Contraction pressure analysis using optical imaging in normal and MYBPC3-mutated hiPSC-derived cardiomyocytes grown on matrices with tunable stiffness

Q3 Biochemistry, Genetics and Molecular Biology Biomaterials and biosystems Pub Date : 2022-12-01 DOI:10.1016/j.bbiosy.2022.100068
Matthijs Snelders , Iris H. Koedijk , Julia Schirmer , Otto Mulleners , Juancito van Leeuwen , Nathalie P. de Wagenaar , Oscar Bartulos , Pieter Voskamp , Stefan Braam , Zeno Guttenberg , A.H. Jan Danser , Danielle Majoor-Krakauer , Erik Meijering , Ingrid van der Pluijm , Jeroen Essers
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引用次数: 1

Abstract

Current in vivo disease models and analysis methods for cardiac drug development have been insufficient in providing accurate and reliable predictions of drug efficacy and safety. Here, we propose a custom optical flow-based analysis method to quantitatively measure recordings of contracting cardiomyocytes on polydimethylsiloxane (PDMS), compatible with medium-throughput systems.

Movement of the PDMS was examined by covalently bound fluorescent beads on the PDMS surface, differences caused by increased substrate stiffness were compared, and cells were stimulated with β-agonist. We further validated the system using cardiomyocytes treated with endothelin-1 and compared their contractions against control and cells incubated with receptor antagonist bosentan. After validation we examined two MYBPC3-mutant patient-derived cell lines.

Recordings showed that higher substrate stiffness resulted in higher contractile pressure, while beating frequency remained similar to control. β-agonist stimulation resulted in both higher beating frequency as well as higher pressure values during contraction and relaxation. Cells treated with endothelin-1 showed an increased beating frequency, but a lower contraction pressure. Cells treated with both endothelin-1 and bosentan remained at control level of beating frequency and pressure. Lastly, both MYBPC3-mutant lines showed a higher beating frequency and lower contraction pressure.

Our validated method is capable of automatically quantifying contraction of hiPSC-derived cardiomyocytes on a PDMS substrate of known shear modulus, returning an absolute value. Our method could have major benefits in a medium-throughput setting.

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使用光学成像分析在硬度可调基质上生长的正常和mybpc3突变的hipsc衍生心肌细胞的收缩压力
目前用于心脏药物开发的体内疾病模型和分析方法不足以提供准确可靠的药物疗效和安全性预测。在这里,我们提出了一种定制的基于光流的分析方法来定量测量收缩心肌细胞在聚二甲基硅氧烷(PDMS)上的记录,与中等通量系统兼容。通过在PDMS表面的共价结合荧光珠检测PDMS的运动,比较底物硬度增加引起的差异,并用β-激动剂刺激细胞。我们用内皮素-1处理的心肌细胞进一步验证了该系统,并比较了它们与对照组和受体拮抗剂波生坦孵育的细胞的收缩。验证后,我们检测了两种mybpc3突变患者来源的细胞系。记录显示,较高的基材刚度导致较高的收缩压力,而敲打频率保持与控制相似。β-激动剂刺激导致心跳频率升高,收缩和舒张时的压力值也升高。内皮素-1处理的细胞搏动频率增加,收缩压力降低。内皮素-1和波生坦处理后的细胞搏动频率和压力均维持在控制水平。最后,两种mybpc3突变系均表现出较高的跳动频率和较低的收缩压力。我们验证的方法能够自动量化hipsc衍生的心肌细胞在已知剪切模量的PDMS底物上的收缩,并返回绝对值。我们的方法在中等吞吐量设置中具有主要优势。
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25 days
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