Thrombospondins deployed by thrombopoietic cells determine angiogenic switch and extent of revascularization
Hans-Georg Kopp, … , Aaron J. Marcus, Shahin Rafii
Hans-Georg Kopp, … , Aaron J. Marcus, Shahin Rafii
Published December 1, 2006
Citation Information: J Clin Invest. 2006;116(12):3277-3291. https://doi.org/10.1172/JCI29314.
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Research Article Vascular biology

Thrombospondins deployed by thrombopoietic cells determine angiogenic switch and extent of revascularization

Abstract

Thrombopoietic cells may differentially promote or inhibit tissue vascularization by releasing both pro- and antiangiogenic factors. However, the molecular determinants controlling the angiogenic phenotype of thrombopoietic cells remain unknown. Here, we show that expression and release of thrombospondins (TSPs) by megakaryocytes and platelets function as a major antiangiogenic switch. TSPs inhibited thrombopoiesis, diminished bone marrow microvascular reconstruction following myelosuppression, and limited the extent of revascularization in a model of hind limb ischemia. We demonstrate that thrombopoietic recovery following myelosuppression was significantly enhanced in mice deficient in both TSP1 and TSP2 (TSP-DKO mice) in comparison with WT mice. Megakaryocyte and platelet levels in TSP-DKO mice were rapidly restored, thereby accelerating revascularization of myelosuppressed bone marrow and ischemic hind limbs. In addition, thrombopoietic cells derived from TSP-DKO mice were more effective in supporting neoangiogenesis in Matrigel plugs. The proangiogenic activity of TSP-DKO thrombopoietic cells was mediated through activation of MMP-9 and enhanced release of stromal cell–derived factor 1. Thus, TSP-deficient thrombopoietic cells function as proangiogenic agents, accelerating hemangiogenesis within the marrow and revascularization of ischemic hind limbs. As such, interference with the release of cellular stores of TSPs may be clinically effective in augmenting neoangiogenesis.

Authors

Hans-Georg Kopp, Andrea T. Hooper, M. Johan Broekman, Scott T. Avecilla, Isabelle Petit, Min Luo, Till Milde, Carlos A. Ramos, Fan Zhang, Tabitha Kopp, Paul Bornstein, David K. Jin, Aaron J. Marcus, Shahin Rafii

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Figure 9

TSP-DKO megakaryocytes are highly angiogenic in a Matrigel plug assay (A) Megakaryocytes derived from TSP-DKO or WT mice were resuspended in growth factor–depleted Matrigel, injected subcutaneously, and plugs were harvested 3 weeks later.

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TSP-DKO megakaryocytes are highly angiogenic in a Matrigel plug assay (...
While the control plugs containing only carrier solution were virtually free of vasculature, the megakaryocyte-containing plugs showed vascular channel formation (red arrows) both in the WT and in the TSP-DKO megakaryocyte-loaded plugs. Representative fields were stained with H&E and anti-panendothelial cell antigen marker clone MECA32 (blood vessels). Scored at original magnification, ×400. (B) The number of MECA32+ neovessels was significantly higher in the plugs loaded with TSP-DKO megakaryocytes (n = 3, P < 0.05).