Abstract
Protease-mediated degradation of proteins is critical in a plethora of physiological processes. Neutrophils secrete serine proteases including cathepsin G (CatG), neutrophile elastase (NE), and proteinase 3 (PR3) together with lactoferrin (LF) as a first cellular immune response against pathogens. Here, we demonstrate that LF increases the catalytic activity of CatG at physiological concentration, with its highest enhancing capacity under acidic (pH 5.0) conditions, and broadens the substrate selectivity of CatG. On a functional level, the enzymatic activity of CatG was increased in the presence of LF in granulocyte-derived supernatant. Furthermore, LF enhanced CatG-induced activation of platelets as determined by cell surface expression of CD62P. Consequently, LF-mediated enhancement of CatG activity might promote innate immunity during acute inflammation.
Publication types
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Research Support, Non-U.S. Gov't
MeSH terms
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Allosteric Regulation / drug effects
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Biocatalysis / drug effects
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Cathepsin G / metabolism*
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Culture Media, Conditioned / pharmacology
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Electrophoresis, Polyacrylamide Gel
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Enzyme Activation / drug effects
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Granulocytes / metabolism
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Humans
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Hydrogen-Ion Concentration
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Immunity, Innate / drug effects*
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Immunoblotting
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Inflammation / immunology
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Lactoferrin / pharmacology*
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Leukocyte Elastase / metabolism
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Platelet Activation / drug effects*
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Proteolysis / drug effects
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Substrate Specificity
Substances
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Culture Media, Conditioned
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LTF protein, human
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Lactoferrin
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CTSG protein, human
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Cathepsin G
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Leukocyte Elastase
Grants and funding
This work was supported by DAAD 91506408, Deutsche Diabetes Stiftung “Das zuckerkranke Kind” (DDS) 226/06/13, and Humboldt DPK-422-1658/2013 grant. The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.