Desmoplakin mutations in cardiac fibroblasts cause TGF?1-mediated pathological fibrogenesis in desmoplakin cardiomyopathy via beclin-1 regulation

HS Vincent Chen, Chuanyu Wei, Shing Fai Chan, Ardan M Saguner, Corinna B Brunckhorst, Firat Duru, Joseph E. Marine, Cynthia A. James, Hugh Calkins, Daniel Judge, Weinian Shou
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Abstract

Background: Pathological fibrosis is a major finding in cardiovascular diseases and can result in arrhythmia and heart failure. Desmosome gene mutations can lead to arrhythmogenic cardiomyopathy (ACM). Among ACM, pathogenic desmoplakin (DSP) variants cause a distinctive cardiomyopathy with excessive cardiac fibrosis that could precede ventricular dysfunction. DSP variants are also linked to other fibrotic diseases. Whether DSP plays any role in pathological fibrosis remain unknown. Methods: Mesenchymal stromal cells (MSCs) are resident fibroblast-like cells that are responsible for fibrogenesis in most organs, including hearts. We first used unbiased genome-wide analyses to generate cardiac fibroblasts-like, induced pluripotent stem cell-derived MSCs from normal donors and ACM patients with DSP mutations. We then studied the fibrogenic responses of cardiac MSCs to transforming growth factor beta-1 (TGF-?1) using Western/Co-IP, autophagy assay, gene knockdowns/over-expressions, genomic analyses, mouse DSP knockdown models, immunostaining, and qPCR. Results: TGF?1 induced excessive accumulations of vimentin (VIM)/fibrillar collagens, and over-activated fibrotic genes in DSP-mutant MSCs when compared to normal MSCs. In normal MSCs, VIMs bind to wild-type DSP during normal fibrogenesis after TGF?1. DSP-mutant MSCs exhibited a haploinsufficient phenotype with increased DSP-unbound VIMs that sequestered beclin-1 (BECN1) from activating autophagy and caveolin-1 (CAV1)-mediated endocytosis. Decreased autophagy caused collagen accumulations and diminished CAV1 endocytosis resulted in abnormal CAV1 plaque formation that over-activated fibrotic genes [COL1A1, COL3A1, and fibronectin (FN)] via heightened p38 activities after TGF?1. Genome-wide analysis and DSP knockdown in mouse fibroblasts confirmed this novel role of DSP mutations in pathological fibrosis. Overexpression of VIM-binding domains of DSP could suppress pathological fibrosis by increasing collagen autophagic degradation and decreasing fibrotic gene expressions. Conclusions: Our data reveal that DSP deficiency in MSCs/fibroblasts leads to exaggerated fibrogenesis in DSP-cardiomyopathy by decreasing BECN1 availability for autophagy and CAV1-endocytosis. Overexpression of VIM binding domains of DSP could be a new strategy to treat pathological fibrosis.
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心脏成纤维细胞中的去瘤素突变通过beclin-1调控导致去瘤素心肌病中TGF?1介导的病理性纤维形成
背景:病理纤维化是心血管疾病的主要表现,可导致心律失常和心力衰竭。脱丝体基因突变可导致心律失常性心肌病(ACM)。在致心律失常性心肌病中,致病性去疱疹病毒蛋白(DSP)变体会导致一种独特的心肌病,其心脏过度纤维化可能先于心室功能障碍。DSP 变体还与其他纤维化疾病有关。DSP 是否在病理纤维化中扮演任何角色仍是未知数。研究方法间充质基质细胞(MSCs)是常驻的成纤维细胞样细胞,在包括心脏在内的大多数器官中负责纤维形成。我们首先利用无偏见的全基因组分析,从正常供体和DSP突变的ACM患者中生成心脏成纤维细胞样、诱导多能干细胞衍生的间充质干细胞。然后,我们使用 Western/Co-IP、自噬检测、基因敲除/过度表达、基因组分析、小鼠 DSP 敲除模型、免疫染色和 qPCR 等方法研究了心脏间充质干细胞对转化生长因子 beta-1(TGF-?1)的纤维化反应。结果与正常间充质干细胞相比,TGF?1能诱导DSP突变间充质干细胞中的波形蛋白(VIM)/纤维胶原过度累积,并过度激活纤维化基因。在正常间充质干细胞中,TGF?1后正常纤维生成过程中,VIMs与野生型DSP结合。DSP突变的间充质干细胞表现出单倍体不足的表型,DSP未结合的VIMs增加,从而封存了beclin-1(BECN1),使其无法激活自噬和洞穴素-1(CAV1)介导的内吞。自噬减少导致胶原蛋白积累,CAV1 内吞减少导致异常的 CAV1 斑块形成,TGF?1 之后,CAV1 斑块通过增强的 p38 活性过度激活纤维化基因[COL1A1、COL3A1 和纤维连接蛋白 (FN)]。全基因组分析和小鼠成纤维细胞中的 DSP 敲除证实了 DSP 突变在病理纤维化中的新作用。过表达 DSP 的 VIM 结合域可通过增加胶原蛋白自噬降解和减少纤维化基因表达来抑制病理性纤维化。结论:我们的数据显示,间充质干细胞/成纤维细胞中 DSP 的缺乏会降低 BECN1 自噬和 CAV1 内吞的可用性,从而导致 DSP-心肌病的纤维化。过表达DSP的VIM结合域可能是治疗病理性纤维化的一种新策略。
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