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Tissue Contraction Force Microscopy for Optimization of Engineered Cardiac Tissue

机译:组织收缩力显微镜用于优化工程心脏组织

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摘要

We developed a high-throughput screening assay that allows for relative comparison of the twitch force of millimeter-scale gel-based cardiac tissues. This assay is based on principles taken from traction force microscopy and uses fluorescent microspheres embedded in a soft polydimethylsiloxane (PDMS) substrate. A gel-forming cell suspension is simply pipetted onto the PDMS to form hemispherical cardiac tissue samples. Recordings of the fluorescent bead movement during tissue pacing are used to determine the maximum distance that the tissue can displace the elastic PDMS substrate. In this study, fibrin gel hemispheres containing human induced pluripotent stem cell-derived cardiomyocytes were formed on the PDMS and allowed to culture for 9 days. Bead displacement values were measured and compared to direct force measurements to validate the utility of the system. The amplitude of bead displacement correlated with direct force measurements, and the twitch force generated by the tissues was the same in 2 and 4 mg/mL fibrin gels, even though the 2 mg/mL samples visually appear more contractile if the assessment were made on free-floating samples. These results demonstrate the usefulness of this assay as a screening tool that allows for rapid sample preparation, data collection, and analysis in a simple and cost-effective platform.
机译:我们开发了一种高通量筛选测定法,该测定法可以相对比较基于毫米级凝胶的心脏组织的抽搐力。该测定法基于从牵引力显微镜获得的原理,并使用嵌入在柔软的聚二甲基硅氧烷(PDMS)基质中的荧光微球。只需将形成凝胶的细胞悬液移至PDMS上,即可形成半球形心脏组织样本。组织起搏期间荧光珠运动的记录用于确定组织可以移位弹性PDMS基底的最大距离。在这项研究中,在PDMS上形成了包含人诱导的多能干细胞衍生的心肌细胞的纤维蛋白凝胶半球,并培养9天。测量了胎圈位移值,并将其与直接力测量值进行比较,以验证系统的实用性。珠位移的幅度与直接力的测量值相关,并且在2和4μmg/ mL纤维蛋白凝胶中,组织产生的抽搐力相同,即使2μmg/ mL样品在视觉上看起来更收缩,自由浮动的样本。这些结果证明了该测定作为筛选工具的有用性,该筛选工具允许在简单且经济高效的平台上快速进行样品制备,数据收集和分析。

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