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用于检测成对心肌细胞间细胞间偶联的微流控系统。

Microfluidic systems to examine intercellular coupling of pairs of cardiac myocytes.

作者信息

Klauke Norbert, Smith Godfrey, Cooper Jonathan M

机构信息

Department of Electronics, University of Glasgow, Glasgow, UK G12 8LT.

出版信息

Lab Chip. 2007 Jun;7(6):731-9. doi: 10.1039/b706175g. Epub 2007 May 17.

Abstract

In this paper we describe a microfluidic environment that enables us to explore cell-to-cell signalling between longitudinally linked primary heart cells. We have chosen to use pairs (or doublets) of cardiac myocyte as a model system, not only because of the importance of cell-cell signalling in the study of heart disease but also because the single cardiomyocytes are both mechanically and electrically active and their synchronous activation due to the intercellular coupling within the doublet can be readily monitored on optical and electrical recordings. Such doublets have specialised intercellular contact structures in the form of the intercalated discs, comprising the adhesive junction (fascia adherens and macula adherens or desmosome) and the connecting junction (known as gap junction). The latter structure enables adjacent heart cells to share ions, second messengers and small metabolites (<1 kDa) between them and thus provides the structural basis for the synchronous (syncytical) behaviour of connected cardiomyocytes. Using the unique environment provided by the microfluidic system, described in this paper, we explore the local ionic conditions that enable the propagation of Ca(2+) waves between two heart cells. We observe that the ability of intracellular Ca(2+) waves to traverse the intercalated discs is dependent on the relative concentrations of diastolic Ca(2+) in the two adjacent cells. These experiments rely upon our ability to independently control both the electrical stimulation of each of the cells (using integrated microelectrodes) and to rapidly change (or switch) the local concentrations of ions and drugs in the extracellular buffer within the microfluidic channel (using a nanopipetting system). Using this platform, it is also possible to make simultaneous optical recordings (including fluorescence and cell contraction) to explore the effect of drugs on one or both cells, within the doublet.

摘要

在本文中,我们描述了一种微流控环境,该环境使我们能够探索纵向连接的原代心脏细胞之间的细胞间信号传导。我们选择使用心肌细胞对(或双联体)作为模型系统,这不仅是因为细胞间信号传导在心脏病研究中的重要性,还因为单个心肌细胞在机械和电方面都具有活性,并且由于双联体内的细胞间耦合导致的同步激活可以在光学和电记录中很容易地监测到。这种双联体具有以闰盘形式存在的特殊细胞间接触结构,闰盘包括黏附连接(黏合带和黏着斑或桥粒)和连接连接(即缝隙连接)。后一种结构使相邻的心脏细胞能够在它们之间共享离子、第二信使和小代谢物(<1 kDa),从而为相连心肌细胞的同步(合胞体)行为提供了结构基础。利用本文所述微流控系统提供的独特环境,我们探索了使Ca(2+)波在两个心脏细胞之间传播的局部离子条件。我们观察到细胞内Ca(2+)波穿越闰盘的能力取决于两个相邻细胞中舒张期Ca(2+)的相对浓度。这些实验依赖于我们独立控制每个细胞电刺激(使用集成微电极)以及快速改变(或切换)微流控通道内细胞外缓冲液中离子和药物局部浓度(使用纳米移液系统)的能力。利用这个平台,还可以进行同步光学记录(包括荧光和细胞收缩),以探索药物对双联体中一个或两个细胞的影响。

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