface. Inset shows profile for the whole cell. 86% of cells analyzed (n=138) were found to show the single-peak intensity profile (e). Bars, 10 µm.

View larger version (55K): [in a new window]   Fig. 3. Keratocytes stained with Alexa-488 phalloidin to reveal F-actin distribution after (a) no treatment, (b) extraction of membrane cholesterol with CD, (c) treatment with CA to stop motility, and (d) CA/CB treatment to depolymerise the actin meshwork. The fluorescence intensity of phalloidin stain was reduced by 25% in CD-treated cells compared with controls. Fluorescence intensities cannot be compared directly in these images because they are displayed on different contrast scales. Bars, 5 µm.

View larger version (18K): [in a new window]   Fig. 4. Number of cells showing blocked dye diffusion at the leading edge (single peak intensity scan) under different labelling conditions. (a) CA treatment reduced the fraction of single peak cells from 86% (n=138) to 51% (n=45). CA/CB treatment further reduced this value to 4% (n=49). (b) The diffusion of carbocyanine dyes that have different acyl chain lengths was equally inhibited during protrusion at the leading edge. Extraction of 35% of cholesterol by CD treatment marginally reduced the fraction of single peak cells from 86% to 75% (n=36).