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细胞分离和记录技术对大鼠快速心脏钠电流电压依赖性的影响。

Influence of cell isolation and recording technique on the voltage dependence of the fast cardiac sodium current of the rat.

作者信息

Eickhorn R, Drägert C, Antoni H

机构信息

Physiologisches Institut I, University of Freiburg, Germany.

出版信息

J Mol Cell Cardiol. 1994 Aug;26(8):1095-108. doi: 10.1006/jmcc.1994.1129.

DOI:10.1006/jmcc.1994.1129
PMID:7799448
Abstract

We measured macroscopic sodium currents (INa) in preparations from adult rat ventricle under four different conditions (I-IV): using the cell attached configuration of the tight-seal patch clamp technique on cells isolated with either trypsin followed by collagenase (I) or with collagenase only (II), and using the loose patch technique on cells isolated with collagenase (II) as well as on multicellular preparations not subjected to enzyme treatment (IV). The voltage dependence of the steady-state activation of INa as well as of the steady-state inactivation differed significantly among condition I and II. Moreover, the recordings were voltage shifted in comparison to the recording condition III and IV. The potentials of half maximal activation and inactivation were: [sequence data: see text] The shift of inactivation was time dependent and continued after 3-5 min after the seal formation in condition I, but not in condition II. No time dependent shift was found in III and IV. We conclude, that the voltage dependence of cardiac sodium current is shifted by gigaseal patch recording. The degree of this shift depends on the type of enzymatic isolation procedure, with trypsin causing more pronounced effects than collagenase. The cell isolation itself seems not to interfere with the voltage dependence of INa, since loose patch recordings from multicellular preparations and from single cells isolated with collagenase show no obvious differences.

摘要

我们在四种不同条件(I - IV)下测量了成年大鼠心室标本中的宏观钠电流(INa):使用紧密密封膜片钳技术的细胞贴附模式,分别对用胰蛋白酶随后用胶原酶分离的细胞(I)或仅用胶原酶分离的细胞(II)进行测量,以及对用胶原酶分离的细胞(III)和未经过酶处理的多细胞标本(IV)使用松散膜片技术进行测量。I和II条件下,INa稳态激活以及稳态失活的电压依赖性存在显著差异。此外,与记录条件III和IV相比,记录的电压发生了偏移。半数最大激活和失活的电位为:[序列数据:见正文]。失活的偏移是时间依赖性的,在条件I中,封接形成后3 - 5分钟仍持续存在,但在条件II中没有。在III和IV中未发现时间依赖性偏移。我们得出结论,千兆封接膜片记录会改变心脏钠电流的电压依赖性。这种偏移的程度取决于酶促分离程序的类型,胰蛋白酶比胶原酶产生更明显的影响。细胞分离本身似乎不会干扰INa的电压依赖性,因为从多细胞标本和用胶原酶分离的单细胞进行的松散膜片记录没有明显差异。

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