Abstract

We have shown that bacterial products (proteoglycan-polysaccharide, PG- APS) found in the lower bowel produce chronic granulomatous inflammation similar to Crohn's disease (regional ileitis) in genetically susceptible rats as well as associated systemic inflammation. Activation of the contact system (CS) in plasma produces plasma kallikrein which activates neutrophils, cleaves high molecular weight kininogen (HK) and releases bradykinin which induces pain, swelling, diarrhea, and muscle contraction, all of which are characteristic symptoms of intestinal inflammation. We have shown that the CS activates mediates acute and chronic phases of intestinal inflammation in susceptible Lewis rats and is selective activated in these rats, but not in the resistant Buffalo rats. A specific kallikrein inhibitor decreases CS activation, acute inflammatory changes (edema, neutrophil infiltration), chronic intestinal inflammation and the systemic complications (arthritis, splenomegaly, hepatomegaly, leukocytosis, and the acute phase reaction. We have recently shown that there is a molecular difference between the plasma kininogen from Lewis rats which results in more rapid cleavage to yield bradykinin than in Buffalo rats. This proposal will test two hypotheses: (1) genetic differences between kininogen in susceptible and resistant rats result in selective activation of the Plasma Cs mediating certain of the pathological changes; (2) locally, intestinal tissue kallikrein is released and contributes to inflammatory changes. We will define the relationship of the single amino acid change to the functional consequences. In the view of the efficacy of plasma kallikrein inhibitors in blocking enterocolitis, we will use recombinant HK derivatives and peptides derived from HK which can distinguish in vitro whether plasma kallikrein stimulation of neutrophils or bradykinin actions are responsible. In vivo, we will use kinin receptor blockers to define the mechanisms responsible for the enterocolitis. If bradykinin (BK) is responsible, then BK receptor blockers already used in clinical trials may merit evaluation in the therapy of chronic granulomatous enterocolitis. If plasma kallikrein is responsible, the development of plasma kallikrein inhibitors should be pursued. We will study the effect of total kininogen deficiency on the development of acute and chronic enterocolitis and systemic inflammation. Our recent studies show that tissue kallikrein (TK) is localized in macrophages of chronic granulomas and that TK may be secreted from inflamed intestinal cells. We will assay low molecular weight kininogen, the substrate of Tk using a newly designed assay as well as the natural protease inhibitor of TK. We will study the behavior of the TK system in intestinal cell lines and macrophages stimulated with PG-APS or inflammatory cytokines. In vivo, we will use a new specific TK inhibitor to attempt to modulate intestinal and systemic inflammation. These studies should demonstrate important mechanisms in the pathogenesis of inflammatory bowel disease. Assays of the CS and/or TK systems could distinguish active form inactive disease. In addition, the inhibitors used alone or in combination could serve in the future as potential therapeutic agents of human disease.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Diabetes and Digestive and Kidney Diseases (NIDDK)
Type
Research Project (R01)
Project #
5R01DK043735-08
Application #
6177148
Study Section
General Medicine A Subcommittee 2 (GMA)
Program Officer
Hamilton, Frank A
Project Start
1992-09-30
Project End
2002-03-31
Budget Start
2000-04-01
Budget End
2001-03-31
Support Year
8
Fiscal Year
2000
Total Cost
$207,585
Indirect Cost

  Institution

Name
Temple University
Department
Internal Medicine/Medicine
Type
Schools of Medicine
DUNS #
City
Philadelphia
State
PA
Country
United States
Zip Code
19122

  Publications

Isordia-Salas, Irma; Pixley, Robin A; Parekh, Hemant et al. (2003) The mutation Ser511Asn leads to N-glycosylation and increases the cleavage of high molecular weight kininogen in rats genetically susceptible to inflammation. Blood 102:2835-42
Stadnicki, Antoni; Mazurek, Urszula; Gonciarz, Maciej et al. (2003) Immunolocalization and expression of kallistatin and tissue kallikrein in human inflammatory bowel disease. Dig Dis Sci 48:615-23
Isordia-Salas, Irma; Pixley, Robin A; Li, Fengling et al. (2002) Kininogen deficiency modulates chronic intestinal inflammation in genetically susceptible rats. Am J Physiol Gastrointest Liver Physiol 283:G180-6
Isordia-Salas, Irma; Pixley, Robin A; Li, Fengling et al. (2002) Chronic intestinal inflammation and angiogenesis in genetically susceptible rats is modulated by kininogen deficiency. Int Immunopharmacol 2:1895-905
Uknis, A B; DeLa Cadena, R A; Janardham, R et al. (2001) Bradykinin receptor antagonists type 2 attenuate the inflammatory changes in peptidoglycan-induced acute arthritis in the Lewis rat. Inflamm Res 50:149-55
Selim, T E; Ghoneim, H R; Abdel Ghaffar, H A et al. (2001) High molecular mass kininogen inhibits cathepsin G-induced platelet activation by forming a complex with cathepsin G. Hematol J 2:371-7
Colman, R W (1999) Plasma and tissue kallikrein in arthritis and inflammatory bowel disease. Immunopharmacology 43:103-8
Stadnicki, A; Sartor, R B; Janardham, R et al. (1998) Kallikrein-kininogen system activation and bradykinin (B2) receptors in indomethacin induced enterocolitis in genetically susceptible Lewis rats. Gut 43:365-74
DeLa Cadena, R A; Kunapuli, S P; Walz, D A et al. (1998) Expression of thrombospondin 1 on the surface of activated platelets mediates their interaction with the heavy chains of human kininogens through Lys 244-Pro 254. Thromb Haemost 79:186-94
Blais Jr, C; Couture, R; Drapeau, G et al. (1997) Involvement of endogenous kinins in the pathogenesis of peptidoglycan-induced arthritis in the Lewis rat. Arthritis Rheum 40:1327-33

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