The understanding of the role of metal ions in blood coagulation has been a
long term goal of this laboratory. To further the understanding of the
structure-function relationships of the Gamma-carboxyglutamic acid residues
in prothrombin to the metal liganding processes of the protein we will
study a naturally occurring variant of prothrombin which contains only
three Gamma-carboxyglutamic acid residues. Normal prothrombin contains ten
Gamma-carboxyglutamic acid residues. We will correlate the sequence
position of the Gamma-carboxyglutamic acid residues in the variant with its
metal binding and conformational properties using amino acid sequence
analysis, state rate dialysis, fluorescence spectroscopy and conformation
specific antibodies. The results of these analyses will be used to compare
and contrast the properties of normal prothrombin and the variant
prothrombin. Platelets secrete Ca(II) upon activation. There is potential
for a significant increase in Ca(II) concentration at the site of platelet
plug formation. In addition, Ca(II) dependent conversion of several plasma
zymogens may occur on the platelet surface. We will use monoclonal
conformation specific antibodies to identify platelet surface antigens
whose conformations are altered depending on the presence or absence of
metal ligands. We will correlate the presence of the antigen to the status
of the platelet (native or activated). We will identify a possible
receptor function for the platelet surface antigens recognized by these
monoclonal antibodies. Finally we have identified a novel cleavage product
of human prothrombin in plasma, fragment 1.2.3. We will access a potential
regulatory role for this fragment in hemostasis. There is currently
heightened interest in understanding the processes that regulate hemostasis
and thrombosis. The studies outlined in this proposal address these
biologically interesting and medically important questions.
No Sub Projects information available for 4R37HL018834-19
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