Fig. 2.
Fig. 2. Distribution of SNAP-23 in platelets. / (A) Platelets were disrupted by freeze-thaw cycles and fractionated into a soluble fraction (S1) and pellet by ultracentrifugation. The pellet was incubated with 1 mol/L KCl on ice for 30 minutes. The supernatant (S2) was collected, and the resulting pellet was either solubilized with 1% Triton X-100 in PBS or washed again with 200 mmol/L Na2CO3 for 30 minutes. The supernatants (Triton-soluble, Stx; and carbonate-released, Sc) were collected and the pellets (Ptx and Pc) were resuspended in SDS-loading buffer. All of the above fractions were subjected to western blotting using ab23 and anti–syntaxin 4 antibody. Based on comparison with the starting material, approximately 38.2%, 16.5%, 33.5%, 31.1%, 14.2%, and 8.5% of the total platelet protein was in S1, S2, Sc, Stx, Ptx, and Pc, respectively. (B) The initial soluble and membrane fractions from A were incubated with 1% Triton X-114 for 30 minutes on ice. The aqueous and detergent phases were separated by warming the samples to 37°C, followed by centrifugation. The aqueous and detergent phases of both the soluble fraction and membrane pellet as well as the Triton X-114–insoluble pellet were analyzed by western blotting using ab23 and anti–syntaxin 4 antibody. His6–SNAP-23 was also subjected to Triton X-114 partitioning, and the aqueous and detergent phases were analyzed by western blotting using ab23. (C) Soluble SNAP-23 is released from platelets after the treatment with 0.8 U/mL SLO. Platelets (108) were treated with 0.8 U/mL SLO for 10 minutes and then pelleted by centrifugation. The supernatant (S) and the pellet (P) were subjected to western blotting with ab23 and anti–syntaxin 4.

Distribution of SNAP-23 in platelets.

(A) Platelets were disrupted by freeze-thaw cycles and fractionated into a soluble fraction (S1) and pellet by ultracentrifugation. The pellet was incubated with 1 mol/L KCl on ice for 30 minutes. The supernatant (S2) was collected, and the resulting pellet was either solubilized with 1% Triton X-100 in PBS or washed again with 200 mmol/L Na2CO3 for 30 minutes. The supernatants (Triton-soluble, Stx; and carbonate-released, Sc) were collected and the pellets (Ptx and Pc) were resuspended in SDS-loading buffer. All of the above fractions were subjected to western blotting using ab23 and anti–syntaxin 4 antibody. Based on comparison with the starting material, approximately 38.2%, 16.5%, 33.5%, 31.1%, 14.2%, and 8.5% of the total platelet protein was in S1, S2, Sc, Stx, Ptx, and Pc, respectively. (B) The initial soluble and membrane fractions from A were incubated with 1% Triton X-114 for 30 minutes on ice. The aqueous and detergent phases were separated by warming the samples to 37°C, followed by centrifugation. The aqueous and detergent phases of both the soluble fraction and membrane pellet as well as the Triton X-114–insoluble pellet were analyzed by western blotting using ab23 and anti–syntaxin 4 antibody. His6–SNAP-23 was also subjected to Triton X-114 partitioning, and the aqueous and detergent phases were analyzed by western blotting using ab23. (C) Soluble SNAP-23 is released from platelets after the treatment with 0.8 U/mL SLO. Platelets (108) were treated with 0.8 U/mL SLO for 10 minutes and then pelleted by centrifugation. The supernatant (S) and the pellet (P) were subjected to western blotting with ab23 and anti–syntaxin 4.

Close Modal
This Feature Is Available To Subscribers Only

or Create an Account

Close Modal
Close Modal