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一种从雪貂心脏高效分离耐钙心室肌细胞的方法及其在电生理研究中的应用。

An efficient isolation procedure of Ca-tolerant ventricular myocytes from ferret heart for applications in electrophysiological studies.

作者信息

Bouron A, Potreau D, Besse C, Raymond G

机构信息

Laboratoire de Physiologie Générale, URA CNRS, Poitiers, France.

出版信息

Biol Cell. 1990;70(3):121-7. doi: 10.1016/0248-4900(90)90367-c.

DOI:10.1016/0248-4900(90)90367-c
PMID:2103519
Abstract

A simple procedure which provides a large yield of isolated ferret ventricular myocytes is described. The enzymatic dissociation was performed by perfusion of the whole heart with the "Langendorff method" at 37 degrees C, without an incubation period. Special attention was given to the period of perfusion with Ca-free or low-calcium containing solutions and to the proportion of both collagenase and elastase used. The viability and calcium tolerance of the isolated cells were tested by ultrastructural and electrophysiological studies. Photo-microscopy showed that 60 to 80% of the isolated cells had an elongated shape (18 microns in diameter, 150 microns in length) and did not beat spontaneously in normal Tyrode solution. The morphological and ultrastructural integrity of these cells was shown in SEM by their smooth surface with regularly spaced T-tubule openings and in TEM by the regular distribution of the transverse tubular system, mitochondrium and sarcomeres. Using the whole-cell patch-clamp technique, they had a resting membrane potential of -72 mV, two types ("Purkinje like" and "ventricular like") of action potentials could be elicited and they were correctly affected by well-known modulators of calcium channels. This technique was successfully applied to the rat heart and could be used for heart dissociation of small mammals. It can simultaneously provide isolated cells of different regions of the heart and can be easily and routinely used by any investigator.

摘要

本文描述了一种能大量分离雪貂心室肌细胞的简单方法。酶解过程采用“Langendorff法”在37℃对整个心脏进行灌注,无需孵育期。特别关注无钙或低钙溶液的灌注时间以及胶原酶和弹性蛋白酶的使用比例。通过超微结构和电生理研究对分离细胞的活力和钙耐受性进行了检测。光学显微镜显示,60%至80%的分离细胞呈细长形(直径18微米,长度150微米),在正常台氏液中不自发搏动。扫描电镜显示这些细胞表面光滑,T小管开口规则分布,透射电镜显示横管系统、线粒体和肌节分布规则,表明这些细胞的形态和超微结构完整。采用全细胞膜片钳技术,它们的静息膜电位为-72mV,可诱发两种类型(“浦肯野样”和“心室样”)的动作电位,且它们能被已知的钙通道调节剂正确影响。该技术已成功应用于大鼠心脏,可用于小型哺乳动物心脏的分离。它能同时提供心脏不同区域的分离细胞,任何研究者都可轻松常规使用。

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An efficient isolation procedure of Ca-tolerant ventricular myocytes from ferret heart for applications in electrophysiological studies.一种从雪貂心脏高效分离耐钙心室肌细胞的方法及其在电生理研究中的应用。
Biol Cell. 1990;70(3):121-7. doi: 10.1016/0248-4900(90)90367-c.
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引用本文的文献

1
Developmental changes in Ca2+ currents from newborn rat cardiomyocytes in primary culture.原代培养新生大鼠心肌细胞Ca2+电流的发育变化
Pflugers Arch. 1994 Oct;428(3-4):241-9. doi: 10.1007/BF00724503.
2
Possible involvement of a chloride conductance in the transient outward current of whole-cell voltage-clamped ferret ventricular myocytes.氯离子电导可能参与全细胞电压钳制的雪貂心室肌细胞的瞬时外向电流。
Pflugers Arch. 1991 Nov;419(5):534-6. doi: 10.1007/BF00370801.