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The Journal of Immunology, 1999, 162: 1032-1041.
Copyright © 1999 by The American Association of Immunologists

The Mast Cell as Site of Tissue-Type Plasminogen Activator Expression and Fibrinolysis1

Christian Sillaber2,*, Mehrdad Baghestanian2,*, Dorian Bevec§, Martin Willheim, Hermine Agis*, Stylianos Kapiotis||, Wolfgang Füreder*, Hans C. Bankl#, Hans P. Kiener{dagger}, Wolfgang Speiser||, Bernd R. Binder{ddagger}, Klaus Lechner* and Peter Valent3,*

* Department of Internal Medicine I, Division of Hematology and Hemostaseology, {dagger} Department of Internal Medicine III, Division of Rheumatology, {ddagger} Institute of Physiology, Department of Vascular Biology and Thrombosis Research, University of Vienna, Vienna, Austria; § Sandoz Research Institute, Vienna, Austria; and Institute of General and Experimental Pathology, || Department of Laboratory Medicine, and # Institute of Clinical Pathology, University of Vienna, Vienna, Austria

Recent data suggest that mast cells (MC) and their products (heparin, proteases) are involved in the regulation of coagulation and fibrino(geno)lysis. The key enzyme of fibrinolysis, plasmin, derives from its inactive progenitor, plasminogen, through catalytic action of plasminogen activators (PAs). In most cell systems, however, PAs are neutralized by plasminogen activator inhibitors (PAIs). We report that human tissue MC as well as the MC line HMC-1 constitutively produce, express, and release tissue-type plasminogen activator (tPA) without producing inhibitory PAIs. As assessed by Northern blotting, highly enriched lung MC (>98% pure) as well as HMC-1 expressed tPA mRNA, but did not express mRNA for PAI-1, PAI-2, or PAI-3. The tPA protein was detectable in MC-conditioned medium by Western blotting and immunoassay, and the MC agonist stem cell factor (c-Kit ligand) was found to promote the release of tPA from MC. In addition, MC-conditioned medium induced fibrin-independent plasmin generation as well as clot lysis in vitro. These observations raise the possibility that MC play an important role in endogenous fibrinolysis.




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