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An adventitial IL-6/MCP1 amplification loop accelerates macrophage-mediated vascular inflammation leading to aortic dissection in mice
Brian C. Tieu, … , Ronald G. Tilton, Allan R. Brasier
Brian C. Tieu, … , Ronald G. Tilton, Allan R. Brasier
Published November 16, 2009
Citation Information: J Clin Invest. 2009;119(12):3637-3651. https://doi.org/10.1172/JCI38308.
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Research Article

An adventitial IL-6/MCP1 amplification loop accelerates macrophage-mediated vascular inflammation leading to aortic dissection in mice

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Abstract

Vascular inflammation contributes to cardiovascular diseases such as aortic aneurysm and dissection. However, the precise inflammatory pathways involved have not been clearly defined. We have shown here that subcutaneous infusion of Ang II, a vasopressor known to promote vascular inflammation, into older C57BL/6J mice induced aortic production of the proinflammatory cytokine IL-6 and the monocyte chemoattractant MCP-1. Production of these factors occurred predominantly in the tunica adventitia, along with macrophage recruitment, adventitial expansion, and development of thoracic and suprarenal aortic dissections. In contrast, a reduced incidence of dissections was observed after Ang II infusion into mice lacking either IL-6 or the MCP-1 receptor CCR2. Further analysis revealed that Ang II induced CCR2+CD14hiCD11bhiF4/80– macrophage accumulation selectively in aortic dissections and not in aortas from Il6–/– mice. Adoptive transfer of Ccr2+/+ monocytes into Ccr2–/– mice resulted in selective monocyte uptake into the ascending and suprarenal aorta in regions of enhanced ROS stress, with restoration of IL-6 secretion and increased incidence of dissection. In vitro, coculture of monocytes and aortic adventitial fibroblasts produced MCP-1– and IL-6–enriched conditioned medium that promoted differentiation of monocytes into macrophages, induced CD14 and CD11b upregulation, and induced MCP-1 and MMP-9 expression. These results suggest that leukocyte-fibroblast interactions in the aortic adventitia potentiate IL-6 production, inducing local monocyte recruitment and activation, thereby promoting MCP-1 secretion, vascular inflammation, ECM remodeling, and aortic destabilization.

Authors

Brian C. Tieu, Chang Lee, Hong Sun, Wanda LeJeune, Adrian Recinos 3rd, Xiaoxi Ju, Heidi Spratt, Dong-Chuan Guo, Dianna Milewicz, Ronald G. Tilton, Allan R. Brasier

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Figure 4

Localization of macrophages, AoAFs, and cytokines in mouse ascending aorta and IL-6 in sporadic type A aortic dissection in human tissue.

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Localization of macrophages, AoAFs, and cytokines in mouse ascending aor...
(A) PKH26-labeled Ccr2+/+ monocytes (red) were transferred into Ccr2–/– mice. Labeled macrophages are detected in cross sections of an ascending dissecting aneurysm invading the media from the adventitia/media border along with disruption of elastic lamellae at the dissection. Nuclei are DAPI stained (blue; right). The small image shows monocytes labeled in vitro. (B) Immunofluorescence staining for IL-6, MCP-1, and AoAF in transverse cryosections (6 μm) of ascending aorta from Ang II–treated Ccr2–/– mice injected with Ccr2+/+ monocytes (positive staining is shown in red). Nuclei are DAPI stained (blue). Elastic lamellae are green. (C) Human type A sporadic dissection was stained for IL-6 (red). Note IL-6 staining is predominantly adventitial (left) and not in the medial or intimal (right) layers. Elastic lamellae are green. Hematoxylin was used as the counterstain. A, adventitia; M, media; I, intima. Original magnification, ×200.

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