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Methods for the Isolation Culture and Functional Characterization of Sinoatrial Node Myocytes from Adult Mice

机译:成年小鼠鼻窦房结肌细胞的分离培养和功能鉴定方法

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摘要

Sinoatrial node myocytes (SAMs) act as the natural pacemakers of the heart, initiating each heart beat by generating spontaneous action potentials (APs). These pacemaker APs reflect the coordinated activity of numerous membrane currents and intracellular calcium cycling. However the precise mechanisms that drive spontaneous pacemaker activity in SAMs remain elusive. Acutely isolated SAMs are an essential preparation for experiments to dissect the molecular basis of cardiac pacemaking. However, the indistinct anatomy, complex microdissection, and finicky enzymatic digestion conditions have prevented widespread use of acutely isolated SAMs. In addition, methods were not available until recently to permit longer-term culture of SAMs for protein expression studies. Here we provide a step-by-step protocol and video demonstration for the isolation of SAMs from adult mice. A method is also demonstrated for maintaining adult mouse SAMs in vitro and for expression of exogenous proteins via adenoviral infection. Acutely isolated and cultured SAMs prepared via these methods are suitable for a variety of electrophysiological and imaging studies.
机译:窦房结肌细胞(SAM)充当心脏的自然起搏器,通过产生自发动作电位(AP)来启动每个心跳。这些起搏器AP反映了许多膜电流和细胞内钙循环的协调活动。但是,驱动SAM中自发性起搏器活动的精确机制仍然难以捉摸。急性分离的SAM是解剖心脏起搏的分子基础的实验必不可少的准备。但是,解剖结构模糊,显微解剖复杂和酶促消化条件复杂,阻止了急性分离的SAM的广泛使用。此外,直到最近才允许将SAM长期培养用于蛋白质表达研究的方法。在这里,我们提供了从成年小鼠中分离SAM的分步协议和视频演示。还证明了一种在体外维持成年小鼠SAM并通过腺病毒感染表达外源蛋白的方法。通过这些方法制备的急性分离和培养的SAM适用于各种电生理和影像学研究。

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