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氯电导抑制剂对兔皮质集合管中氯自我交换的影响。

Effects of inhibitors of Cl conductance on Cl self-exchange in rabbit cortical collecting tubule.

作者信息

Tago K, Warden D H, Schuster V L, Stokes J B

出版信息

Am J Physiol. 1986 Dec;251(6 Pt 2):F1009-17. doi: 10.1152/ajprenal.1986.251.6.F1009.

Abstract

Electroneutral vs. conductive pathways of Cl transport were examined by measuring transepithelial conductance (GT) and the lumen-to-bath 36Cl rate coefficient (KCl). Experimental conditions minimized both Cl-HCO3 exchange [HCO3/CO2-free, N-2-hydroxyethylpiperazine-N'-2-ethane-sulfonic acid (HEPES)-buffered solutions] and the electrical driving force for paracellular Cl diffusion (amiloride in the perfusate, transepithelial voltage near zero). Two agents known to inhibit Cl conductances in other epithelia, anthracene-9-carboxylate (9AC, 1 mM) and diphenylamine carboxylate (DPC, 0.1-0.5 mM) reversibly reduced GT and KCl when added to the bath. Both reduced KCl to values consistent with paracellular diffusion. Bath DPC had no effect on GT in the presence of 4 mM lumen Ba2+, suggesting that the DPC-sensitive conductance is in series with an apical K conductance, i.e., resides on the basolateral membrane. Lumen DPC also reduced GT and KCl, but was less potent than bath DPC. Because the lumen DPC effect on GT was also blocked by lumen Ba2+, lumen DPC probably inhibits a basolateral Cl conductance. K removal and ouabain (0.5 mM) had no effect on KCl, suggesting that Cl tracer movement is not predominantly through the principal cell. We assume that these agents are inhibiting Cl conductive pathways and propose a model in which transcellular Cl movement through the intercalated cell occurs via an apical electroneutral entry step in series with a basolateral conductive pathway.

摘要

通过测量跨上皮电导(GT)和管腔到浴液的36Cl速率系数(KCl),研究了Cl转运的电中性途径与导电途径。实验条件将Cl-HCO3交换(无HCO3/CO2,N-2-羟乙基哌嗪-N'-2-乙烷磺酸(HEPES)缓冲溶液)和细胞旁Cl扩散的电驱动力(灌流液中加入氨氯吡脒,跨上皮电压接近零)均降至最低。已知两种可抑制其他上皮细胞中Cl电导的试剂,蒽-9-羧酸盐(9AC,1 mM)和二苯胺羧酸盐(DPC,0.1 - 0.5 mM),加入浴液后可使GT和KCl可逆性降低。两者均将KCl降低至与细胞旁扩散一致的值。在存在4 mM管腔Ba2+的情况下,浴液中的DPC对GT无影响,这表明DPC敏感的电导与顶端K电导串联,即位于基底外侧膜上。管腔中的DPC也降低了GT和KCl,但效力低于浴液中的DPC。由于管腔DPC对GT的影响也被管腔Ba2+阻断,管腔DPC可能抑制了基底外侧的Cl电导。去除K和哇巴因(0.5 mM)对KCl无影响,表明Cl示踪剂的移动并非主要通过主细胞。我们假设这些试剂正在抑制Cl导电途径,并提出一个模型,其中跨细胞的Cl通过闰细胞的移动是通过与基底外侧导电途径串联的顶端电中性进入步骤发生的。

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