Protein S is a cofactor for activated protein C neutralization of an inhibitor of plasminogen activation released from platelets

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Abstract

Platelets stimulated with thrombin release an inhibitor of plasminogen activator (PAI), which has been shown previously to be neutralized by activated protein C (APC). The requirements for optimal neutralization of PAI activity were investigated. The releasate of gel-filtered human platelets stimulated with thrombin served as a source of PAI. When 6 x 108 platelets/mL were incubated with thrombin (1 IU/mL), the releasate contained 18 to 26 ng/mL PAI as determined by incubation of the releasate with urokinase and measurement of residual urokinase activity on plasminogen (S2251). Preincubation of PAI with up to 4 μg/mL APC for two hours yielded less than 20% neutralization of PAI activity. In the presence of protein S, phospholipid, and Ca2+, neutralization of PAI activity was time-dependent with 50% neutralization occurring in two hours with 1 μg/mL APC. The cofactor effects of protein S and phospholipid were concentration-dependent with half-maximal acceleration at approximately 3 μg/mL protein S and 10 μg/mL phospholipid when the experiments were performed at 1 μg/mL APC. Diisopropylfluorophosphate-inactivated APC, gla-domainless APC, and thrombin-cleaved protein S had no effect on PAI activity, indicating requirement for preservation of the APC active site and of the Ca2+ binding ability of both APC and protein S. These results suggest coordinate binding of APC and protein S onto phospholipid membrane as a prerequisite for optimal expression of PAI neutralized by APC.

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D’Angelo, A., Lockhart, M. S., D’Angelo, S. V., & Taylor, F. B. (1987). Protein S is a cofactor for activated protein C neutralization of an inhibitor of plasminogen activation released from platelets. Blood, 69(1), 231–237. https://doi.org/10.1182/blood.v69.1.231.231

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