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Amiloride: a molecular probe of sodium transport in tissues and cells.氨氯地平:组织和细胞中钠转运的分子探针。
Am J Physiol. 1982 Mar;242(3):C131-45. doi: 10.1152/ajpcell.1982.242.3.C131.
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Biosynthesis and intracellular transport of acetylcholine receptors.
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Apical sodium uptake in toad kidney epithelial cell line A6.蟾蜍肾上皮细胞系A6中的顶端钠摄取
Am J Physiol. 1983 Sep;245(3):C167-71. doi: 10.1152/ajpcell.1983.245.3.C167.
4
Methylation increases sodium transport into A6 apical membrane vesicles: possible mode of aldosterone action.甲基化增加钠向A6顶端膜囊泡的转运:醛固酮作用的可能模式。
Science. 1984 Aug 17;225(4663):745-6. doi: 10.1126/science.6463652.
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Effects of thyromimetic drugs on aldosterone-dependent sodium transport in the toad bladder.拟甲状腺药物对蟾蜍膀胱中醛固酮依赖性钠转运的影响。
J Membr Biol. 1984;77(1):15-23. doi: 10.1007/BF01871096.
6
Amiloride-sensitive trypsinization of apical sodium channels. Analysis of hormonal regulation of sodium transport in toad bladder.顶端钠通道的氨氯吡咪敏感胰蛋白酶消化法。蟾蜍膀胱钠转运激素调节的分析。
J Gen Physiol. 1983 Jun;81(6):785-803. doi: 10.1085/jgp.81.6.785.
7
Effects of butyrate on histone deacetylation and aldosterone-dependent Na+ transport in the toad bladder.丁酸盐对蟾蜍膀胱中组蛋白去乙酰化及醛固酮依赖性钠转运的影响。
J Biol Chem. 1983 Mar 10;258(5):3388-95.
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Endocytosis and degradation mediated by the asialoglycoprotein receptor in isolated rat hepatocytes.
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Transport properties of toad kidney epithelia in culture.培养的蟾蜍肾上皮细胞的转运特性。
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10
Low temperature selectively inhibits fusion between pinocytic vesicles and lysosomes during heterophagy of 125I-asialofetuin by the perfused rat liver.低温在灌注大鼠肝脏对125I-去唾液酸胎球蛋白进行异体吞噬期间,选择性抑制胞饮小泡与溶酶体之间的融合。
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非洲爪蟾卵母细胞中上皮钠通道的表达

Expression of epithelial Na channels in Xenopus oocytes.

作者信息

Palmer L G, Corthesy-Theulaz I, Gaeggeler H P, Kraehenbuhl J P, Rossier B

机构信息

Institute of Pharmacology, University of Lausanne, Switzerland.

出版信息

J Gen Physiol. 1990 Jul;96(1):23-46. doi: 10.1085/jgp.96.1.23.

DOI:10.1085/jgp.96.1.23
PMID:2170563
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2228986/
Abstract

Epithelial Na channel activity was expressed in oocytes from Xenopus laevis after injection of mRNA from A6 cells, derived from Xenopus kidney. Poly A(+) RNA was extracted from confluent cell monolayers grown on either plastic or permeable supports. 1-50 ng RNA was injected into stage 5-6 oocytes. Na channel activity was assayed as amiloride-sensitive current (INa) under voltage-clamp conditions 1-3 d after injection. INa was not detectable in noninjected or water-injected oocytes. This amiloride-sensitive pathway induced by the mRNA had a number of characteristics in common with that in epithelial cells, including (a) high selectivity for Na over K, (b) high sensitivity to amiloride with an apparent K1 of approximately 100 nM, (c) saturation with respect to external Na with an apparent Km of approximately 10 mM, and (d) a time-dependent activation of current with hyperpolarization of the oocyte membrane. Expression of channel activity was temperature dependent, being slow at 19 degrees C but much more rapid at 25 degrees C. Fractionation of mRNA on a sucrose density gradient revealed that the species of RNA inducing channel activity had a sedimentation coefficient of approximately 17 S. Treatment of filter-grown cells with 300 nM aldosterone for 24 h increased Na transport in the A6 cells by up to fivefold but did not increase the ability of mRNA isolated from those cells to induce channel activity in oocytes. The apparent abundance of mRNA coding for channel activity was 10-fold less in cells grown on plastic than in those grown on filters, but was increased two- to threefold by aldosterone.

摘要

在注射源自非洲爪蟾肾脏的A6细胞的mRNA后,非洲爪蟾卵母细胞中表达了上皮钠通道活性。从生长在塑料或可渗透支持物上的汇合细胞单层中提取多聚腺苷酸(Poly A(+))RNA。将1 - 50 ng RNA注射到5 - 6期卵母细胞中。在注射后1 - 3天的电压钳制条件下,将钠通道活性测定为氨氯地平敏感电流(INa)。在未注射或注射水的卵母细胞中未检测到INa。由mRNA诱导的这种氨氯地平敏感途径具有许多与上皮细胞中相同的特征,包括:(a)对Na的选择性高于K;(b)对氨氯地平高度敏感,表观解离常数(K1)约为100 nM;(c)对外源性Na呈饱和状态,表观米氏常数(Km)约为10 mM;(d)随着卵母细胞膜超极化,电流呈时间依赖性激活。通道活性的表达依赖于温度,在19℃时缓慢,但在25℃时快得多。在蔗糖密度梯度上对mRNA进行分级分离显示,诱导通道活性的RNA种类沉降系数约为17 S。用300 nM醛固酮处理滤膜生长的细胞24小时,可使A6细胞中的Na转运增加多达五倍,但并未增加从这些细胞中分离的mRNA在卵母细胞中诱导通道活性的能力。编码通道活性的mRNA在塑料上生长的细胞中的表观丰度比在滤膜上生长的细胞中低10倍,但醛固酮可使其增加2 - 3倍。