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Enrichment of neonatal rat cardiomyocytes in primary culture facilitates long-term maintenance of contractility in vitro

机译:在原代培养物中富集新生大鼠心肌细胞有助于长期保持体外收缩力

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摘要

Long-term culture of primary neonatal rat cardiomyocytes is limited by the loss of spontaneous contractile phenotype within weeks in culture. This may be due to loss of contractile cardiomyocytes from the culture or overgrowth of the non-cardiomyocyte population. Using the mitochondria specific fluorescent dye, tetramethylrhodamine methyl ester perchlorate (TMRM), we showed that neonatal rat cardiomyocytes enriched by fluorescence-activated cell sorting can be maintained as contractile cultures for long periods (24-wk culture vs. 2 wk for unsorted cardiomyocytes). Long-term culture of this purified cardiomyocyte (TMRM high) population retained the expression of cardiomyocyte markers, continued calcium cycling, and displayed cyclic electrical activity that could be regulated pharmacologically. These findings suggest that non-cardiomyocyte populations can negatively influence contractility of cardiomyocytes in culture and that by purifying cardiomyocytes, the cultures retain potential as an experimental model for longitudinal studies of cardiomyocyte biology in vitro.
机译:原代新生大鼠心肌细胞的长期培养受到培养数周内自发收缩表型丧失的限制。这可能是由于培养的收缩性心肌细胞丢失或非心肌细胞群体过度生长所致。使用线粒体特异的荧光染料四甲基罗丹明甲酯高氯酸盐(TMRM),我们显示了通过荧光激活细胞分选富集的新生大鼠心肌细胞可以长期保持收缩培养(24周培养,而未分选的心肌细胞为2周) 。长期培养的这种纯化的心肌细胞(TMRM高)群体保留了心肌细胞标志物的表达,持续的钙循环以及显示可以通过药理学调节的循环电活动。这些发现表明,非心肌细胞群体可对培养物中的心肌细胞收缩性产生负面影响,并且通过纯化心肌细胞,培养物保留了作为体外纵向研究心肌细胞生物学实验模型的潜力。

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