A Platform Integrating Biophysical and Biochemical Stimuli to Enhance Differentiation and Maturation of Cardiomyocyte Subtypes Derived from Human Induced Pluripotent Stem Cells.

IF 2.3 4区 医学 Q2 CARDIAC & CARDIOVASCULAR SYSTEMS Journal of Cardiovascular Development and Disease Pub Date : 2025-02-04 DOI:10.3390/jcdd12020056
Zhonggang Feng, Kota Sawada, Iori Ando, Riku Yoshinari, Daisuke Sato, Tadashi Kosawada
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Abstract

To enhance the differentiation and maturation of cardiomyocytes derived from human induced pluripotent stem cells, we developed a bioreactor system that simultaneously imposes biophysical and biochemical stimuli on these committed cardiomyocytes. The cells were cultured within biohydrogels composed of the extracellular matrix extracted from goat ventricles and purchased rat-origin collagen, which were housed in the elastic PDMS culture chambers of the bioreactor. Elastic and flexible electrodes composed of PEDOT/PSS, latex, and graphene flakes were embedded in the hydrogels and chamber walls, allowing cyclic stretch and electrical pulses to be simultaneously and coordinately applied to the cultured cells. Furthermore, a dynamic analysis method employing the transverse forced oscillation theory of a cantilever was used to analyze and discriminate the subtype-specific beating behavior of the cardiomyocytes. It was found that myosin light chain 2v (MLC2v), a ventricular cell marker, was primarily upregulated in cells aggregated on the (+) electrode side, while cardiomyocytes with faint MLC2v but strong cardiac troponin T (cTNT) expression aggregated at the ground electrode (GND) side. mRNA analysis using rtPCR and the gel beating dynamics further suggested a subtype deviation on the different electrode sides. This study demonstrated the potential of our bioreactor system in enhancing cardiac differentiation and maturation, and it showed an intriguing phenomenon of cardiomyocyte subtype aggregation on different electrodes, which may be developed into a new method to enhance the maturation and separation of cardiomyocyte subtypes.

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一个整合生物物理和生化刺激的平台,以促进人类诱导多能干细胞衍生的心肌细胞亚型的分化和成熟。
为了增强人类诱导多能干细胞衍生的心肌细胞的分化和成熟,我们开发了一种生物反应器系统,同时对这些心肌细胞施加生物物理和生化刺激。细胞被培养在由从山羊脑室提取的细胞外基质和购买的大鼠胶原组成的生物水凝胶中,这些水凝胶被安置在生物反应器的弹性PDMS培养室中。由PEDOT/PSS、乳胶和石墨烯薄片组成的弹性和柔性电极嵌入水凝胶和室壁,使循环拉伸和电脉冲同时协调地施加于培养细胞。此外,采用悬臂梁横向强迫振荡理论的动力学分析方法,分析和区分了心肌细胞的亚型特异性跳动行为。结果发现,心室细胞标志物肌球蛋白轻链2v (MLC2v)主要在聚集在(+)电极侧的细胞中上调,而MLC2v表达微弱但心肌肌钙蛋白T (cTNT)表达强烈的心肌细胞聚集在地电极(GND)侧。利用rtPCR和凝胶加热动力学分析mRNA进一步表明,不同电极侧存在亚型偏差。本研究证明了我们的生物反应器系统在促进心脏分化和成熟方面的潜力,并显示了心肌细胞亚型聚集在不同电极上的有趣现象,这可能成为促进心肌细胞亚型成熟和分离的新方法。
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来源期刊
Journal of Cardiovascular Development and Disease
Journal of Cardiovascular Development and Disease CARDIAC & CARDIOVASCULAR SYSTEMS-
CiteScore
2.60
自引率
12.50%
发文量
381
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