spacer gif spacer gif spacer gif spacer gif spacer gif
QUICK SEARCH:   [advanced]


spacer gif
     Home     Help     Feedback     Subscriptions     Archive     Search     Table of Contents    

Right arrow Help viewing high resolution images
Right arrow Return to article
(Downloading may take up to 30 seconds.
If the slide opens in your browser, select File -> Save As to save it.)
Click on image to view larger version.



Fig. 3. PECAM-1 ligation enhances cell-surface expression of {alpha}6 integrins on mouse blood neutrophils in vitro as quantified by flow cytometry and observed by confocal microscopy. Blood-derived neutrophils incubated for 30 minutes in wells of 96-well plates, coated with BSA (control) or different combinations of PECAM-1, ICAM-1 and IL-8, were assayed for {alpha}6 integrins expression by flow cytometry. The binding of the primary mAb GoH3, relative to the binding of an isotype-matched control mAb, is expressed in terms of relative fluorescence intensity (RFI). (A) Cell-surface expression of {alpha}6 integrins on WT blood neutrophils after adhesion to different proteins and protein combinations. (C) Cell-surface expressions of {alpha}6 integrins on WT neutrophils incubated in wells in the presence or absence of anti-ICAM-1 or anti-ß2 mAbs, and expression on the cell surface of PECAM-1-deficient neutrophils. Results represent means±s.e.m. from three to six samples in each condition using different neutrophil preparations. Asterisks and crosses indicate significant differences from samples incubated in BSA-coated wells: *P<0.05; **P<0.01; ***P<0.001 (A,C), and significant differences from samples incubated in wells coated with PECAM-1, ICAM-1 and IL-8 (total protein being 10 µg ml–1): +P<0.05; +++P<0.001 (C). (B,D) Representative histograms from experiments shown in A,C, with the hatched histograms representing binding of control IgG. Selected samples were also analysed using a confocal laser-scanning microscope (Zeiss LSM 5 Pascal incorporating a 100x oil A-plan objective with a numerical aperture of 1.25) equipped with an argon laser (excitation wavelength of 488 nm). Expression of {alpha}6 integrins was indirectly observed using the mAb GoH3 against {alpha}6 integrins and an Alexa-Fluor-488-conjugated secondary antibody. Representative images of mid-level sections of cells from different conditions are shown. (E) WT neutrophils incubated in BSA-coated wells. (F) WT neutrophils incubated in PECAM-1/ICAM-1/IL-8 (10 µg ml–1)-coated wells. (G) PECAM KO neutrophils incubated in PECAM-1/ICAM-1/IL-8 (10 µg ml–1)-coated wells. The binding of the anti-{alpha}6-integrin mAb under different experimental conditions, corrected for the binding of an isotype-matched control mAb and expressed in terms of mean fluorescence intensity (arbitrary units), is also shown (mean±s.e.m. from three to six samples in each condition using at least three different neutrophil preparations). Bar, 10 µm.





Right arrow Return to article