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Chemical kinetic measurements of a mammalian acetylcholine receptor by a fast-reaction technique.

机译:通过快速反应技术对哺乳动物乙酰胆碱受体的化学动力学测量。

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摘要

In the presence of acetylcholine, the nicotinic acetylcholine receptor undergoes two rapid conformational changes: one in the 1-ms time region, leading to the formation of a transmembrane channel and signal transmission between cells, and the other in the 100-ms time region, leading to an inactive "desensitized" form with altered ligand-binding properties. To determine the properties of the receptor that are relevant for channel opening and signal transmission, we have developed a cell-flow technique that allows measurements to be made with cells prior to receptor desensitization. Here we illustrate the usefulness of the technique. A wide concentration range of both a ligand that controls the opening of receptor channels (carbamoylcholine) and a receptor inhibitor (procaine) was used to measure the dissociation constant of the receptor site controlling channel opening (2.4 X 10(-4) M), the channel-opening equilibrium constant (5.5), the inhibition constant for procaine (5.8 X 10(-5) M), and the rate coefficients for two desensitization processes of 5 s-1 and 0.2 s-1. The cell-flow technique illustrated here is of interest because, by rapid-reaction techniques, it extends the chemical kinetic approach from investigations of reactions in solutions to investigations of many different receptors that exist in membranes of central nervous system cells and whose properties are not well known.
机译:在存在乙酰胆碱的情况下,烟碱乙酰胆碱受体经历两个快速的构象变化:一个在1毫秒的时间范围内,导致跨膜通道的形成和细胞之间的信号传输,另一个在100毫秒的时间范围内,导致配体结合特性改变的非活性“脱敏”形式。为了确定与通道开放和信号传输相关的受体特性,我们开发了一种细胞流技术,该技术允许在受体脱敏之前对细胞进行测量。在这里,我们说明了该技术的实用性。控制受体通道(氨甲酰胆碱)打开的配体和受体抑制剂(普鲁卡因)的浓度范围很宽,可用来测量控制通道打开的受体位点的解离常数(2.4 X 10(-4)M),通道开放平衡常数(5.5),普鲁卡因的抑制常数(5.8 X 10(-5)M)以及两个5 s-1和0.2 s-1的脱敏过程的速率系数。此处说明的细胞流动技术之所以引起人们的关注,是因为它通过快速反应技术将化学动力学方法从溶液中的反应研究扩展到了对中枢神经系统细胞膜中存在的许多不同受体的研究,而这些受体的性质却不众所周知。

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