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机械刺激引起的Z线弯曲:整合素依赖性离子通道调节的输入信号?

Bending of z-lines by mechanical stimuli: an input signal for integrin dependent modulation of ion channels?

作者信息

Dyachenko V, Christ A, Gubanov R, Isenberg G

机构信息

Department of Physiology, Martin-Luther-University Halle, Halle, Germany.

出版信息

Prog Biophys Mol Biol. 2008 Jun-Jul;97(2-3):196-216. doi: 10.1016/j.pbiomolbio.2008.02.007. Epub 2008 Feb 13.

DOI:10.1016/j.pbiomolbio.2008.02.007
PMID:18367237
Abstract

We studied which components of mechanical cell deformation are involved in "stretch modulated ion currents" (SMIC). Murine ventricular myocytes were attached to glass coverslips and deformed in x, y and z with a 16 microm thin glass stylus (S) of calibrated stiffness. Three-dimensional confocal microscopy characterized cell deformation (T-tubular membranes, mitochondria) and bending of S (indicative of the applied force). Axial (x-) displacement of S sheared the upper cell part versus the attached bottom, close to S, it changed sarcomere length and bent z-lines ("z-line displacement"). Vertical (z-press) or transversal (y-shear) displacement of S bulged cytoplasm and mitochondria transversally without detectable z-line displacement. Axial stiffness increased with the extent of stress ("stress stiffening"). Depolymerization of F-actin or block of integrin receptors reduced stiffness. SMIC served as a proxy readout of deformation-induced signaling. Axial deformation activated a non-selective cation conductance (Gns) and deactivated an inwardly rectifying K+ conductance (GK1), z-press or y-shear did not induce SMIC. Depolymerization of F-actin or block of integrin receptors reduced SMIC. SMIC did not depend on changes in sarcomere length but correlated with the extent of z-line bending. We discuss that both shear stress at the attached cell bottom and z-line bending could activate mechanosensors. Since SMIC was absent during deformations without z-line bending we postulate that z-line bending is a necessary component for SMIC signaling.

摘要

我们研究了机械性细胞变形的哪些成分参与了“拉伸调节离子电流”(SMIC)。将小鼠心室肌细胞附着于玻璃盖玻片上,并用校准刚度的16微米细玻璃探针(S)在x、y和z方向上使其变形。三维共聚焦显微镜观察细胞变形(T小管膜、线粒体)以及探针S的弯曲情况(指示所施加的力)。探针S的轴向(x-)位移使靠近探针S的细胞上部相对于附着的底部发生剪切,改变了肌节长度并使z线弯曲(“z线位移”)。探针S的垂直(z向压力)或横向(y向剪切)位移使细胞质和线粒体横向鼓起,未检测到z线位移。轴向刚度随应力程度增加(“应力硬化”)。F-肌动蛋白解聚或整合素受体阻断会降低刚度。SMIC作为变形诱导信号传导的替代读数。轴向变形激活了一种非选择性阳离子电导(Gns)并使内向整流钾电导(GK1)失活,z向压力或y向剪切未诱导出SMIC。F-肌动蛋白解聚或整合素受体阻断会降低SMIC。SMIC不依赖于肌节长度的变化,但与z线弯曲程度相关。我们讨论了附着细胞底部的剪切应力和z线弯曲都可能激活机械传感器。由于在没有z线弯曲的变形过程中不存在SMIC,我们推测z线弯曲是SMIC信号传导的必要成分。

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