Tumor cell adhesion and migration supported by interaction of a receptor-protease complex with its inhibitor
Edgar G. Fischer, … , Barbara M. Mueller, Wolfram Ruf
Edgar G. Fischer, … , Barbara M. Mueller, Wolfram Ruf
Published November 1, 1999
Citation Information: J Clin Invest. 1999;104(9):1213-1221. https://doi.org/10.1172/JCI7750.
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Article

Tumor cell adhesion and migration supported by interaction of a receptor-protease complex with its inhibitor

Abstract

Tissue factor (TF), the cell-surface receptor for coagulation factor VIIa, supports metastasis. Equally important for this process are (a) interactions of the TF cytoplasmic domain, which binds the mobility-enhancing actin-binding protein 280, and (b) the formation of a proteolytically active TF-VIIa complex on the tumor cell surface. In primary bladder carcinoma cells, we find that this complex localizes to the invasive edge, in proximity to tumor-infiltrating vessels that stain intensely for TF pathway inhibitor (TFPI-1), the major inhibitor of the protease activity of the complex. In culture, binding of VIIa to TF-expressing tumor cells is sufficient to allow cell adhesion, migration, and intracellular signaling on immobilized TFPI-1. Immobilized heparin, a mimic for extracellular matrix–associated proteoglycans, binds physiological concentrations of TFPI-1 in a conformation that supports TF-VIIa–dependent cell adhesion. Consistent with a functional role of TFPI-1 in complex extracellular matrices, we show that TF cooperates with integrin-mediated adhesion and migration on composite matrices that contain ligands for both integrins and the TF-VIIa complex. This study thus provides evidence for a novel mechanism of protease-supported migration that is independent of proteolytic matrix degradation but rather involves protease-dependent bridging of TF’s extracellular domain to an ECM-associated inhibitor.

Authors

Edgar G. Fischer, Matthias Riewald, Hui-Yu Huang, Yohei Miyagi, Yoshinobu Kubota, Barbara M. Mueller, Wolfram Ruf

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Figure 6

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Adhesion on composite matrix. Wells were coated with equal concentration...
Adhesion on composite matrix. Wells were coated with equal concentrations of fibronectin and TFPI-1, as indicated on the x axis. (a) Effect of 10 nM VIIa on the adhesion to the composite matrix. The adhesion buffer contained 5 U/mL heparin to block proteoglycan-dependent cell adhesion to TFPI-1. (b) Effect of function-blocking anti-β1 integrin antibody on the binding to composite matrix. The antibody at 50 μg/mL completely blocked adhesion in the absence of VIIa (anti-β1, no VIIa). Adhesion to the composite matrix in the presence (+ anti-β1) or absence of the blocking antibody was analyzed at various concentrations of immobilized matrix and in the presence of 10 nM VIIa and 5 U/mL heparin.