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淡水狭盐性金鱼原代培养鳃上皮细胞的渗透特性和闭合蛋白表达。

Permeability properties and occludin expression in a primary cultured model gill epithelium from the stenohaline freshwater goldfish.

机构信息

Department of Biology, York University, 4700 Keele Street, Toronto, ON, M3J 1P3, Canada.

出版信息

J Comp Physiol B. 2011 May;181(4):487-500. doi: 10.1007/s00360-010-0535-1. Epub 2010 Nov 18.

Abstract

Techniques for the primary culture of fish gill epithelia on permeable supports have provided 'reconstructed' gill models appropriate for the study of gill permeability characteristics in vitro. Models developed thus far have been derived from euryhaline fish species that can tolerate a wide range of environmental salinity. This study reports on procedures for the primary culture of a model gill epithelium derived from goldfish, a stenohaline freshwater (FW) fish that cannot tolerate high environmental salt concentrations. The reconstructed goldfish gill epithelium was cultured on permeable filter inserts and using electron microscopy and immunocytochemical techniques, was determined to be composed exclusively of gill pavement cells. When cultured under symmetrical conditions (i.e. with culture medium bathing both apical and basolateral surfaces), epithelial preparations generated appreciable transepithelial resistance (TER) (e.g. 1,150 ± 46 Ωcm(2)) within 36-42 h post-seeding in inserts. When apical medium was replaced with FW (asymmetrical conditions to mimic conditions that occur in vivo), epithelia exhibited increased TER and elevated paracellular permeability. Changes in permeability occurred in association with altered occludin-immunoreactive band position by western blot and no change in occludin mRNA abundance. We contend that the goldfish gill model will provide a useful in vitro tool for examining the molecular components of a stenohaline fish gill epithelium that participate in the regulation of gill permeability. The model will allow molecular observations to be made together with assessment of changing physiological properties that relate to permeability. Together, this will allow further insight into mechanisms that regulate gill permeability in fishes.

摘要

在可渗透支持物上对鱼类鳃上皮细胞进行原代培养的技术为体外研究鳃通透性特性提供了“重建”的鳃模型。迄今为止,所开发的模型源自能够耐受广泛环境盐度范围的广盐性鱼类物种。本研究报告了从金鱼(一种不能耐受高环境盐浓度的狭盐性淡水(FW)鱼类)中获得模型鳃上皮细胞的原代培养程序。重建的金鱼鳃上皮细胞在可渗透的滤器插入物上进行培养,并通过电子显微镜和免疫细胞化学技术,确定仅由鳃扁细胞组成。当在对称条件(即培养基同时浸浴上皮细胞的顶侧和基底外侧表面)下进行培养时,上皮细胞在插入物中培养 36-42 小时后即可产生可观的跨上皮电阻(TER)(例如 1,150 ± 46 Ωcm2)。当用 FW 替换顶侧培养基(非对称条件以模拟体内发生的情况)时,上皮细胞表现出增加的 TER 和升高的旁细胞通透性。通透性的变化与通过western blot 改变封闭蛋白免疫反应性带位置以及封闭蛋白 mRNA 丰度没有变化相关。我们认为,金鱼鳃模型将为研究参与调节鳃通透性的狭盐性鱼类鳃上皮细胞的分子组成提供有用的体外工具。该模型将允许进行分子观察,并评估与通透性相关的生理特性变化。两者结合将使我们进一步了解调节鱼类鳃通透性的机制。

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