Essential role of sphingosine 1–phosphate receptor 2 in pathological angiogenesis of the mouse retina
Athanasia Skoura, … , Richard L. Proia, Timothy Hla
Athanasia Skoura, … , Richard L. Proia, Timothy Hla
Published September 4, 2007
Citation Information: J Clin Invest. 2007;117(9):2506-2516. https://doi.org/10.1172/JCI31123.
View: Text | PDF
Research Article Ophthalmology

Essential role of sphingosine 1–phosphate receptor 2 in pathological angiogenesis of the mouse retina

Abstract

Sphingosine 1–phosphate (S1P), a multifunctional lipid mediator that signals via the S1P family of G protein–coupled receptors (S1PR), regulates vascular maturation, permeability, and angiogenesis. In this study, we explored the role of S1P 2 receptor (S1P2R) in normal vascularization and hypoxia-triggered pathological angiogenesis of the mouse retina. S1P2R is strongly induced in ECs during hypoxic stress. When neonatal mice were subjected to ischemia-driven retinopathy, pathologic neovascularization in the vitreous chamber was suppressed in S1p2–/– mice concomitant with reduction in endothelial gaps and inflammatory cell infiltration. In addition, EC patterning and normal revascularization into the avascular zones of the retina were augmented. Reduced expression of the proinflammatory enzyme cyclooxygenase-2 (COX-2) and increased expression of eNOS were observed in the S1p2–/– mouse retina. S1P2R activation in ECs induced COX-2 expression and suppressed the expression of eNOS. These data identify the S1P2R-driven inflammatory process as an important molecular event in pathological retinal angiogenesis. We propose that antagonism of the S1P2R may be a novel therapeutic approach for the prevention and/or treatment of pathologic ocular neovascularization.

Authors

Athanasia Skoura, Teresa Sanchez, Kevin Claffey, Suzanne M. Mandala, Richard L. Proia, Timothy Hla

×

Figure 5

S1P2 regulates inflammatory response in ischemic retinas.

Options: View larger image (or click on image) Download as PowerPoint
S1P2 regulates inflammatory response in ischemic retinas. ...
Retinal cross sections stained with F4/80 macrophage marker show increased inflammatory response in S1p2+/+ retinas (A) in areas of neovascularization (arrows) and in close association with ECs between GCL and INL (arrowheads) compared with S1p2–/– retinas (B). (C) At P15, the mean number of F4/80-positive cells was 30.57 ± 8.23 (n = 2) for S1p2+/+ retinas, 33.91 ± 9.5 (n = 4) for S1p2+/– retinas, and 16.85 ± 4.33 (n = 4; *P < 0.02) for S1p2–/– retinas. (D) At P17, the mean number of F4/80-positive cells was 83.76 ± 20.93 (n = 3) for S1p2+/+ retinas and 31.81 ± 9.88 (n = 3; *P < 0.02) for S1p2–/– retinas. At P17, whole mount retinas were perfused with FITC–RCA I, which highlights endothelial gaps (arrowheads) but is excluded from nonperfused vascular tufts areas (arrows) in S1p2+/+ (E) and in S1p2–/– retinas (F). Values represent mean ± SD. Scale bars: 100 μm (E and F) and 10 μm (A and B).