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HSPA12A acts as a scaffolding protein to inhibit cardiac fibroblast activation and cardiac fibrosis

心脏纤维化 肌成纤维细胞 下调和上调 纤维化 基因敲除 纤维连接蛋白 环己酰亚胺 MG132型 支架蛋白 细胞生物学 化学 生物 癌症研究 内科学 分子生物学 细胞外基质 医学 信号转导 蛋白质生物合成 细胞凋亡 生物化学 蛋白酶体抑制剂 蛋白酶体 基因
作者
Qian Mao,Xiaojin Zhang,Jinna Yang,Qiuyue Kong,Hao Cheng,Wansu Yu,Xiaofei Cao,Yuehua Li,Chuanfu Li,Li Liu,Zhengnian Ding
出处
期刊:Journal of Advanced Research [Elsevier]
标识
DOI:10.1016/j.jare.2024.01.012
摘要

Cardiac fibrosis is the main driver for adverse remodeling and progressive functional decline in nearly all types of heart disease including myocardial infarction (MI). The activation of cardiac fibroblasts (CF) into myofibroblasts is responsible for cardiac fibrosis. Unfortunately, no ideal approach for controlling CF activation currently exists. This study investigated the role of Heat shock protein 12A (HSPA12A), an atypical member of the HSP70 family, in CF activation and MI-induced cardiac fibrosis. Primary CF and Hspa12a knockout mice were used in the experiments. CF activation was indicated by the upregulation of myofibroblast characters including alpha-Smooth muscle actin (αSMA), Collagen, and Fibronectin. Cardiac fibrosis was illustrated by Masson’s trichrome and picrosirius staining. Cardiac function was examined using echocardiography. Glycolytic activity was indicated by levels of extracellular lactate and the related protein expression. Protein stability was examined following cycloheximide and MG132 treatment. Protein-protein interaction was examined by immunoprecipitation-immunoblotting analysis. HSPA12A displayed a high expression level in quiescent CF but showed a decreased expression in activated CF, while ablation of HSPA12A in mice promoted CF activation and cardiac fibrosis following MI. HSPA12A overexpression inhibited the activation of primary CF through inhibiting glycolysis, while HSPA12A knockdown showed the opposite effects. Moreover, HSPA12A upregulated the protein expression of transcription factor p53, by which mediated the HSPA12A-induced inhibition of glycolysis and CF activation. Mechanistically, this action of HSPA12A was achieved by acting as a scaffolding protein to bind p53 and ubiquitin specific protease 10 (USP10), thereby promoting the USP10-mediated p53 protein stability and the p53-medicated glycolysis inhibition. The present study provided clear evidence that HSPA12A is a novel endogenous inhibitor of CF activation and cardiac fibrosis. Targeting HSPA12A in CF could represent a promising strategy for the management of cardiac fibrosis in patients.
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