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Fibroblast-specific IKK-β deficiency ameliorates angiotensin II–induced adverse cardiac remodeling in mice
Weiwei Lu, Zhaojie Meng, Rebecca Hernandez, Changcheng Zhou
Weiwei Lu, Zhaojie Meng, Rebecca Hernandez, Changcheng Zhou
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Research Article Cardiology

Fibroblast-specific IKK-β deficiency ameliorates angiotensin II–induced adverse cardiac remodeling in mice

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Abstract

Cardiac inflammation and fibrosis contribute significantly to hypertension-related adverse cardiac remodeling. IκB kinase β (IKK-β), a central coordinator of inflammation through activation of NF-κB, has been demonstrated as a key molecular link between inflammation and cardiovascular disease. However, the cell-specific contribution of IKK-β signaling toward adverse cardiac remodeling remains elusive. Cardiac fibroblasts are one of the most populous nonmyocyte cell types in the heart that play a key role in mediating cardiac fibrosis and remodeling. To investigate the function of fibroblast IKK-β, we generated inducible fibroblast-specific IKK-β–deficient mice. Here, we report an important role of IKK-β in the regulation of fibroblast functions and cardiac remodeling. Fibroblast-specific IKK-β–deficient male mice were protected from angiotensin II–induced cardiac hypertrophy, fibrosis, and macrophage infiltration. Ablation of fibroblast IKK-β inhibited angiotensin II–stimulated fibroblast proinflammatory and profibrogenic responses, leading to ameliorated cardiac remodeling and improved cardiac function in IKK-β–deficient mice. Findings from this study establish fibroblast IKK-β as a key factor regulating cardiac fibrosis and function in hypertension-related cardiac remodeling.

Authors

Weiwei Lu, Zhaojie Meng, Rebecca Hernandez, Changcheng Zhou

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Figure 7

Angiotensin II–induced cardiac inflammation was inhibited in IKK-β–deficient mice.

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Angiotensin II–induced cardiac inflammation was inhibited in IKK-β–defic...
Eight-week-old male IKKβfl/fl and IKKβΔFib mice were i.p. injected with 2 mg tamoxifen per day for 5 days. At the age of 10 weeks, those mice were infused with 1000 ng/kg/min of angiotensin II (Ang II) or vehicle control for 1 week. (A) Western blot analysis of the protein levels of total and phosphorylated (p) IKK-β and NF-κB subunit p65 in the hearts of IKKβfl/fl and IKKβΔFib mice. (B) qPCR analysis of the mRNA levels of inflammatory cytokines and chemokines in the hearts of IKKβfl/fl and IKKβΔFib mice (n = 4–5; 2-way ANOVA; *P < 0.05, **P < 0.01, ***P < 0.001). (C and D) Representative images of immunofluorescence staining (left) and the quantifications (right) of IL-6 (C) and MCP-1 (D) in the hearts of IKKβfl/fl and IKKβΔFib mice. The nuclei were visualized with DAPI (blue) (n = 3–4; 2-way ANOVA; ***P < 0.001; scale bar: 50 μm).

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