Abstract

Intimal thickening is a complex, common response to many forms of vascular injury. It occurs during native atherosclerosis as well as after angioplasty or vein graft arterialization, and is mediated in part by growth factor stimulated smooth muscle cell (SMC) proliferation, migration, and matrix accumulation. The molecular and cellular events controlling these responses are poorly understood; discovery of novel mechanisms of regulation may enable new therapeutic modalities. Our laboratory has studied the regulation of plasminogen activators (PA) by vascular cells. PAs, which are secreted by SMC after vascular injury, may bind to specific cellular receptors, thereby generating plasmin locally and facilitating the movement of SMC through tissue barriers and extracellular matrix. Three recent findings have suggested additional mechanisms of PA regulation of SMC function: l) tissue-type PA (t-PA) activity directly stimulates SMC proliferation; 2) low density lipoprotein receptor related protein (LRP) can internalize and degrade PAs and PA/PA inhibitor complexes; and 3) urokinase-type PA receptor (u-PAR) directly modulates monocyte migration independent of u-PA activity. We have hypothesized that: a) t-PA, possibly in the presence of a cofactor, can proteolytically cleave SMC thrombin receptors, inducing proliferation; b) interaction of PAs with one of several possible receptors will alter migration and matrix invasion; c) intimal thickening in diseased vessels and arterialized vein grafts is associated with an altered expression of plasminogen activator system components in the vessel wall; and d) genetic deletion of u-PA or t-PA but not PAI-1 in mice will limit the vascular injury response in vivo. Using radioligand binding studies and ELISAs with monoclonal antibodies to different portions of the human thrombin receptor, we will determine if t-PA binds to and cleaves the SMC thrombin receptor. We will study the effect of alterations in the plasminogen activator system in vitro on vascular smooth muscle cell proliferation, migration, and invasion, and preliminarily determine which domains of the molecules are involved. We will determine the extent and location of protein and mRNA expression for plasminogen activator system components in normal and diseased human vascular tissue and in rabbit jugular veins before and after arterialization. We will use a carotid injury model in mice genetically deficient in u-PA, t-PA, or PAI-1 to determine the effect of deletion of these specific PA system components on the vascular response to injury. Finally, to identify genes that are upregulated early after vascular injury, we will use differential display and RNA isolated from normal rabbit jugular vein and arterialized vein grafts. Candidate amplified cDNAs will be labeled for use in Northern blotting to confirm altered expression and then sequenced. At least two full length cDNA clones will be obtained from cDNA libraries for apparently novel sequences. Vascular cell expression will be evaluated by in situ hybridization. In summary, a greater understanding of the basic pathobiologic processes underlying intimal thickening following vascular injury should allow better development of pharmacologic agents to inhibit these processes.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Heart, Lung, and Blood Institute (NHLBI)
Type
Research Project (R01)
Project #
5R01HL047839-06
Application #
2519330
Study Section
Pathology A Study Section (PTHA)
Project Start
1991-09-30
Project End
1999-08-31
Budget Start
1997-09-01
Budget End
1998-08-31
Support Year
6
Fiscal Year
1997
Total Cost
Indirect Cost

  Institution

Name
University of Pennsylvania
Department
Internal Medicine/Medicine
Type
Schools of Medicine
DUNS #
042250712
City
Philadelphia
State
PA
Country
United States
Zip Code
19104

  Publications

Bdeir, K; Murciano, J C; Tomaszewski, J et al. (2000) Urokinase mediates fibrinolysis in the pulmonary microvasculature. Blood 96:1820-6
Kariko, K; Kuo, A; Barnathan, E (1999) Overexpression of urokinase receptor in mammalian cells following administration of the in vitro transcribed encoding mRNA. Gene Ther 6:1092-100
Kariko, K; Kuo, A; Barnathan, E S et al. (1998) Phosphate-enhanced transfection of cationic lipid-complexed mRNA and plasmid DNA. Biochim Biophys Acta 1369:320-34
Chang, A W; Kuo, A; Barnathan, E S et al. (1998) Urokinase receptor-dependent upregulation of smooth muscle cell adhesion to vitronectin by urokinase. Arterioscler Thromb Vasc Biol 18:1855-60
Okada, S S; Golden, M A; Raghunath, P N et al. (1998) Native atherosclerosis and vein graft arterialization: association with increased urokinase receptor expression in vitro and in vivo. Thromb Haemost 80:140-7
Neschis, D G; Safford, S D; Raghunath, P N et al. (1998) Thermal preconditioning before rat arterial balloon injury: limitation of injury and sustained reduction of intimal thickening. Arterioscler Thromb Vasc Biol 18:120-6
Molino, M; Raghunath, P N; Kuo, A et al. (1998) Differential expression of functional protease-activated receptor-2 (PAR-2) in human vascular smooth muscle cells. Arterioscler Thromb Vasc Biol 18:825-32
Barnathan, E S; Raghunath, P N; Tomaszewski, J E et al. (1997) Immunohistochemical localization of defensin in human coronary vessels. Am J Pathol 150:1009-20
Molino, M; Barnathan, E S; Numerof, R et al. (1997) Interactions of mast cell tryptase with thrombin receptors and PAR-2. J Biol Chem 272:4043-9
Weisz, P B; Joullie, M M; Hunter, C M et al. (1997) A basic compositional requirement of agents having heparin-like cell-modulating activities. Biochem Pharmacol 54:149-57

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