Sine S M, Claudio T, Sigworth F J
Department of Cellular and Molecular Physiology, Yale University School of Medicine, New Haven, Connecticut 06510.
J Gen Physiol. 1990 Aug;96(2):395-437. doi: 10.1085/jgp.96.2.395.
The experiments described examine single channel currents recorded through Torpedo acetylcholine receptor channels stably expressed by a mouse fibroblast cell line. Closed-duration histograms were constructed from currents elicited by 0.5-300 microM acetylcholine (ACh). The concentration dependence of closed durations is well described by a four-state linear scheme with the addition of open-channel block by ACh. Analysis of closed durations measured at low concentrations gives estimates of the rate of opening of doubly liganded receptors, beta, the rate of dissociation of ACh from doubly liganded receptors, k-2, and the rate of channel closing, alpha. The rate of ACh dissociation from singly liganded receptors, k-1, is then deduced from closed-duration histograms obtained at intermediate ACh concentrations. With k-1, k-2 and beta determined, the rates of ACh association, k+1 and k+2, are estimated from fitting closed-duration histograms obtained over a range of high ACh concentrations. A complete set of rate constants is presented for three experimental conditions: (a) Ca2(+)-free extracellular solution containing 1 mM free Mg2+ at 22 degrees C, (b) Ca2(+)-free solution at 12 degrees C, and (c) extracellular Ca2+ and Mg2+, both at 0.5 mM, at 22 degrees C. For all three conditions the dissociation constant for the first agonist binding site is approximately 100-fold lower than that for the second site. The different affinities are due primarily to different dissociation rates. Both the association and dissociation rates depend strongly on temperature. At 22 degrees C ACh associates at diffusion-limited rates, whereas at 12 degrees C association is 30- to 60-fold slower. Also slowed at 12 degrees C are beta (4-fold), k-2 (3-fold), k-1 (25-fold), and alpha (15-fold). In contrast to the activation rate constants, those for ACh-induced block decrease only twofold between 22 and 12 degrees C. Changing from a Ca2(+)-free to a Ca2(+)-containing extracellular solution does not affect k+1 and k+2, but increases beta (twofold) and decreases k-2, k-1, and alpha (all twofold). Spectral analysis of single channel currents supports the parameter estimates obtained from fitting the open- and closed-duration histograms, and improves resolution of brief channel blockages produced by ACh.
所述实验研究了通过小鼠成纤维细胞系稳定表达的电鳐乙酰胆碱受体通道记录的单通道电流。根据0.5 - 300微摩尔乙酰胆碱(ACh)引发的电流构建了关闭持续时间直方图。关闭持续时间的浓度依赖性可以通过一个四态线性模型很好地描述,该模型中加入了ACh对开放通道的阻断作用。对低浓度下测量的关闭持续时间进行分析,可以得出双配体受体的开放速率β、ACh从双配体受体上解离的速率k - 2以及通道关闭的速率α。然后从在中等ACh浓度下获得的关闭持续时间直方图中推导出ACh从单配体受体上解离的速率k - 1。在确定了k - 1、k - 2和β之后,通过拟合在一系列高ACh浓度下获得的关闭持续时间直方图来估计ACh结合的速率k + 1和k + 2。给出了三种实验条件下的完整速率常数集:(a)在22℃下含有1毫摩尔游离镁离子的无钙细胞外溶液;(b)在12℃下的无钙溶液;(c)在22℃下细胞外钙离子和镁离子浓度均为0.5毫摩尔。对于所有这三种条件,第一个激动剂结合位点的解离常数比第二个位点的解离常数低约100倍。不同的亲和力主要是由于不同的解离速率。结合和解离速率都强烈依赖于温度。在22℃时,ACh以扩散限制速率结合,而在12℃时结合速度慢30至60倍。在12℃时β(4倍)、k - 2(3倍)、k - 1(25倍)和α(15倍)也会减慢。与激活速率常数相反,ACh诱导的阻断的速率常数在22℃和12℃之间仅降低两倍。从无钙细胞外溶液转变为含钙细胞外溶液不会影响k + 1和k + 而增加β(两倍)并降低k - 2、k - 1和α(均为两倍)。单通道电流的频谱分析支持了通过拟合开放和关闭持续时间直方图获得的参数估计,并提高了由ACh产生的短暂通道阻断的分辨率。
