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用于细胞信号传导和体外心肌肥大研究的成年小鼠心肌细胞的分离与培养。

Isolation and culture of adult mouse cardiomyocytes for cell signaling and in vitro cardiac hypertrophy.

作者信息

Li Daxiang, Wu Jian, Bai Yan, Zhao Xiaochen, Liu Lijun

机构信息

Department of Biochemistry and Cancer Biology, University of Toledo College of Medicine and Life Sciences.

Department of Physiology and Pharmacology, University of Toledo College of Medicine and Life Sciences.

出版信息

J Vis Exp. 2014 May 21(87):51357. doi: 10.3791/51357.

Abstract

Technological advances have made genetically modified mice, including transgenic and gene knockout mice, an essential tool in many research fields. Adult cardiomyocytes are widely accepted as a good model for cardiac cellular physiology and pathophysiology, as well as for pharmaceutical intervention. Genetically modified mice preclude the need for complicated cardiomyocyte infection processes to generate the desired genotype, which are inefficient due to cardiomyocytes' terminal differentiation. Isolation and culture of high quantity and quality functional cardiomyocytes will dramatically benefit cardiovascular research and provide an important tool for cell signaling transduction research and drug development. Here, we describe a well-established method for isolation of adult mouse cardiomyocytes that can be implemented with little training. The mouse heart is excised and cannulated to an isolated heart system, then perfused with a calcium-free and high potassium buffer followed by type II collagenase digestion in Langendorff retrograde perfusion mode. This protocol yields a consistent result for the collection of functional adult mouse cardiomyocytes from a variety of genetically modified mice.

摘要

技术进步使转基因小鼠,包括转基因小鼠和基因敲除小鼠,成为许多研究领域的重要工具。成年心肌细胞被广泛认为是心脏细胞生理学、病理生理学以及药物干预的良好模型。转基因小鼠无需进行复杂的心肌细胞感染过程来产生所需的基因型,因为心肌细胞的终末分化导致这些过程效率低下。分离和培养大量高质量的功能性心肌细胞将极大地促进心血管研究,并为细胞信号转导研究和药物开发提供重要工具。在此,我们描述一种成熟的成年小鼠心肌细胞分离方法,该方法几乎无需培训即可实施。切除小鼠心脏并插管至离体心脏系统,然后用无钙高钾缓冲液灌注,接着以Langendorff逆行灌注模式进行II型胶原酶消化。该方案对于从各种转基因小鼠中收集功能性成年小鼠心肌细胞产生一致的结果。

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