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The role of protease‐activated receptors PAR‐1 and PAR‐2 in the repair of 16HBE 14o − epithelial cell monolayers in vitro
Author(s) -
Ewen D.,
Clarke S.L.,
Smith J.R.,
Berger C.,
Salmon G.,
Trevethick M.,
Shute J.K.
Publication year - 2010
Publication title -
clinical and experimental allergy
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 1.462
H-Index - 154
eISSN - 1365-2222
pISSN - 0954-7894
DOI - 10.1111/j.1365-2222.2010.03453.x
Subject(s) - proteases , receptor , serine protease , fibrin , microbiology and biotechnology , chemistry , protease , neutralizing antibody , coagulation , in vitro , protease activated receptor 2 , cell culture , biology , antibody , biochemistry , immunology , enzyme , medicine , enzyme linked receptor , genetics
Summary Background We recently reported that repair following mechanical wounding of epithelial cell layers in vitro is dependent on fibrin formation and the activity of locally expressed coagulation cascade proteins. Serine proteases of the coagulation cascade are an important group of protease‐activated receptor (PAR) activators and PAR‐1 to 4 are expressed by the normal bronchial epithelium. Objective We tested the hypothesis that activation of PAR‐1 and PAR‐2 by coagulation cascade proteases stimulates epithelial repair via effects on fibrin formation. Methods Using mechanically wounded 16HBE 14o − epithelial cell layers in culture, we investigated the effect of PAR‐1 and PAR‐2 agonist peptides, control partially scrambled peptides and PAR‐neutralizing antibodies on the rate of repair and fibrin formation. Coagulation factors in culture supernatants were measured by immunoblot. RT‐PCR was used to investigate PAR‐1, PAR‐2 and PGE2 receptor (EP‐1 to EP‐4) expression in this model and qRT‐PCR to quantify responses to wounding. Additionally, we investigated the effect of exogenously added factor Xa (FXa) and neutrophil elastase and the influence of PGE2 and indomethacin on the repair response. Results PAR‐1 and PAR‐2 peptide agonists stimulated the rate of repair and enhanced the formation of a fibrin provisional matrix to support the repair process. Conversely, PAR‐neutralizing antibodies inhibited repair. Under serum‐free culture conditions, 16HBE 14o − cells expressed EP‐2 and EP‐3, but not EP‐1 or EP‐4, receptors. Wounding induced an increased expression of EP‐3 but did not alter EP‐2, PAR‐1 or PAR‐2 expression. In the absence of PAR agonists, there was no evidence for a role for PGE2 in fibrin formation or the repair process. Indomethacin attenuated fibrin formation in wounded cultures only in the presence of the PAR‐2 peptide. FXa stimulated epithelial repair while neutrophil elastase reduced the levels of coagulation factors and inhibited repair. Conclusion Locally expressed serine proteases of the coagulation cascade activate PAR‐1 and PAR‐2 to enhance fibrin formation and bronchial epithelial repair. Cite this as : D. Ewen, S.L. Clarke, J.R. Smith, C. Berger, G. Salmon, M. Trevethick and J.K. Shute, Clinical & Experimental Allergy , 2010 (40) 435–449.

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