Macrophage-derived MMP12 promotes fibrosis through sustained damage to endothelial cells

巨噬细胞 细胞外基质 内皮干细胞 纤维化 细胞生物学 基质金属蛋白酶 炎症 生物 M2巨噬细胞 免疫学 化学 病理 医学 生物化学 体外
作者
Xinbei Zhou,Cong Zhang,Shaoqi Yang,Liliang Yang,Wei Luo,Wei Zhang,Xinxin Zhang,Jie Chao
出处
期刊:Journal of Hazardous Materials [Elsevier BV]
卷期号:461: 132733-132733 被引量:16
标识
DOI:10.1016/j.jhazmat.2023.132733
摘要

Macrophages are essential for the maintenance of endothelial cell function. However, the potential impact and mechanisms of crosstalk between macrophages and endothelial cells during silicosis progression remain unexplored. To fill this knowledge gap, a mouse model of silicosis was established. Single cell sequencing, spatial transcriptome sequencing, western blotting, immunofluorescence staining, tube-forming and wound healing assays were used to explore the effects of silicon dioxide on macrophage-endothelial interactions. To investigate the mechanism of macrophage-mediated fibrosis, MMP12 was specifically inactivated using siRNA and pharmacological approaches, and macrophages were depleted using disodium chlorophosphite liposomes. Compared to the normal saline group, the silica dust group showed altered macrophage-endothelial interactions. Matrix metalloproteinase family member MMP12 was identified as a key mediator of the altered function of macrophage-endothelial interactions after silica exposure, which was accompanied by pro-inflammatory macrophage activation and fibrotic progression. By using ablation strategies, macrophage-derived MMP12 was shown to mediate endothelial cell dysfunction by accumulating on the extracellular matrix. During the inflammatory phase of silicosis, MMP12 secreted by pro-inflammatory macrophages caused decreased endothelial cell viability, reduced migration, decreased trans-endothelial resistance and increased permeability; while during the fibrotic phase, macrophage-derived MMP12 sustained endothelial cell injury through accumulation on the extracellular matrix.
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