Abstract

The lonq term objective of the proposed research is to understand the critical early events in the initiation and regulation of blood platelet function in hemostasis. Evidence is increasing that platelets need to be activated in seconds or fractions of a second to prevent excessive bleeding from rapidly-flowing blood. Biochemical changes, such as an increase in cellular calcium, phospholipid hydrolysis, or phosphorylation of 1 specific proteins, have been detected within 0.5 sec of platelet activation by ADP or thrombin. However, important questions exist as to the regulation and mechanisms leading to platelet """"""""shape change"""""""", aggregation and secretion. Perhaps the most significant platelet activator is ADP, and how it initiates siqnal transduction is not well understood. The sources of necessary intracellular calcium are not clear, or whether phosphatidylinositol hydrolysis is necessarily linked to the early ( 2 sec) major rise in cytoplasmic Ca++. Potential changes in intracellular location of some important enzymes such as protein kinase C, are not known during the first 5 sec after activation, or the functional consequences of such chanqes. Platelet function will be analyzed by a new quenched-flow approach which enables precise control of reaction times down to about 0.1 sec after initiation.
Aims are to test the hypothesis that turnover of phosphatidylinositol is requried for the rapid ( 2 sec) increase in intracellular calcium caused by ADP, in contrast to thrombin. Special interest will be directed to potential ADP-induced lipid hydrolysis and corresponding formation of the cyclic or non-cyclic inositol phosphates. The importance of extracellular Na+ and cyclic GMP in the regulation of rapid calcium fluxes will be assessed. An important member of a new group of four phosphoproteins (185,140 104 and 77 kDa) will be studied, since their kinetics and very early phosphorylation (0.3 sec) are quite distinct from the well-defined 20 and 47 kDa proteins. We will test by immuno-blottinq procedures the hypothesis that the 77 kDa protein is protein kinase or possibly caldesmon, ADP will serve as major agonist, but thrombin will also be used as a classic stimulator of phosphatidylinositol turnover, Lastly, using a new sprayfreezing method coupled to immuno-electromicroscopy, we propose to study the intra- platelet localization-and functional consequences of protein kinase C during the first few seconds after platelet activation.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Heart, Lung, and Blood Institute (NHLBI)
Type
Research Project (R01)
Project #
5R01HL027014-08
Application #
3338864
Study Section
Hematology Subcommittee 2 (HEM)
Project Start
1981-09-01
Project End
1992-06-30
Budget Start
1990-07-01
Budget End
1991-06-30
Support Year
8
Fiscal Year
1990
Total Cost
Indirect Cost

  Institution

Name
University of Virginia
Department
Type
Schools of Medicine
DUNS #
001910777
City
Charlottesville
State
VA
Country
United States
Zip Code
22904

  Publications

Polanowska-Grabowska, R; Gear, A R (2000) Heat-shock proteins and platelet function. Platelets 11:22-Jun
Polanowska-Grabowska, R; Gear, A R (1999) Activation of protein kinase C is required for the stable attachment of adherent platelets to collagen but is not needed for the initial rapid adhesion under flow conditions. Arterioscler Thromb Vasc Biol 19:3044-54
Simon Jr, C G; Holloway, P W; Gear, A R (1999) Exchange of C(16)-ceramide between phospholipid vesicles. Biochemistry 38:14676-82
Simon Jr, C G; Gear, A R (1999) Sphingolipid metabolism during human platelet activation. Thromb Res 94:13-23
Polanowska-Grabowska, R; Simon Jr, C G; Gear, A R (1999) Platelet adhesion to collagen type I, collagen type IV, von Willebrand factor, fibronectin, laminin and fibrinogen: rapid kinetics under shear. Thromb Haemost 81:118-23
Simon Jr, C G; Chatterjee, S; Gear, A R (1998) Sphingomyelinase activity in human platelets. Thromb Res 90:155-61
Simon Jr, C G; Gear, A R (1998) Membrane-destabilizing properties of C2-ceramide may be responsible for its ability to inhibit platelet aggregation. Biochemistry 37:2059-69
Polanowska-Grabowska, R; Simon Jr, C G; Falchetto, R et al. (1997) Platelet adhesion to collagen under flow causes dissociation of a phosphoprotein complex of heat-shock proteins and protein phosphatase 1. Blood 90:1516-26
Polanowska-Grabowska, R; Gear, A R (1994) Role of cyclic nucleotides in rapid platelet adhesion to collagen. Blood 83:2508-15
Gear, A R (1994) Platelet adhesion, shape change, and aggregation: rapid initiation and signal transduction events. Can J Physiol Pharmacol 72:285-94

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