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人二倍体成纤维细胞的制备及离子转运研究。

Preparation of individual human diploid fibroblasts and study of ion transport.

作者信息

Abraham E H, Breslow J L, Epstein J, Chang-Sing P, Lechene C

出版信息

Am J Physiol. 1985 Jan;248(1 Pt 1):C154-64. doi: 10.1152/ajpcell.1985.248.1.C154.

DOI:10.1152/ajpcell.1985.248.1.C154
PMID:3966540
Abstract

A method for analyzing individual mammalian cells with electron probe microanalysis has been developed using human diploid fibroblasts. Cells were grown on the same support that is used for experimental manipulations and analysis. Steady-state cation and anion concentrations and kinetic processes during experimental perturbations could be measured on populations of less than 1,000 cells. Human diploid fibroblasts in normal tissue culture medium had the following intracellular concentrations (in mM): K, 168; Na, 25.0; Cl, 51.2; P, 84.1; S, 16.5; Ca, 6.04; and Mg, 10.0. The ratios of K to Na were equivalent when measured in the nuclear or cytoplasmic area of the cells. Serum in the incubation medium was found to increase the cellular effective permeability to Na by a factor of 2.5, while leaving the effective permeability to K unchanged. When returned to control medium after 7 h of incubation in K-free medium, the cells recovered normal K/Na in less than 1 h. In some experiments the coupling ratio of the ouabain-inhibitable cellular transport of Na to K was 3:2 and the ratio of Cl to K was 1:2. The sum of intracellular content (Na + K) (an estimate of cellular volume) did not change when the cells were placed in K-free medium and increased by less than 30% after ouabain treatment. After 5-7 h of ouabain treatment or of incubation in K-free medium, long after the intracellular K had been replaced by Na, the cellular chloride content had not changed significantly.

摘要

一种利用人二倍体成纤维细胞通过电子探针微分析来分析单个哺乳动物细胞的方法已被开发出来。细胞在用于实验操作和分析的相同载体上生长。在少于1000个细胞的群体上可以测量实验扰动期间的稳态阳离子和阴离子浓度以及动力学过程。处于正常组织培养基中的人二倍体成纤维细胞具有以下细胞内浓度(以毫摩尔计):钾,168;钠,25.0;氯,51.2;磷,84.1;硫,16.5;钙,6.04;镁,10.0。当在细胞核或细胞质区域测量时,钾与钠的比率是相等的。发现培养介质中的血清会使细胞对钠的有效通透性增加2.5倍,而对钾的有效通透性保持不变。在无钾培养基中孵育7小时后再回到对照培养基时,细胞在不到1小时内恢复正常的钾/钠水平。在一些实验中,哇巴因抑制的细胞钠钾转运偶联比为三比二,氯与钾的比为一比二。当细胞置于无钾培养基中时,细胞内含量(钠 + 钾)的总和(细胞体积的估计值)没有变化,在哇巴因处理后增加不到30%。在哇巴因处理或在无钾培养基中孵育5 - 7小时后,在细胞内的钾被钠取代很久之后,细胞内氯含量没有显著变化。

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