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缝隙连接选择性的定量分析。

Quantification of gap junction selectivity.

作者信息

Ek-Vitorín Jose F, Burt Janis M

机构信息

Dept. of Physiology, Univ. of Arizona, PO Box 245051, Tucson, AZ 85724-5051, USA.

出版信息

Am J Physiol Cell Physiol. 2005 Dec;289(6):C1535-46. doi: 10.1152/ajpcell.00182.2005. Epub 2005 Aug 10.

DOI:10.1152/ajpcell.00182.2005
PMID:16093281
Abstract

Gap junctions, which are essential for functional coordination and homeostasis within tissues, permit the direct intercellular exchange of small molecules. The abundance and diversity of this exchange depends on the number and selectivity of the comprising channels and on the transjunctional gradient for and chemical character of the permeant molecules. Limited knowledge of functionally significant permeants and poor detectability of those few that are known have made it difficult to define channel selectivity. Presented herein is a multifaceted approach to the quantification of gap junction selectivity that includes determination of the rate constant for intercellular diffusion of a fluorescent probe (k2-DYE) and junctional conductance (gj) for each junction studied, such that the selective permeability (k2-DYE/gj) for dyes with differing chemical characteristics or junctions with differing connexin (Cx) compositions (or treatment conditions) can be compared. In addition, selective permeability can be correlated using single-channel conductance when this parameter is also measured. Our measurement strategy is capable of detecting 1) rate constants and selective permeabilities that differ across three orders of magnitude and 2) acute changes in that rate constant. Using this strategy, we have shown that 1) the selective permeability of Cx43 junctions to a small cationic dye varied across two orders of magnitude, consistent with the hypothesis that the various channel configurations adopted by Cx43 display different selective permeabilities; and 2) the selective permeability of Cx37 vs. Cx43 junctions was consistently and significantly lower.

摘要

间隙连接对于组织内的功能协调和内环境稳定至关重要,它允许小分子在细胞间直接交换。这种交换的丰富性和多样性取决于组成通道的数量和选择性,以及通透分子的跨连接梯度和化学性质。对于功能上重要的通透分子了解有限,且已知的少数通透分子的可检测性较差,这使得难以定义通道选择性。本文介绍了一种多方面的方法来量化间隙连接选择性,包括测定荧光探针细胞间扩散的速率常数(k2-DYE)和所研究的每个连接的连接电导(gj),以便能够比较具有不同化学特性的染料或具有不同连接蛋白(Cx)组成(或处理条件)的连接的选择性通透性(k2-DYE/gj)。此外,当也测量单通道电导时,选择性通透性可以与之相关联。我们的测量策略能够检测到:1)速率常数和选择性通透性在三个数量级上存在差异;2)该速率常数的急性变化。使用这种策略,我们已经表明:1)Cx43连接对一种小阳离子染料的选择性通透性在两个数量级上变化,这与Cx43采用的各种通道构型显示不同选择性通透性的假设一致;2)Cx37与Cx43连接的选择性通透性始终且显著更低。

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Quantification of gap junction selectivity.缝隙连接选择性的定量分析。
Am J Physiol Cell Physiol. 2005 Dec;289(6):C1535-46. doi: 10.1152/ajpcell.00182.2005. Epub 2005 Aug 10.
2
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