Novoheart, Vancouver, British Columbia, V6C 2V6, Canada.
Rare Disease Research Unit, Worldwide Research and Development, Pfizer, 610 Main Street, Cambridge, MA, 02139, USA.
Stem Cell Res Ther. 2019 Jul 8;10(1):203. doi: 10.1186/s13287-019-1305-y.
Friedreich's ataxia (FRDA) is an autosomal recessive disease caused by a non-coding mutation in the first intron of the frataxin (FXN) gene that suppresses its expression. Compensatory hypertrophic cardiomyopathy, dilated cardiomyopathy, and conduction system abnormalities in FRDA lead to cardiomyocyte (CM) death and fibrosis, consequently resulting in heart failure and arrhythmias. Murine models have been developed to study disease pathology in the past two decades; however, differences between human and mouse physiology and metabolism have limited the relevance of animal studies in cardiac disease conditions. To bridge this gap, we aimed to generate species-specific, functional in vitro experimental models of FRDA using 2-dimensional (2D) and 3-dimensional (3D) engineered cardiac tissues from FXN-deficient human pluripotent stem cell-derived ventricular cardiomyocytes (hPSC-hvCMs) and to compare their contractile and electrophysiological properties with healthy tissue constructs.
Healthy control and FRDA patient-specific hPSC-hvCMs were derived by directed differentiation using a small molecule-based protocol reported previously. We engineered the hvCMs into our established human ventricular cardiac tissue strip (hvCTS) and human ventricular cardiac anisotropic sheet (hvCAS) models, and functional assays were performed on days 7-17 post-tissue fabrication to assess the electrophysiology and contractility of FRDA patient-derived and FXN-knockdown engineered tissues, in comparison with healthy controls. To further validate the disease model, forced expression of FXN was induced in FXN-deficient tissues to test if disease phenotypes could be rescued.
Here, we report for the first time the generation of human engineered tissue models of FRDA cardiomyopathy from hPSCs: FXN-deficient hvCTS displayed attenuated developed forces (by 70-80%) compared to healthy controls. High-resolution optical mapping of hvCAS with reduced FXN expression also revealed electrophysiological defects consistent with clinical observations, including action potential duration prolongation and maximum capture frequency reduction. Interestingly, a clear positive correlation between FXN expression and contractility was observed (ρ > 0.9), and restoration of FXN protein levels by lentiviral transduction rescued contractility defects in FXN-deficient hvCTS.
We conclude that human-based in vitro cardiac tissue models of FRDA provide a translational, disease-relevant biomimetic platform for the evaluation of novel therapeutics and to provide insight into FRDA disease progression.
弗里德赖希共济失调症(FRDA)是一种常染色体隐性疾病,由 FXN 基因第一内含子中非编码突变引起,该突变抑制其表达。FRDA 导致的代偿性肥厚性心肌病、扩张型心肌病和传导系统异常导致心肌细胞(CM)死亡和纤维化,进而导致心力衰竭和心律失常。在过去的二十年中,已经开发出了用于研究疾病病理学的小鼠模型;然而,人类和小鼠生理学和代谢之间的差异限制了动物研究在心脏疾病条件下的相关性。为了弥合这一差距,我们旨在使用来自 FXN 缺陷的人类多能干细胞衍生的心室心肌细胞(hPSC-hvCM)的 2 维(2D)和 3 维(3D)工程心脏组织生成物种特异性、功能性体外 FRDA 实验模型,并将其与健康组织构建体的收缩和电生理特性进行比较。
通过先前报道的基于小分子的方案,使用定向分化技术从健康对照和 FRDA 患者特异性 hPSC-hvCM 中衍生出健康对照和 FRDA 患者特异性 hPSC-hvCM。我们将 hvCM 工程化到我们已建立的人类心室心脏组织条(hvCTS)和人类心室心脏各向异性片(hvCAS)模型中,并在组织制造后第 7-17 天进行功能测定,以评估 FRDA 患者衍生和 FXN 敲低工程组织的电生理和收缩特性,并与健康对照进行比较。为了进一步验证疾病模型,我们在 FXN 缺陷组织中诱导 FXN 的强制表达,以测试疾病表型是否可以得到挽救。
在这里,我们首次报道了从 hPSC 生成 FRDA 心肌病的人类工程组织模型:与健康对照相比,FXN 缺陷的 hvCTS 显示出收缩力减弱(减少 70-80%)。具有降低 FXN 表达的 hvCAS 的高分辨率光学映射也揭示了与临床观察一致的电生理缺陷,包括动作电位持续时间延长和最大捕获频率降低。有趣的是,观察到 FXN 表达与收缩力之间存在明显的正相关(ρ>0.9),并且通过慢病毒转导恢复 FXN 蛋白水平可挽救 FXN 缺陷的 hvCTS 的收缩力缺陷。
我们得出结论,FRDA 的基于人类的体外心脏组织模型为评估新的治疗方法提供了转化的、与疾病相关的仿生平台,并深入了解 FRDA 疾病的进展。
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