Banderali U, Roy G
Département de Physique, Université de Montréal, Québec, Canada.
J Membr Biol. 1992 Mar;126(3):219-34. doi: 10.1007/BF00232319.
Single-channel patch-clamp experiments were performed on MDCK cells in order to characterize the ionic channels participating in regulatory volume decrease (RVD). Subconfluent layers of cultured cells were exposed to a hypotonic medium (150 mOsm), and the membrane currents at the single-channel level were measured in cell-attached experiments. The results indicate that MDCK cells respond to a hypotonic swelling by activating several different ionic conductances. In particular, a potassium and a chloride channel appeared in the recordings more frequently than other channels, and this allowed a more detailed study of their properties in the inside-out configuration of the patch-clamp technique. The potassium channel had a linear I/V curve with a unitary conductance of 24 +/- 4 pS in symmetrical K+ concentrations (145 mM). It was highly selective for K+ ions vs. Na+ ions: PNa/PK less than 0.04. The time course of its open probability (P0) showed that the cells responded to the hypotonic shock with a rapid activation of this channel. This state of high activity was maintained during the first minute of hypotonicity. The chloride channel participating in RVD was an outward-rectifying channel: outward slope conductance of 63.3 +/- 4.7 pS and inward slope conductance of 26.1 +/- 4.9 pS. It was permeable to both Cl- and NO3- and its maximal activation after the hypotonic shock was reached after several seconds (between 30 and 100 sec). The activity of this anionic channel did not depend on cytoplasmic calcium concentration. Quinine acted as a rapid blocker of both channels when applied to the cytoplasmic side of the membrane. In both cases, 1 mM quinine reversibly reduced single-channel current amplitudes by 20 to 30%. These results indicate that MDCK cells responded to a hypotonic swelling by an early activation of highly selective potassium conductances and a delayed activation of anionic conductances. These data are in good agreement with the changes of membrane potential measured during RVD.
为了表征参与调节性容积减小(RVD)的离子通道,对MDCK细胞进行了单通道膜片钳实验。将亚汇合的培养细胞层暴露于低渗培养基(150 mOsm)中,并在细胞贴附实验中测量单通道水平的膜电流。结果表明,MDCK细胞通过激活几种不同的离子电导来响应低渗肿胀。特别是,钾通道和氯通道在记录中出现的频率比其他通道更高,这使得能够在膜片钳技术的内面向外配置中更详细地研究它们的特性。在对称的K⁺浓度(145 mM)下,钾通道具有线性的I/V曲线,单通道电导为24±4 pS。它对K⁺离子与Na⁺离子具有高度选择性:PNa/PK小于0.04。其开放概率(P0)的时间进程表明,细胞对低渗休克的反应是该通道迅速激活。在低渗状态的第一分钟内保持这种高活性状态。参与RVD的氯通道是外向整流通道:外向斜率电导为63.3±4.7 pS,内向斜率电导为26.1±4.9 pS。它对Cl⁻和NO₃⁻都有通透性,低渗休克后几秒钟(30至100秒之间)达到最大激活。这种阴离子通道的活性不依赖于细胞质钙浓度。当应用于膜的细胞质侧时,奎宁作为两种通道的快速阻滞剂。在两种情况下,1 mM奎宁可逆地将单通道电流幅度降低20%至30%。这些结果表明,MDCK细胞通过早期激活高度选择性的钾电导和延迟激活阴离子电导来响应低渗肿胀。这些数据与RVD期间测量的膜电位变化非常一致。
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