离体人汗腺的电生理研究。

C J Jones, D Hyde, C M Lee, T Kealey
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引用次数: 7

摘要

用剪切法分离人内分泌汗腺,用填充4 M醋酸钾的倾斜微电极测定基底外侧膜上的电位差。静息电位高达-81 mV。在静息电位高的细胞中,外部钾浓度从1.2到100 mM的变化导致膜电位在70 mV范围内变化,这表明基底外侧膜主要是钾渗透的。输入阻抗由恒流注入确定,在4-80 M ω范围内。对乙酰胆碱进行大剂量注射,使其终浓度为10(-6)-10(-7)M时,观察到四种反应:去极化,在部分细胞静息电位的-66 - -80 mV (n = 19),超极化,在一群细胞静息电位的-47 - -70 mV (n = 22),没有变化,在-40年到-81年的一些细胞mV静态电位(n = 22)和micro-electrode变位(n = 8)。在细胞去极化的乙酰胆碱,去极化是短暂的和13例是紧随其后的是一个“反弹”超极化。在三分之一(n = 5)可以进行满意测量的细胞中,输入阻抗在去极化期间下降,在去极化的最后阶段或反弹超极化期间增加。在对乙酰胆碱超极化的细胞中,这种超极化通常伴随着输入阻抗的增加。在22个细胞中,有10个细胞在第一次服用乙酰胆碱后没有表现出变化,它们至少再服用两次激动剂。在两个细胞(静息电位-62 mV, -64 mV)中观察到超极化,而在另外三个细胞(静息电位-66 mV, -70 mV, -81 mV)中观察到去极化。乙酰胆碱的作用,无论是去极化还是超极化,都被阿托品可逆地抑制,而被乌阿班不可逆地降低。在补充的RPMI 1640组织培养基中维持腺体长达30小时的实验结果与在新分离的腺体上进行的实验结果基本相似。
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Electrophysiological studies on isolated human eccrine sweat glands.

Human eccrine sweat glands were isolated by shearing and the potential differences across the basolateral membranes determined using bevelled micro-electrodes filled with 4 M potassium acetate. Stable resting potentials of up to -81 mV were recorded. Alterations in external potassium concentration from 1.2 to 100 mM caused the membrane potential to change over a 70 mV range in cells of high resting potential, indicating that the basolateral membrane is largely potassium permeable. Input impedance was determined by constant current injection and found to be in the range 4-80 M omega. On giving a bolus injection of acetylcholine to produce a final concentration of 10(-6)-10(-7) M, four types of response were observed: depolarization, in a proportion of cells with resting potentials of -66 to -80 mV (n = 19), hyperpolarization, in a group of cells with resting potentials of -47 to -70 mV (n = 22), no change, in some cells of -40 to -81 mV resting potential (n = 22) and micro-electrode dislodgement (n = 8). In cells depolarizing to acetylcholine, the depolarization was short-lived and in thirteen cases was followed by a 'rebound' hyperpolarization. Input impedance decreased during depolarization in one-third (n = 5) of the cells in which satisfactory measurement could be made and increased during the final phase of depolarization or during rebound hyperpolarization. In cells hyperpolarizing to acetylcholine, the hyperpolarization was usually accompanied by an increase in input impedance. In ten of the twenty-two cells which showed no change to a first dose of acetylcholine, the agonist was administered at least two more times. In two cells (resting potentials -62 mV, -64 mV) a hyperpolarization was observed whereas in three others (resting potentials -66 mV, -70 mV, -81 mV) depolarization occurred. The effects of acetylcholine, whether depolarizing or hyperpolarizing, were reversibly inhibited by atropine and irreversibly reduced by ouabain. Experiments performed on glands maintained for up to 30 h in supplemented RPMI 1640 tissue culture medium yielded essentially similar results to those performed on freshly isolated glands.

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The school of Bernard Katz. London, 5 April 1989. Proceedings. Extracellular magnesium regulates acetylcholine-evoked amylase secretion and calcium mobilization in rat pancreatic acinar cells. Structure and function of the carotid body in New Zealand genetically hypertensive rats. Intracellular signalling and regulation of gastric acid secretion. Metabolism and inactivation of gastrin releasing peptide by endopeptidase-24.11 in the dog.
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