Brief Overview of Regulation of Hemostasis by Serpins and Two On-going Vascular Biology Projects in the Laboratory

 

Introduction: Hemostasis is described as the balance between procoagulant and anticoagulant forces that act in concert to maintain the fluidity of blood under physiologic conditions.  This system responds rapidly to vascular injury via the coagulation cascade, whose primary role is to prevent the flow of blood from the vasculature.  When a vessel is injured, hemostasis is achieved by several mechanisms, including vessel spasm, formation of a platelet plug, blood coagulation, and eventual healing of the injured area.  Platelets adhere to extracellular matrix proteins that are exposed from damaged blood vessel endothelial cells, and then become activated and secrete factors that attract and activate nearby platelets.  The coagulation “cascade” is activated both by factors exposed on and secreted from the injured tissues and platelets.  These events ultimately result in the formation of fibrin threads that enmesh platelets, blood cells, and plasma proteins to form the hemostatic plug or thrombus.  If left unchecked, the clotting cascade would result in widespread thrombosis and vessel blockage; thus “anticoagulant” pathways are also immediately activated that regulate the activities of procoagulant factors.

Regulation of Blood Coagulation by Antithrombin (AT), Heparin Cofactor II (HCII), Protein C Inhibitor (PCI) and Plasminogen Activator Inhibitor-1 (PAI-1):   The majority of coagulation proteases are inhibited by two serpins, antithrombin (AT; systematic name SERPINC1) and heparin cofactor II (HCII; systematic name SERPIND1).  The serpin-protease complexes are then cleared from the plasma by the non-specific low-density lipoprotein receptor related protein found on hepatocytes.  AT inhibits thrombin, factors IXa, Xa, XIa, XIIa, kallikrein, and plasmin.  However, a comparison of the inhibition rates indicates that only the reactions with thrombin, factor Xa, and factor IXa are physiologically important.  Thrombin is the only coagulation protease that HCII inhibits.  Target protease inhibition by AT and HCII is greatly accelerated by glycosaminoglycans, such as heparin and heparan sulfate.  The anticoagulant effect of commercial heparin is based upon its ability to accelerate the inhibition of thrombin, factor Xa, and factor IXa by AT.  In vivo, heparan sulfate-containing proteoglycans that are localized to the endothelial cell membrane serve to accelerate this reaction.  HCII inhibition of thrombin is also accelerated by dermatan sulfate and dermatan sulfate-containing proteoglycans, which are localized on the plasma membranes of extravascular cells.  Thus, it is postulated that HCII plays an important role in the regulation of thrombin activity in the extravasculature.  Additionally, both protein C inhibitor and plasminogen activator inhibitor-1/vitronectin can also inhibit thrombin, although the physiological relevance of these serpin-thrombin inhibition reactions is not clear.



Protein C System and the Role of APC in Cell Migration/Invasion:  Once activated in the coagulation pathway, thrombin can proceed down one of several pathways.  It can continue to cleave fibrinogen and activate Factor V and Factor VIII, thus stimulating clot formation, or it can bind to thrombomodulin (TM).  TM is a membrane bound protein on the surface of endothelial cells.  Thrombin now recognizes another zymogen of a serine protease, protein C, as a substrate.  Zymogen protein C binds to endothelial cell protein C receptor (EPCR).  Thrombin-TM can then activate protein C bound to EPCR.  Activated protein C (APC) requires protein S as a cofactor for full activity.  APC specifically cleaves the two cofactors involved in thrombin generation, Factor Va and Factor VIIIa.  The destruction of these essential cofactors results in cessation of thrombin generation, and thus helps stop thrombus formation.  The importance of this pathway is apparent in the discovery of familial thrombophilia due to the Factor V Leiden mutation.  We are trying to better understand the process by which PCI and PAI-1/VN regulate the protein C system proteases, and to refine their inhibition mechanism by directly looking at assay systems with phospholipids and with endothelial cells that generate both thrombin and APC.  Interestingly, APC has other activities beyond its role as an anticoagulant protease.  APC is currently being used to treat sepsis to replace decreased APC levels, e.g., in children with severe meningococcal sepsis.  Yet the mechanism of how APC achieves this anti-inflammatory role is just beginning to be understood.  Three groups have recently analyzed various gene chip arrays and have identified several anti-inflammatory genes that are up or down regulated on vascular endothelium following incubation of APC with cells.  Joyce et al found that APC directly down-regulated major gene in a pattern of anti-inflammatory and cell survival pathways.  Riewald et al. reported that the major anti-inflammatory effect of APC was due to activation of the classic thrombin receptor PAR-1 (protease activated receptor-1), dependent on APC being bound to EPCR.  We are currently studying the effect of the protein C system in cellular migration and invasion using various cell types, and we are working on the molecular mechanism of this interaction of APC with cell surface receptors.  Furthermore, we are characterizing the role of serpins to down-regulate the migration/invasion response, and the signaling pathways promoted by APC-cell interactions.


Localization of Heparin Cofactor II in Atherosclerotic Lesions: The role of HCII in atherosclerosis is poorly understood, we and others have explored the occurrence of HCII and other serpins in normal and diseased vessels, we and others have characterized DSPG/HSPG from these diseased lesions compared to normal artery wall and found as the disease progressed the character of the GAG changed to be less effective at catalyzing thrombin inhibition by HCII.  Thus, we initiated this project to further explore the occurrence of HCII compared to AT.  Multiple microscopic sections from 33 individual cases of human left anterior descending (LAD) coronary artery with some degree of atherosclerosis were obtained from the Pathobiological Determinants of Atherosclerosis in Youth (PDAY) Study.  Liver sections obtained from Surgical Pathology at the University of North Carolina were used as positive controls because both HCII and AT are synthesized in the liver and therefore should be detectable using immunohistochemistry (these results are not shown).  All subjects in this study were persons from the ages of 15-34 who died of external causes (accidents, homicides, suicides) from fifteen cooperating centers managed by the Department of Pathology at Louisiana State University Health Science Center.  Data from each case was recorded in a database for analysis including, age, gender, race, total cholesterol and high-density cholesterol (HDLC) and this long-term study was termed PDAY.

Each case was probed for the presence of heparin cofactor II (HCII) or antithrombin (AT).  Liver slides for each run were subjected to the exact same conditions as the LAD slides being probed.  HCII antigen was detected by first incubating with goat anti-human HCII affinity purified polyclonal IgG.  AT was probed for using goat anti-human AT polyclonal IgG.  Mouse anti-human maspin monoclonal IgG was used as one negative control because it is a serpin that is not produced in the liver and not thought to be in the blood vessels or atheromas.  Goat IgG was used as another negative control to ensure that any antigen binding was not nonspecific binding due to IgG interactions.   Using the American Heart Association (AHA) classification system, each atherosclerotic lesion from each case was blindly graded by three individuals. The intensity of staining was also independently ranked on a scale of 0 to 3 with 0 indicating no staining, 1 indicating weak staining, 2 indicating intermediate staining and 3 indicating strong staining.   As evidenced by the Spearman correlation coefficient of 0.76 (two-sided p-value <0.0001) and the Nonzero correlation statistic of 16.9039 (exact p-value <0.0001), there is a significant positive correlation between lesion severity and HCII staining intensity.