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细胞膜拉伸调节牛眼小梁网细胞中的高电导钙激活钾通道。

Cell membrane stretch modulates the high-conductance Ca2+-activated K+ channel in bovine trabecular meshwork cells.

作者信息

Gasull Xavier, Ferrer Elisa, Llobet Artur, Castellano Antonio, Nicolás Jose M, Palés Jordi, Gual Arcadi

机构信息

Laboratory of Neurophysiology, Department of Physiological Sciences I, Institute of Biomedical Investigations August Pi i Sunyer (IDIBAPS), Faculty of Medicine, University of Barcelona, Barcelona, Spain.

出版信息

Invest Ophthalmol Vis Sci. 2003 Feb;44(2):706-14. doi: 10.1167/iovs.02-0384.

Abstract

PURPOSE

Anterior chamber structures are subjected to changes in intraocular pressure (IOP). Several studies have pointed out that trabecular meshwork (TM) cells are sensitive to mechanical stretch and that cell-signaling mechanisms are activated in response to elevated pressure. Because membrane stretch has been shown to be a modulator of several ionic conductances, this study was conducted to determine its effects on the high-conductance Ca(2+)-activated K(+) (BK(Ca)) channels present in TM cells.

METHODS

Primary cultures of TM cells from bovine eyes were used. Patch-clamp recordings were performed in the cell-attached, inside-out, and whole-cell configurations. To stretch the cell membrane, both suction to the rear end of the patch pipette and hypotonic shock were used. Intracellular calcium concentration (Ca(2+)) was measured in TM cells loaded with fura-2, using an epifluorescence microscope coupled to a charge-coupled device (CCD) camera.

RESULTS

Electrophysiological characterization of BK(Ca) channels was in agreement with previous studies. In cell-attached patches, the open probability of the BK(Ca) channel (i.e., the amount of time the channel is open) increased consistently when 14- to 45-mm Hg suctions were applied at a constant depolarized voltage. At a constant pressure (25 or 45 mm Hg), channel openings increased when depolarizing pulses were applied to the patch. Stretch activation of the BK(Ca) channel was not mediated by increases in Ca(2+), because it was present in inside-out patches maintained at a constant Ca(2+) concentration. Nevertheless, it cannot be ruled out that at low suction levels, a minimum Ca(2+) concentration is necessary for channel activation. Whole-cell currents carried by BK(Ca) channels increased when the isotonic solution in the bath was exchanged with a hypotonic solution and were selectively blocked by iberiotoxin. In our conditions, the hypotonic shock did not modify Ca(2+).

CONCLUSIONS

The data show that in TM cells, open probability of the BK(Ca) channel is enhanced by membrane stretching as well as by membrane depolarization and Ca(2+). Changes in membrane tension induced by cell volume increase also activated whole-cell BK(Ca) currents. Homeostatic mechanisms in TM cells may involve BK(Ca) channel activation in response either to changes in cell volume or changes in IOP.

摘要

目的

前房结构会受到眼内压(IOP)变化的影响。多项研究指出,小梁网(TM)细胞对机械拉伸敏感,且细胞信号传导机制会因压力升高而被激活。由于膜拉伸已被证明是几种离子电导的调节因子,因此进行本研究以确定其对TM细胞中存在的高电导钙激活钾(BK(Ca))通道的影响。

方法

使用牛眼TM细胞的原代培养物。在细胞贴附式、内面向外式和全细胞模式下进行膜片钳记录。为了拉伸细胞膜,采用了对膜片吸管后端的抽吸以及低渗休克两种方法。使用与电荷耦合器件(CCD)相机相连的落射荧光显微镜,测量加载了fura-2的TM细胞内的钙浓度(Ca(2+))。

结果

BK(Ca)通道的电生理特性与先前研究一致。在细胞贴附式膜片中,当在恒定的去极化电压下施加14至45毫米汞柱的抽吸时,BK(Ca)通道的开放概率(即通道开放的时间量)持续增加。在恒定压力(25或45毫米汞柱)下,当向膜片施加去极化脉冲时,通道开放增加。BK(Ca)通道的拉伸激活不是由Ca(2+)的增加介导的,因为它存在于保持在恒定钙浓度的内面向外式膜片中。然而,不能排除在低抽吸水平下,最低钙浓度对于通道激活是必要的。当浴中的等渗溶液被低渗溶液替换时,BK(Ca)通道携带的全细胞电流增加,并被iberiotoxin选择性阻断。在我们的条件下,低渗休克并未改变Ca(2+)

结论

数据表明,在TM细胞中,BK(Ca)通道的开放概率通过膜拉伸以及膜去极化和Ca(2+)而增强。细胞体积增加引起的膜张力变化也激活了全细胞BK(Ca)电流。TM细胞中的稳态机制可能涉及BK(Ca)通道响应细胞体积变化或IOP变化而激活。

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