Release of RGS10 from binding sites on spinophilin leads to a rise in free RGS10 levels in platelets incubated with agonists or PGI₂. (A) Human platelets were incubated for 3 minutes with a PAR1 agonist peptide (SFLLRN 50 µM), a TxA₂ mimetic (U46619 10 µM), ADP (10 µM), or collagen (10 µg/mL) in the absence or presence of 100 μM aspirin (ASA) and 1 U/mL apyrase (APY), as indicated. Lysates were precipitated with anti-RGS10 and probed for spinophilin before reprobing with anti-RGS10 (data are mean ± SEM, N = 3). (B) Human platelets were incubated for 3 minutes with ADP (10 µM) in the absence or presence of 100 μM aspirin (ASA). Lysates were precipitated with anti-RGS10 and probed for spinophilin (SPL) before reprobing with anti-RGS10 (data are mean ± SEM, N = 4). (C) Human platelets were incubated with 20 µM forskolin (Forsk) or 15 µM PGI₂, with or without 1 µM okadaic acid, as indicated. Proteins were precipitated with anti-RGS10 or nonimmune immunoglobulin (Ig) and then probed with anti-spinophilin before reprobing with anti-RGS10 (data mean ± SEM, N = 4). P values are relative to resting platelets. (D) Lysates were prepared from resting platelets and from platelets incubated with PGI₂ (15 µM) or the PAR1 agonist peptide SFLLRN (50 µM). The lysates were then incubated with GST-Gi2α coupled to glutathione beads in the presence of GDP plus AlF₄⁻ or GDP alone, as indicated. Bound proteins were subjected to electrophoresis and probed with anti-RGS10 and Gi2α antibodies to detect RGS10 and GST–Gi2α fusion protein, respectively (upper panels). Summary of 3 experiments expressed as the percentage of the result obtained with resting platelets (data are mean ± SEM) (lower panel). P values are relative to resting platelets.