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Mucus Detachment by Host Metalloprotease Meprin β Requires Shedding of Its Inactive Pro-form, which Is Abrogated by the Pathogenic Protease RgpB
Author(s) -
Rielana Wichert,
Anna Ermund,
Stefanie Schmidt,
Matthias Schweinlin,
Mirosław Książęk,
Philipp Arnold,
Katharina Knittler,
Frederike Wilkens,
Barbara Potempa,
Björn Rabe,
Marit Stirnberg,
Ralph Lucius,
Jörg W. Bartsch,
Susanikolaus,
Maren FalkPaulsen,
Philip Rosenstiel,
Marco Metzger,
Stefan RoseJohn,
Jan Potempa,
Gunnar C. Hansson,
Peter J. Dempsey,
Christoph BeckerPauly
Publication year - 2017
Publication title -
cell reports
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 6.264
H-Index - 154
eISSN - 2639-1856
pISSN - 2211-1247
DOI - 10.1016/j.celrep.2017.10.087
Subject(s) - metalloproteinase , proteases , protease , microbiology and biotechnology , mucus , mucin , disintegrin , biology , cysteine protease , secretion , chemistry , biochemistry , matrix metalloproteinase , enzyme , ecology
The host metalloprotease meprin β is required for mucin 2 (MUC2) cleavage, which drives intestinal mucus detachment and prevents bacterial overgrowth. To gain access to the cleavage site in MUC2, meprin β must be proteolytically shed from epithelial cells. Hence, regulation of meprin β shedding and activation is important for physiological and pathophysiological conditions. Here, we demonstrate that meprin β activation and shedding are mutually exclusive events. Employing ex vivo small intestinal organoid and cell culture experiments, we found that ADAM-mediated shedding is restricted to the inactive pro-form of meprin β and is completely inhibited upon its conversion to the active form at the cell surface. This strict regulation of meprin β activity can be overridden by pathogens, as demonstrated for the bacterial protease Arg-gingipain (RgpB). This secreted cysteine protease potently converts membrane-bound meprin β into its active form, impairing meprin β shedding and its function as a mucus-detaching protease.

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