Bilayer Membrane Modulation of Membrane Type 1 Matrix Metalloproteinase (MT1-MMP) Structure and Proteolytic Activity

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作者
Linda Cerofolini
Sabrina Amar
Janelle L. Lauer
Tommaso Martelli
Marco Fragai
Claudio Luchinat
Gregg B. Fields
机构
[1] Giotto Biotech S.R.L.,Department of Chemistry & Biochemistry
[2] Florida Atlantic University,Department of Chemistry “U. Schiff”
[3] Max Planck Institute of Molecular Cell Biology and Genetics,Department of Chemistry
[4] CERM,Departments of Chemistry and Biology
[5] University of Florence,undefined
[6] University of Florence,undefined
[7] The Scripps Research Institute/Scripps Florida,undefined
[8] Torrey Pines Institute for Molecular Studies,undefined
[9] 33458,undefined
[10] Port St. Lucie,undefined
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Cell surface proteolysis is an integral yet poorly understood physiological process. The present study has examined how the pericellular collagenase membrane-type 1 matrix metalloproteinase (MT1-MMP) and membrane-mimicking environments interplay in substrate binding and processing. NMR derived structural models indicate that MT1-MMP transiently associates with bicelles and cells through distinct residues in blades III and IV of its hemopexin-like domain, while binding of collagen-like triple-helices occurs within blades I and II of this domain. Examination of simultaneous membrane interaction and triple-helix binding revealed a possible regulation of proteolysis due to steric effects of the membrane. At bicelle concentrations of 1%, enzymatic activity towards triple-helices was increased 1.5-fold. A single mutation in the putative membrane interaction region of MT1-MMP (Ser466Pro) resulted in lower enzyme activation by bicelles. An initial structural framework has thus been developed to define the role(s) of cell membranes in modulating proteolysis.
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