Blocking the proteolytic activity of zymogen matriptase with antibody-based inhibitors

Trine Tamberg, Zebin Hong, Daphné De Schepper, Signe Skovbjerg, Daniel M. Dupont, Lars Vitved, Christine R. Schar, Karsten Skjoedt, Lotte K. Vogel, Jan K. Jensen*

*Corresponding author for this work
5 Citations (Scopus)

Abstract

Matriptase is a member of the type-II transmembrane serine protease (TTSP) family and plays a crucial role in the development and maintenance of epithelial tissues. As all chymotrypsin-like serine proteases, matriptase is synthesized as a zymogen (proform), requiring a cleavage event for full activity. Recent studies suggest that the zymogen of matriptase possesses enough catalytic activity to not only facilitate autoactivation, but also carry out its in vivo functions, which include activating several proteolytic and signaling cascades. Inhibition of zymogen matriptase may therefore be a highly effective approach for limiting matriptase activity. To this end, here we sought to characterize the catalytic activity of human zymogen matriptase and to develop mAb inhibitors against this enzyme form. Using a mutated variant of matriptase in which the serine protease domain is locked in the zymogen conformation, we confirmed that the zymogen form of human matriptase has catalytic activity. Moreover, the crystal structure of the catalytic domain of zymogen matriptase was solved to 2.5 Å resolution to characterize specific antibody-based matriptase inhibitors and to further structure-based studies. Finally, we describe the first antibody-based competitive inhibitors that target both the zymogen and activated forms of matriptase. We propose that these antibodies provide a more efficient way to regulate matriptase activity by targeting the protease both before and after its activation and may be of value for both research and preclinical applications.

Original languageEnglish
JournalJournal of Biological Chemistry
Volume294
Issue number1
Pages (from-to)314-326
Number of pages13
ISSN0021-9258
DOIs
Publication statusPublished - 4 Jan 2019

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