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苯那明敏感的钠离子内流在虹鳟鱼离体鳃上皮细胞中的定位与特性研究

Localization and characterization of phenamil-sensitive Na+ influx in isolated rainbow trout gill epithelial cells.

作者信息

Reid Scott D, Hawkings G S, Galvez F, Goss G G

机构信息

Dept of Biology, Okanagan University College, Kelowna, British Columbia, VIV 1V7, Canada.

出版信息

J Exp Biol. 2003 Feb;206(Pt 3):551-9. doi: 10.1242/jeb.00109.

Abstract

Percoll density-gradient separation, combined with peanut lectin agglutinin (PNA) binding and magnetic bead separation, was used to separate dispersed fish gill cells into sub-populations. Functional characterization of each of the sub-populations was performed to determine which displayed acid-activated phenamil- and bafilomycin-sensitive Na(+) uptake. Analysis of the mechanism(s) of (22)Na(+) influx was performed in control and acid-activated (addition of 10 mmoll(-1) proprionic acid) cells using a variety of Na(+) transport inhibitors (ouabain, phenamil, HOE-694 and bumetanide) and a V-type ATPase inhibitor (bafilomycin). We found that cells migrating to a 1.03-1.05 g ml(-1) Percoll interface [pavement cells (PVCs)] possessed the lowest rates of Na(+) uptake and that influx was unchanged during either bafilomycin (10 nmoll(-1)) treatment or internal acidification with addition of proprionic acid (10 mmoll(-1)). Mitochondria-rich (MR) cells that migrated to the 1.05-1.09 g ml(-1) interface of the Percoll gradient demonstrated acidification-activated bafilomycin and phenamil-sensitive Na(+) influx. Further separation of the MR fraction into PNA(+) and PNA(-) fractions using magnetic separation demonstrated that only the PNA(-) cells (alpha-MR cells) demonstrated phenamil-and bafilomycin-sensitive acid-activated (22)Na(+) uptake. We confirm the coupling of a V-type H(+)-ATPase with phenamil-sensitive Na(+) uptake activity and conclude that high-density alpha-MR cells function in branchial Na(+) uptake in freshwater fish.

摘要

采用Percoll密度梯度分离法,结合花生凝集素(PNA)结合和磁珠分离法,将分散的鱼鳃细胞分离成亚群。对每个亚群进行功能表征,以确定哪些亚群表现出酸激活的苯那明和巴弗洛霉素敏感的Na(+)摄取。使用多种Na(+)转运抑制剂(哇巴因、苯那明、HOE-694和布美他尼)和V型ATP酶抑制剂(巴弗洛霉素),在对照细胞和酸激活细胞(添加10 mmol l(-1)丙酸)中分析(22)Na(+)内流的机制。我们发现,迁移到1.03-1.05 g ml(-1) Percoll界面的细胞[扁平细胞(PVCs)]的Na(+)摄取率最低,并且在巴弗洛霉素(10 nmol l(-1))处理或添加丙酸(10 mmol l(-1))进行内部酸化期间,内流没有变化。迁移到Percoll梯度的1.05-1.09 g ml(-1)界面的富含线粒体(MR)的细胞表现出酸化激活的巴弗洛霉素和苯那明敏感的Na(+)内流。使用磁分离法将MR部分进一步分离为PNA(+)和PNA(-)部分,结果表明只有PNA(-)细胞(α-MR细胞)表现出苯那明和巴弗洛霉素敏感的酸激活(22)Na(+)摄取。我们证实了V型H(+)-ATP酶与苯那明敏感的Na(+)摄取活性的偶联,并得出结论,高密度的α-MR细胞在淡水鱼的鳃Na(+)摄取中起作用。

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