Figure 2
Figure 2. PI3Kβ is required for incorporation of new platelets into an existing thrombus under high shear rate in mice and humans. (A) Unlabeled whole blood from p110βflox/flox control (WT) mice were perfused through a collagen-coated microcapillary at 500 seconds−1. Control blood was then replaced by DIOC6-labeled platelets in whole blood from p110βflox/flox control (WT) or PF4-Cre/p110βflox/flox (p110βnull) mice and was perfused at a high shear rate (4000 seconds−1). Surface covered (%) by fluorescent platelets (1 minute, 4000 seconds−1) was then analyzed using ImageJ software. Results shown are mean ± SEM of 5 experiments. Student t test, ***P < .001. Representative images at the end of the high shear rate are shown for both genotypes. Scale bar, 20 µm. (B) Unlabeled human platelets in whole blood were perfused through a collagen-coated microcapillary at 1500 seconds−1. Control blood was then replaced by DIOC6-labeled human whole blood treated or not with the PI3Kβ inhibitor AZD6482 and perfused at a high shear rate (4000 seconds−1). Surface covered (%) by fluorescent platelets (2 minutes, 4000 seconds−1) was then analyzed using ImageJ software. Results shown are mean ± SEM of 5 experiments. Student t test, ***P < .001. Representative images at the end of the high shear rate are shown for both conditions. Scale bar, 20 µm.

PI3Kβ is required for incorporation of new platelets into an existing thrombus under high shear rate in mice and humans. (A) Unlabeled whole blood from p110βflox/flox control (WT) mice were perfused through a collagen-coated microcapillary at 500 seconds−1. Control blood was then replaced by DIOC6-labeled platelets in whole blood from p110βflox/flox control (WT) or PF4-Cre/p110βflox/flox (p110βnull) mice and was perfused at a high shear rate (4000 seconds−1). Surface covered (%) by fluorescent platelets (1 minute, 4000 seconds−1) was then analyzed using ImageJ software. Results shown are mean ± SEM of 5 experiments. Student t test, ***P < .001. Representative images at the end of the high shear rate are shown for both genotypes. Scale bar, 20 µm. (B) Unlabeled human platelets in whole blood were perfused through a collagen-coated microcapillary at 1500 seconds−1. Control blood was then replaced by DIOC6-labeled human whole blood treated or not with the PI3Kβ inhibitor AZD6482 and perfused at a high shear rate (4000 seconds−1). Surface covered (%) by fluorescent platelets (2 minutes, 4000 seconds−1) was then analyzed using ImageJ software. Results shown are mean ± SEM of 5 experiments. Student t test, ***P < .001. Representative images at the end of the high shear rate are shown for both conditions. Scale bar, 20 µm.

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