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致密斑细胞顶端钾离子通道的基本特性及潜在调节因子

Basic properties and potential regulators of the apical K+ channel in macula densa cells.

作者信息

Hurst A M, Lapointe J Y, Laamarti A, Bell P D

机构信息

Groupe de Recherche en Transport Membranaire, Université de Montréal, Québec.

出版信息

J Gen Physiol. 1994 Jun;103(6):1055-70. doi: 10.1085/jgp.103.6.1055.

Abstract

These studies examine the properties of an apical potassium (K+) channel in macula densa cells, a specialized group of cells involved in tubuloglomerular feedback signal transmission. To this end, individual glomeruli with thick ascending limbs (TAL) and macula densa cells were dissected from rabbit kidney and the TAL covering macula densa cells was removed. Using patch clamp techniques, we found a high density (up to 54 channels per patch) of K+ channels in the apical membrane of macula densa cells. An inward conductance of 41.1 +/- 4.8 pS was obtained in cell-attached patches (patch pipette, 140 mM K+). In inside-out patches (patch pipette, 140 mM; bath, 5 mM K+), inward currents of 1.1 +/- 0.1 pA (n = 11) were observed at 0 mV and single channel current reversed at a pipette potential of -84 mV giving a permeability ratio (PK/PNa) of over 100. In cell-attached patches, mean channel open probability (N,Po, where N is number of channels in the patch and Po is single channel open probability) was unaffected by bumetanide, but was reduced from 11.3 +/- 2.7 to 1.6 +/- 1.3 (n = 5, p < 0.02) by removal of bath sodium (Na+). Simultaneous removal of bath Na+ and calcium (Ca2+) prevented the Na(+)-induced decrease in N.Po indicating that the effect of Na+ removal on N.Po was probably mediated by stimulation of Ca2+ entry. This interpretation was supported by studies where ionomycin, which directly increases intracellular Ca2+, produced a fall in N.Po from 17.8 +/- 4.0 to 5.9 +/- 4.1 (n = 7, p < 0.02). In inside-out patches, the apical K+ channel was not sensitive to ATP but was directly blocked by 2 mM Ca2+ and by lowering bath pH from 7.4 to 6.8. These studies constitute the first single channel observations on macula densa cells and establish some of the characteristics and regulators of this apical K+ channel. This channel is likely to be involved in macula densa transepithelial Cl- transport and perhaps in the tubuloglomerular feedback signaling process.

摘要

这些研究检测了致密斑细胞顶膜钾(K+)通道的特性,致密斑细胞是参与球管反馈信号传导的一组特殊细胞。为此,从兔肾中分离出带有厚壁升支(TAL)和致密斑细胞的单个肾小球,并去除覆盖致密斑细胞的TAL。使用膜片钳技术,我们发现在致密斑细胞顶膜中有高密度的K+通道(每个膜片多达54个通道)。在细胞贴附式膜片中(膜片吸管内为140 mM K+),内向电导为41.1±4.8 pS。在外翻式膜片中(膜片吸管内为140 mM;浴槽内为5 mM K+),在0 mV时观察到内向电流为1.1±0.1 pA(n = 11),单通道电流在吸管电位为 -84 mV时反转,通透率比(PK/PNa)超过100。在细胞贴附式膜片中,平均通道开放概率(N,Po,其中N是膜片中的通道数量,Po是单通道开放概率)不受布美他尼影响,但通过去除浴槽中的钠(Na+),该概率从11.3±2.7降至1.6±1.3(n = 5,p < 0.02)。同时去除浴槽中的Na+和钙(Ca2+)可防止Na+诱导的N.Po降低,这表明去除Na+对N.Po的影响可能是由刺激Ca2+内流介导的。这一解释得到了相关研究的支持,即离子霉素可直接增加细胞内Ca2+,使N.Po从17.8±4.0降至5.9±4.1(n = 7,p < 0.02)。在外翻式膜片中,顶膜K+通道对ATP不敏感,但可被2 mM Ca2+以及将浴槽pH从7.4降至6.8直接阻断。这些研究是对致密斑细胞进行的首次单通道观察,并确定了该顶膜K+通道的一些特性和调节因子。该通道可能参与致密斑跨上皮Cl-转运,或许还参与球管反馈信号传导过程。

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