| Literature DB >> 27539859 |
Michael Regn1, Bernhard Laggerbauer1, Claudia Jentzsch1, Deepak Ramanujam1, Andrea Ahles1, Sonja Sichler1, Julia Calzada-Wack2, Rory R Koenen3, Attila Braun4, Bernhard Nieswandt4, Stefan Engelhardt5.
Abstract
A key response of the myocardium to stress is the secretion of factors with paracrine or endocrine function. Intriguing in this respect is peptidase inhibitor 16 (PI16), a member of the CAP family of proteins which we found to be highly upregulated in cardiac disease. Up to this point, the mechanism of action and physiological function of PI16 remained elusive. Here, we show that PI16 is predominantly expressed by cardiac fibroblasts, which expose PI16 to the interstitium via a glycophosphatidylinositol (-GPI) membrane anchor. Based on a reported genetic association of PI16 and plasma levels of the chemokine chemerin, we investigated whether PI16 regulates post-translational processing of its precursor pro-chemerin. PI16-deficient mice were engineered and found to generate higher levels of processed chemerin than wildtype mice. Purified recombinant PI16 efficiently inhibited cathepsin K, a chemerin-activating protease, in vitro. Moreover, we show that conditioned medium from PI16-overexpressing cells impaired the activation of pro-chemerin. Together, our data indicate that PI16 suppresses chemerin activation in the myocardium and suggest that this circuit may be part of the cardiac stress response.Entities:
Keywords: Chemerin; Chemerin processing; Peptidase inhibitor 16 (PI16); Protease inhibition; RARRES2; TIG2
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Year: 2016 PMID: 27539859 DOI: 10.1016/j.yjmcc.2016.08.010
Source DB: PubMed Journal: J Mol Cell Cardiol ISSN: 0022-2828 Impact factor: 5.000