IRF5 governs macrophage adventitial infiltration to fuel abdominal aortic aneurysm formation
Yidong Wang, … , Zhejun Cai, Meixiang Xiang
Yidong Wang, … , Zhejun Cai, Meixiang Xiang
Published January 4, 2024
Citation Information: JCI Insight. 2024;9(3):e171488. https://doi.org/10.1172/jci.insight.171488.
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Research Article Vascular biology

IRF5 governs macrophage adventitial infiltration to fuel abdominal aortic aneurysm formation

Abstract

Abdominal aortic aneurysm (AAA) is a chronic inflammatory disease characterized by the expansion of the aortic wall. One of the most significant features is the infiltration of macrophages in the adventitia, which drives vasculature remodeling. The role of macrophage-derived interferon regulatory factor 5 (IRF5) in macrophage infiltration and AAA formation remains unknown. RNA sequencing of AAA adventitia identified Irf5 as the top significantly increased transcription factor that is predominantly expressed in macrophages. Global and myeloid cell–specific deficiency of Irf5 reduced AAA progression, with a marked reduction in macrophage infiltration. Further cellular investigations indicated that IRF5 promotes macrophage migration by direct regulation of downstream phosphoinositide 3-kinase γ (PI3Kγ, Pik3cg). Pik3cg ablation hindered AAA progression, and myeloid cell–specific salvage of Pik3cg restored AAA progression and macrophage infiltration derived from Irf5 deficiency. Finally, we found that IRF5 and PI3Kγ expression in the adventitia is significantly increased in patients with AAA. These findings reveal that the IRF5-dependent regulation of PI3Kγ is essential for AAA formation.

Authors

Yidong Wang, Zhenjie Liu, Shen Song, Jianfang Wang, Chunna Jin, Liangliang Jia, Yuankun Ma, Tan Yuan, Zhejun Cai, Meixiang Xiang

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Figure 3

IRF5 contributes to macrophage migration.

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IRF5 contributes to macrophage migration. (A and B) Dot plots represent ...
(A and B) Dot plots represent enrichment analysis of genes corresponding to the downregulated (A) and upregulated (B) differentially expressed genes in Irf5–/– AAA tissues versus WT AAA tissues. Enrichment analysis was performed with Metascape, with cutoffs defined as adjusted P value < 0.05 and log2(fold change) > 1. The top 20 gene ontologies are listed. (C) Left: Representative pictures of wound healing assays conducted with macrophages from Irf5fl/fl and Irf5ΔMΦ mice immediately after scratching and 24 hours later (n = 9). Right: Cells migrating to the wound zone were quantified. (D) Left: Schematic of the Transwell system in which macrophages were seeded in the upper chamber, and medium with TNF-α was placed in the lower chamber. Right: Cells transmigrating through the filter to the underside of membranes were stained with DAPI and quantified (n = 9). Scale bar: 50 μm. Data in C and D are presented as mean ± SD, and significance was determined by unpaired, 2-tailed Student’s t test. **P < 0.01, ***P < 0.001.