Figure 1
Figure 1. Freshly isolated platelets extend projections with distinct cell bodies. (A) Localization of actin (green, phalloidin) in human platelets that were fixed immediately after isolation (Baseline) or after 6 hours in suspension (Cultured). The bottom row displays corresponding transmission images. This figure is representative of more than 20 independent experiments. Scale bars represent 5 μm. (B) Lower magnification of freshly isolated platelets that were stained for actin at baseline or after they were cultured for 6 hours (scale bars, 10 μm). Panel is representative of more than 20 experiments. (C) The bar graph indicates the number of extended platelets with at least 2 cell bodies per microliter of culture media (mean ± SEM; n = 13). *P < .05, baseline versus cultured. (D) Two separate cultures of platelets were labeled (blue or green) and then incubated with one another for 6 hours. Left and right panels: 2 independent experiments, which are representative of 3. (E) Platelets were loaded into “parked” microdrops and examined at baseline or after 6 hours (Cultured). The thin arrows point to single platelets (Baseline) or the same platelet that formed 2 distinct cell bodies after 6 hours (Cultured). The thick arrows point to unique landmarks for each position in the microfluidic device. (F) Sequential images of platelets using low-resolution wide-field microscopy. The arrows highlight the location of the platelets within each drop during the course of the experiment and the formation of 2 distinct cell bodies after 6 hours (far right panels). Distance between the white brackets (E-F, far left panels) is 50 μm.

Freshly isolated platelets extend projections with distinct cell bodies. (A) Localization of actin (green, phalloidin) in human platelets that were fixed immediately after isolation (Baseline) or after 6 hours in suspension (Cultured). The bottom row displays corresponding transmission images. This figure is representative of more than 20 independent experiments. Scale bars represent 5 μm. (B) Lower magnification of freshly isolated platelets that were stained for actin at baseline or after they were cultured for 6 hours (scale bars, 10 μm). Panel is representative of more than 20 experiments. (C) The bar graph indicates the number of extended platelets with at least 2 cell bodies per microliter of culture media (mean ± SEM; n = 13). *P < .05, baseline versus cultured. (D) Two separate cultures of platelets were labeled (blue or green) and then incubated with one another for 6 hours. Left and right panels: 2 independent experiments, which are representative of 3. (E) Platelets were loaded into “parked” microdrops and examined at baseline or after 6 hours (Cultured). The thin arrows point to single platelets (Baseline) or the same platelet that formed 2 distinct cell bodies after 6 hours (Cultured). The thick arrows point to unique landmarks for each position in the microfluidic device. (F) Sequential images of platelets using low-resolution wide-field microscopy. The arrows highlight the location of the platelets within each drop during the course of the experiment and the formation of 2 distinct cell bodies after 6 hours (far right panels). Distance between the white brackets (E-F, far left panels) is 50 μm.

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