4.4 Article

Isolation of Human Ventricular Cardiomyocytes from Vibratome-Cut Myocardial Slices

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出版社

JOURNAL OF VISUALIZED EXPERIMENTS
DOI: 10.3791/61167

关键词

Biology; Issue 159; human; heart failure; myocardial slices; cardiomyocyte isolation; vibratome; contractile myocytes; calcium imaging; cardiac excitation-contraction coupling

资金

  1. DZHK (German Centre for Cardiovascular Research)
  2. Interdisciplinary Centre for Clinical Research (IZKF) at the University Hospital of the University of Erlangen-Nurnberg
  3. Universitatsbund Erlangen-Nurnberg

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The isolation of ventricular cardiac myocytes from animal and human hearts is a fundamental method in cardiac research. Animal cardiomyocytes are commonly isolated by coronary perfusion with digestive enzymes. However, isolating human cardiomyocytes is challenging because human myocardial specimens usually do not allow for coronary perfusion, and alternative isolation protocols result in poor yields of viable cells. In addition, human myocardial specimens are rare and only regularly available at institutions with on-site cardiac surgery. This hampers the translation of findings from animal to human cardiomyocytes. Described here is a reliable protocol that enables efficient isolation of ventricular myocytes from human and animal myocardium. To increase the surface-to-volume ratio while minimizing cell damage, myocardial tissue slices 300 mu m thick are generated from myocardial specimens with a vibratome. Tissue slices are then digested with protease and collagenase. Rat myocardium was used to establish the protocol and quantify yields of viable, calcium-tolerant myocytes by flow-cytometric cell counting. Comparison with the commonly used tissue-chunk method showed significantly higher yields of rod-shaped cardiomyocytes (41.5 +/- 11.9 vs. 7.89 +/- 3.6%, p < 0.05). The protocol was translated to failing and non-failing human myocardium, where yields were similar as in rat myocardium and, again, markedly higher than with the tissue-chunk method (45.0 +/- 15.0 vs. 6.87 +/- 5.23 cells/mg, p < 0.05). Notably, with the protocol presented it is possible to isolate reasonable numbers of viable human cardiomyocytes (9-200 cells/mg) from minimal amounts of tissue (<50 mg). Thus, the method is applicable to healthy and failing myocardium from both human and animal hearts. Furthermore, it is possible to isolate excitable and contractile myocytes from human tissue specimens stored for up to 36 h in cold cardioplegic solution, rendering the method particularly useful for laboratories at institutions without on-site cardiac surgery.

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