ACTIVATION OF CALPAIN-I IN THROMBIN-STIMULATED PLATELETS IS REGULATED BY THE INITIAL ELEVATION OF THE CYTOSOLIC CA2+ CONCENTRATION

The source and concentration of Ca2+ required to activate calpain I were investigated in thrombin-stimulated platelets. The concentration of cytosolic free Ca2+ ([Ca2+]i) was measured in platelets containing fura-2-AM, and exhibited a biphasic response after stimulation with 0.05, 0.1 or 0.5 NIH units of thrombin/ml. An initial transient elevation, which was predominantly dependent upon Ca2+ released from the internal stores into the cytosol, peaked at 15 s after stimulation, and a secondary sustained elevation, which was due to Ca2+ influx, was observed following the initial elevation. Calpain I was present at about 540 ng/ 10(8) unstimulated platelets, as measured by immunoblotting using rabbit anti-(human calpain I) IgG. Calpain I was activated 10 s after thrombin stimulation, as determined by the appearance of the 78 kDa and 76 kDa forms on immunoblots. The activation ratio of calpain I was calculated as the amount of the 78 + 76 kDa forms as a percentage of the total (80 + 78 + 76 kDa), and was influenced by the extent of the initial transient [Ca2+]i elevation after stimulation. An initial increase in [Ca2+]i of 300 nm was required to achieve the maximal activation (60 %) of calpain 1, and half-maximal activation occurred at 160 nm-[Ca2+]i. These results suggest that the activation of calpain I in platelets is regulated by the initial elevation in [Ca2+]i after thrombin stimulation, and does not necessarily require a Ca2+ influx.