P2X7 receptor signaling contributes to tissue factor–dependent thrombosis in mice
Christian Furlan-Freguia, … , Zaverio M. Ruggeri, Wolfram Ruf
Christian Furlan-Freguia, … , Zaverio M. Ruggeri, Wolfram Ruf
Published June 13, 2011
Citation Information: J Clin Invest. 2011;121(7):2932-2944. https://doi.org/10.1172/JCI46129.
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Research Article Hematology

P2X7 receptor signaling contributes to tissue factor–dependent thrombosis in mice

Abstract

Thrombosis is initiated by tissue factor (TF), a coagulation cofactor/receptor expressed in the vessel wall, on myeloid cells, and on microparticles (MPs) with variable procoagulant activity. However, the molecular pathways that generate prothrombotic TF in vivo are poorly defined. The oxidoreductase protein disulfide isomerase (PDI) is thought to be involved in the activation of TF. Here, we found that in mouse myeloid cells, ATP-triggered signaling through purinergic receptor P2X, ligand-gated ion channel, 7 (P2X7 receptor; encoded by P2rx7) induced activation (decryption) of TF procoagulant activity and promoted release of TF+ MPs from macrophages and SMCs. The generation of prothrombotic MPs required P2X7 receptor–dependent production of ROS leading to increased availability of solvent-accessible extracellular thiols. An antibody to PDI with antithrombotic activity in vivo attenuated the release of procoagulant MPs. In addition, P2rx7–/– mice were protected from TF-dependent FeCl3-induced carotid artery thrombosis. BM chimeras revealed that P2X7 receptor prothrombotic function was present in both hematopoietic and vessel wall compartments. In contrast, an alternative anti-PDI antibody showed activities consistent with cellular activation typically induced by P2X7 receptor signaling. This anti-PDI antibody restored TF-dependent thrombosis in P2rx7–/– mice. These data suggest that PDI regulates a critical P2X7 receptor–dependent signaling pathway that generates prothrombotic TF, defining a link between inflammation and thrombosis with potential implications for antithrombotic therapy.

Authors

Christian Furlan-Freguia, Patrizia Marchese, András Gruber, Zaverio M. Ruggeri, Wolfram Ruf

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Figure 1

ATP activation of P2X7 receptor induces macrophage TF activation coupled to TF+ MP release.

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ATP activation of P2X7 receptor induces macrophage TF activation coupled...
(A) TF activity, measured by FXa generation assays on macrophage cell surfaces or released MPs after stimulation with ATP (5 mM) or ionomycin (10 μM). FVIIai (100 nM) was used to demonstrate TF specificity (n ≥ 4). *P < 0.01 vs. control; #P < 0.01 vs. ATP. (B) Western blotting for TF in WT or P2rx7–/– macrophages before and after stimulation with 5 mM ATP for 30 minutes; blots are representative of at least 3 independent experiments. (C) Western blotting for MP-associated proteins; blots are representative of at least 4 independent experiments. (D) FACS analysis of MPs released from ATP stimulated macrophages. ATP sup., supernatants of ATP-stimulated cells after MP depletion by centrifugation. Shown are typical plots of MP detection on a LSR-II flow cytometer and quantitation of particle counts from 2–3 experiments performed in triplicate; *P < 0.001 vs. control.