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哺乳动物动脉平滑肌中细胞钙和收缩性的调节:钠钙交换的作用。

Regulation of cell calcium and contractility in mammalian arterial smooth muscle: the role of sodium-calcium exchange.

作者信息

Ashida T, Blaustein M P

机构信息

Department of Physiology, University of Maryland School of Medicine, Baltimore 21201.

出版信息

J Physiol. 1987 Nov;392:617-35. doi: 10.1113/jphysiol.1987.sp016800.

Abstract
  1. The contraction and relaxation of rings of rat thoracic aorta and bovine tail artery were examined as a function of changes in the Na+ electrochemical gradient in order to determine the role of Na-Ca exchange in the control of contractility. 2. Inhibition of the Na+ pump in rat aorta by K+-free media or a low concentration (5 x 10(-5) M) of strophanthidin reversibly increased the contractile responses to caffeine and noradrenaline. These effects were dependent upon external Ca2+ and were observed even in the presence of a Ca2+ channel blocker (10 microM-verapamil or 10 microM-diltiazem) and an alpha-receptor blocker (10 microM-phentolamine). 3. Reduction of external Na+ concentration, [Na+]o (replaced by N-methylglucamine, tetramethylammonium or Tris), also caused an external Ca2+-dependent increase in tonic tension and, in rat aorta, an increase in the response to caffeine. These effects were also observed in the presence of verapamil and phentolamine. 4. Caffeine relaxed the bovine tail artery, but increased the sensitivity of the rat aorta to reduced [Na+]o. The latter effect was presumably due to block of Ca2+ sequestration in the sarcoplasmic reticulum, so that entering Ca2+ was more effective in raising the intracellular free Ca2+ level, [Ca2+]i. 5. Relaxation from K+-free or low-Na+ contractions, in Ca2+-free media, depended upon [Na+]o. Reduction of [Na+]o to 1.2 or 7.5 mM slowed the relaxation of rat aorta (5 mM-caffeine present) 3- to 5-fold, and the relaxation of bovine tail artery (without caffeine) 5- to 10-fold. These effects were seen in the presence of verapamil and phentolamine. 6. These observations are all consistent with an Na-Ca exchange transport system that can move Ca2+ either into or out of the arterial smooth muscle cells. Ca2+ entry is enhanced by raising [Na+]i (by Na+ pump inhibition) and/or lowering [Na+]o. Ca2+ extrusion from the contracted muscles is largely dependent upon external Na+. The latter observation implies that, when [Ca2+] exceeds the contraction threshold, Ca2+ efflux is mediated primarily by the Na-Ca exchanger, rather than by the sarcolemmal ATP-driven Ca2+ pump. 7. When bovine tail artery was treated with verapamil and phentolamine, and [Na+]o was reduced from 139.2 to 43.9 mM, substitution of K+ for Na+ induced a larger external Ca2+-dependent contraction than did substitution of Tris for Na+. The amplitudes of these contractions were greatly increased when the Na+ pump was inhibited by 5 x 10(-5) M-strophanthidin, presumably because of the rise in [Na+]i.(ABSTRACT TRUNCATED AT 400 WORDS)
摘要
  1. 为了确定钠钙交换在收缩性控制中的作用,研究了大鼠胸主动脉环和牛尾动脉环的收缩与舒张作为钠电化学梯度变化的函数。2. 无钾培养基或低浓度(5×10⁻⁵ M)毒毛花苷对大鼠主动脉钠泵的抑制作用可逆地增加了对咖啡因和去甲肾上腺素的收缩反应。这些作用依赖于细胞外钙离子,即使在存在钙离子通道阻滞剂(10 μM维拉帕米或10 μM地尔硫䓬)和α受体阻滞剂(10 μM酚妥拉明)的情况下也能观察到。3. 降低细胞外钠浓度[Na⁺]ₒ(用N - 甲基葡糖胺、四甲基铵或Tris替代)也会导致细胞外钙离子依赖性的张力增加,并且在大鼠主动脉中,对咖啡因的反应增强。在存在维拉帕米和酚妥拉明的情况下也能观察到这些作用。4. 咖啡因使牛尾动脉舒张,但增加了大鼠主动脉对降低的[Na⁺]ₒ的敏感性。后一种作用可能是由于肌浆网中钙螯合的阻断,因此进入的钙离子在提高细胞内游离钙水平[Ca²⁺]ᵢ方面更有效。5. 在无钙培养基中,从无钾或低钠收缩状态的舒张依赖于[Na⁺]ₒ。将[Na⁺]ₒ降低到1.2或7.5 mM会使大鼠主动脉(存在5 mM咖啡因)的舒张减慢3至5倍,使牛尾动脉(无咖啡因)的舒张减慢5至10倍。在存在维拉帕米和酚妥拉明的情况下能看到这些作用。6. 这些观察结果都与一种钠钙交换转运系统一致,该系统可以将钙离子移入或移出动脉平滑肌细胞。通过提高[Na⁺]ᵢ(通过抑制钠泵)和/或降低[Na⁺]ₒ来增强钙离子进入。收缩肌肉中的钙离子外流在很大程度上依赖于细胞外钠。后一种观察结果意味着,当[Ca²⁺]超过收缩阈值时,钙离子外流主要由钠钙交换体介导,而不是由肌膜ATP驱动的钙泵介导。7. 当用维拉帕米和酚妥拉明处理牛尾动脉,且[Na⁺]ₒ从139.2 mM降低到43.9 mM时,用钾替代钠比用Tris替代钠诱导出更大的细胞外钙离子依赖性收缩。当钠泵被5×10⁻⁵ M毒毛花苷抑制时,这些收缩的幅度大大增加,可能是由于[Na⁺]ᵢ的升高。(摘要截断于400字)

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