Characterization of the catalytic properties of the membrane-anchored metalloproteinase ADAM9 in cell-based assays

Thorsten Maretzky; Steven Swendeman; Elin Mogollon; Gisela Weskamp; Umut Sahin; Karina Reiss; Carl P Blobel

doi:10.1042/BCJ20170075

Characterization of the catalytic properties of the membrane-anchored metalloproteinase ADAM9 in cell-based assays

Biochem J. 2017 Apr 13;474(9):1467-1479. doi: 10.1042/BCJ20170075.

Authors

Thorsten Maretzky¹, Steven Swendeman^{1

2}, Elin Mogollon¹, Gisela Weskamp¹, Umut Sahin^{1

3}, Karina Reiss⁴, Carl P Blobel^{5

6

7}

Affiliations

¹ Arthritis and Tissue Degeneration Program, Hospital for Special Surgery at Weill Cornell Medicine, New York, NY 10021, U.S.A.
² Boston Children's Hospital, Boston, MA 02115, U.S.A.
³ Center for Life Sciences and Technologies, Bogazici University, Istanbul 34342, Turkey.
⁴ Department of Dermatology, University Hospital Schleswig-Holstein, Campus Kiel, Kiel 24105, Germany.
⁵ Arthritis and Tissue Degeneration Program, Hospital for Special Surgery at Weill Cornell Medicine, New York, NY 10021, U.S.A. blobelc@hss.edu.
⁶ Department of Physiology, Biophysics and Systems Biology, Weill Cornell Medicine, New York, NY, U.S.A.
⁷ Institute for Advanced Study, Technical University Munich, Garching 85748, Germany.

Abstract

ADAM9 (A Disintegrin And Metalloprotease 9) is a membrane-anchored metalloproteinase that has been implicated in pathological retinal neovascularization and in tumor progression. ADAM9 has constitutive catalytic activity in both biochemical and cell-based assays and can cleave several membrane proteins, including epidermal growth factor and Ephrin receptor B4; yet little is currently known about the catalytic properties of ADAM9 and its post-translational regulation and inhibitor profile in cell-based assays. To address this question, we monitored processing of the membrane-anchored Ephrin receptor B4 (EphB4) by co-expressing ADAM9, with the catalytically inactive ADAM9 E > A mutant serving as a negative control. We found that ADAM9-dependent shedding of EphB4 was not stimulated by three commonly employed activators of ADAM-dependent ectodomain shedding: phorbol esters, pervanadate or calcium ionophores. With respect to the inhibitor profile, we found that ADAM9 was inhibited by the hydroxamate-based metalloprotease inhibitors marimastat, TAPI-2, BB94, GM6001 and GW280264X, and by 10 nM of the tissue inhibitor of metalloproteinases (TIMP)-3, but not by up to 20 nM of TIMP-1 or -2. Additionally, we screened a non-hydroxamate small-molecule library for novel ADAM9 inhibitors and identified four compounds that selectively inhibited ADAM9-dependent proteolysis over ADAM10- or ADAM17-dependent processing. Taken together, the present study provides new information about the molecular fingerprint of ADAM9 in cell-based assays by showing that it is not stimulated by strong activators of ectodomain shedding and by defining a characteristic inhibitor profile. The identification of novel non-hydroxamate inhibitors of ADAM9 could provide the basis for designing more selective compounds that block the contribution of ADAM9 to pathological neovascularization and cancer.

Keywords: ADAM9 (A Disintegrin And Metalloproteinase 9); EphB4; ectodomain shedding; molecular fingerprint.

MeSH terms

ADAM Proteins / antagonists & inhibitors*
ADAM Proteins / metabolism*
Animals
COS Cells
Catalysis
Cell Membrane / drug effects
Cell Membrane / enzymology*
Chlorocebus aethiops
Dose-Response Relationship, Drug
Enzyme Inhibitors / pharmacology
Membrane Proteins / antagonists & inhibitors*
Membrane Proteins / metabolism*
Mice

Substances

Enzyme Inhibitors
Membrane Proteins
ADAM Proteins
ADAM9 protein, human

Grants and funding

R01 GM064750/GM/NIGMS NIH HHS/United States