Abstract

The goal of this research is to understand, at the molecular level, how blood coagulation is regulated by serine protease inhibitors. The role of heparin and other glycosaminoglycans (GAGs), procoagulant cofactor proteins, divalent metal ions and GAG- binding proteins is modulating the rate of neutralization of blood coagulation-proteases by antithrombin III and other inhibitors will be investigated by rapid kinetic and equilibrium binding studies. Whether heparin and other modulators promote the initial encounter of protease and inhibitor or alter the limiting rate of protease neutralization and whether these effects are mediated by induced protein conformational changes will be evaluated. Inhibitors and proteases modified chemically or by natural mutation will serve as probes of the mechanism of action of GAG and other effectors on inhibitor/protease reactions. The enhancement by heparin and possibly other GAGs of inhibitor turnover and inactivation by proteases during their neutralization, and the modulation of this reaction by effectors, will be investigated as a potential regulatory mechanism for protection of these proteases from neutralization. Whether this reaction reflects a mechanism in which the protease is trapped by an inhibitor conformational change during turnover of the inhibitor as a normal protease substrate, will be elucidated. These studies will employ fluorescence or absorbance probes to quantitate interactions between proteins, GAGs and metal ions, as well as reactions between inhibitors and their target proteases in the presence and absence of modulators. Quantitative affinity chromatography studies of binding interactions and direct monitoring of inhibitor/protease kinetics by residual protease activity will serve to validate probes as signals for these interactions and reactions. These studies should enable us to determine what limits the rate at which inhibitors can neutralize their target proteases under physiological conditions and will provide a basis for evaluating the relative importance of in vivo regulation of each protease as well as the potential role of GAGs on the vascular endothelium or in the extravascular space in this regulation.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Heart, Lung, and Blood Institute (NHLBI)
Type
First Independent Research Support & Transition (FIRST) Awards (R29)
Project #
5R29HL039888-05
Application #
3471849
Study Section
Hematology Subcommittee 2 (HEM)
Project Start
1988-04-01
Project End
1993-03-31
Budget Start
1992-04-01
Budget End
1993-03-31
Support Year
5
Fiscal Year
1992
Total Cost
Indirect Cost

  Institution

Name
Henry Ford Health System
Department
Type
DUNS #
073134603
City
Detroit
State
MI
Country
United States
Zip Code
48202

  Publications

Yang, Likui; Ding, Qiulan; Huang, Xin et al. (2012) Characterization of the heparin-binding site of the protein z-dependent protease inhibitor. Biochemistry 51:4078-85
Huang, Xin; Rezaie, Alireza R; Broze Jr, George J et al. (2011) Heparin is a major activator of the anticoagulant serpin, protein Z-dependent protease inhibitor. J Biol Chem 286:8740-51
Richard, Benjamin; Swanson, Richard; Olson, Steven T (2009) The signature 3-O-sulfo group of the anticoagulant heparin sequence is critical for heparin binding to antithrombin but is not required for allosteric activation. J Biol Chem 284:27054-64
Gettins, Peter G W; Olson, Steven T (2009) Activation of antithrombin as a factor IXa and Xa inhibitor involves mitigation of repression rather than positive enhancement. FEBS Lett 583:3397-400
Gettins, Peter G W; Olson, Steven T (2009) Exosite determinants of serpin specificity. J Biol Chem 284:20441-5