首页> 美国卫生研究院文献>The Journal of Physiology >Stretch-sensitive channels in developing muscle cells from a mouse cell line.
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Stretch-sensitive channels in developing muscle cells from a mouse cell line.

机译:小鼠细胞系中发育的肌肉细胞中的拉伸敏感通道。

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摘要

1. Recordings of single-channel activity were made from cell-attached patches on mouse C2 muscle cells at morphologically identifiable stages of myogenesis in vitro. We have identified Ca2(+)-permeable, cation-selective channels that are gated by applying suction to the patch electrode and by changes in membrane potential and have analysed single-channel properties as well as channel expression during myogenesis. 2. Single-channel activity could be detected when the membrane was held at steady negative potentials. With monovalent cations in the electrode, the single-channel current-voltage (i-V) relations were linear. The channel is permeable to Li+, Na+, K+, Rb+ and Cs+, but is not strongly selective among the monovalent cations as judged by measurements of single-channel conductance and reversal potential. 3. With 110 mM of either CaCl2 or BaCl2 as the only inward change carrier, slope conductances were approximately 13 and 24 pS and currents reversed at approximately +22 and +17 mV, respectively. The relative permeability of Ca2+ to K+ calculated from the constant-field equation was PCa/PK = approximately 2. 4. Channel openings occurred as bursts of brief openings and closings separated by much longer closed periods. Closed-time histograms were best fitted with three exponential components, while histograms of burst duration were best fitted with two exponential components, reflecting the short and long bursts in the single-channel records. 5. Applying suction to the patch electrode while recording at steady negative membrane potentials produced channel openings to discrete current levels. Mean channel open probability depended linearly on the square of the applied pressure and was greater at positive membrane potentials. The permeability of the channel to monovalent and divalent cations was indistinguishable from the spontaneous activity recorded at steady negative potentials. 6. Channel activity recorded from cell-attached patches in the absence of applied pressure depended on membrane potential increasing approximately e-fold per 38 mV with depolarization. Analysis of the kinetics of the response to membrane potential showed that the depolarization reduced the duration of the slowest component of the closed-time distribution. 7. The lanthanide cation gadolinium (Gd) reduced the amplitude of the unitary currents in a concentration-dependent manner. The amplitudes of both inward and outward currents were reduced to the same extent suggesting block is voltage-independent. Gd produced half-maximal inhibition of the unitary current at approximately 6 microM.(ABSTRACT TRUNCATED AT 400 WORDS)
机译:1.记录了小鼠C2肌肉细胞上细胞附着的斑块在体外成肌的形态学可识别阶段的单通道活性。我们已经确定了Ca2(+)-可渗透的阳离子选择性通道,这些通道通过向贴片电极施加吸力和膜电位的变化而被门控,并分析了单通道特性以及在肌发生过程中的通道表达。 2.当膜保持稳定的负电位时,可以检测到单通道活性。电极中存在一价阳离子时,单通道电流-电压(i-V)关系是线性的。通道对Li +,Na +,K +,Rb +和Cs +具有渗透性,但是通过测量单通道电导和反转电位判断,该通道在单价阳离子中不是很强的选择性。 3.用110 mM的CaCl2或BaCl2作为唯一的向内变化的载体,斜率电导分别约为13和24 pS,电流分别以大约+22和+17 mV反向。由恒定场方程计算得出的Ca2 +对K +的相对磁导率为PCa / PK =2。4.通道打开是由于短暂的打开和关闭的脉冲被较长的关闭时间间隔分开而发生的。封闭时间直方图最适合三个指数成分,而突发持续时间的直方图最适合两个指数成分,这反映了单通道记录中的短脉冲和长脉冲。 5.在稳定的负膜电位下记录的同时,向贴片电极施加吸力,使通道开口达到离散电流水平。平均通道打开概率线性依​​赖于所施加压力的平方,并且在正膜电位下更大。通道对一价和二价阳离子的渗透性与在稳定的负电位下记录的自发活性没有区别。 6.在没有施加压力的情况下,从细胞附着的贴片记录的通道活性取决于膜电位随着去极化而每38 mV大约增加e倍。对膜电势响应的动力学分析表明,去极化减少了闭合时间分布中最慢分量的持续时间。 7.镧系阳离子g(Gd)以浓度依赖的方式降低了单位电流的幅度。内向电流和外向电流的幅度均减小到相同程度,表明阻塞与电压无关。 Gd在约6 microM处产生最大的单位电流抑制一半(抽象截断为400字)

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