Figure 3
Figure 3. Confocal immunodetection of TF and GPIbα in human, nonpermeabilized platelets. After fixation, blockade of nonspecific binding sites, and overnight incubation at 4°C, EDTA-PGE1 platelets were immunolabeled with polyclonal anti-TF and/or α-GPIbα (α-CD42b, clone SZ2; Immunotech, Westbrook, ME). For TF, incubation with rabbit anti-sheep IgG was required before incubating with the appropriate FITC antibody. Alexa 555 (Invitrogen) was used to visualize the GPIbα. Top row shows, from left to right: nonstimulated, freshly prepared platelets labeled for TF, GPIbα, and merge imaging. Bottom row shows an aliquot of the same sample stimulated with TRAP and collagen for 2 hours. A striking enhancement of both labels is noticed with a significant increase in the colocalization of both proteins. No leukocytes were observed in all the experiments.

Confocal immunodetection of TF and GPIbα in human, nonpermeabilized platelets. After fixation, blockade of nonspecific binding sites, and overnight incubation at 4°C, EDTA-PGE1 platelets were immunolabeled with polyclonal anti-TF and/or α-GPIbα (α-CD42b, clone SZ2; Immunotech, Westbrook, ME). For TF, incubation with rabbit anti-sheep IgG was required before incubating with the appropriate FITC antibody. Alexa 555 (Invitrogen) was used to visualize the GPIbα. Top row shows, from left to right: nonstimulated, freshly prepared platelets labeled for TF, GPIbα, and merge imaging. Bottom row shows an aliquot of the same sample stimulated with TRAP and collagen for 2 hours. A striking enhancement of both labels is noticed with a significant increase in the colocalization of both proteins. No leukocytes were observed in all the experiments.

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