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首页> 外文期刊>The Journal of Physiology >Cytosolic calcium concentration in resting and stimulated endothelium of excised intact rat aorta.
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Cytosolic calcium concentration in resting and stimulated endothelium of excised intact rat aorta.

机译:切除的完整大鼠主动脉的静息和刺激内皮细胞中的钙离子浓度。

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1. Optical fibres were used to excite and record fluorescence from the lumenal face of rat aorta or tail artery loaded with fura-2. 2. Acetylcholine (ACh) evoked an endothelium-dependent rise in the fura-2 340/380 nm excitation ratio in both vessels. High [K+] or phenylephrine evoked an endothelium-independent rise in ratio in tail artery but failed to increase the ratio in aorta. These observations indicate that fura-2 fluorescence and therefore cytosolic calcium concentration ([Ca2+]i) may be selectively recorded from the endothelium of intact rat aorta. 3. In aortic endothelium, resting [Ca2+]i was 95 +/- 8 nM (n = 44). ACh evoked a monophasic rise in [Ca2+]i which was temporally coincident with a membrane hyperpolarization. 4. ATP in most (22/35) preparations evoked a rise in [Ca2+]i which declined towards resting and was followed by a secondary rise. The biphasic [Ca2+]i responses were accompanied by biphasic electrical responses of initial hyperpolarization followed by depolarization above the resting potential and subsequent restoration towards rest. In the presence of high [K+] or the K+ ionophore valinomycin, ATP did not evoke changes in membrane potential and only monophasic rises in [Ca2+]i were observed. In some (7/35) preparations, ATP evoked oscillations in [Ca2+]i, with membrane potential oscillating in antiphase. 5. These data suggest interplay between [Ca2+]i and membrane potential in the generation of agonist-evoked responses in native endothelium in situ. The observed oscillations in [Ca2+]i imply spatio-temporal synchronization of Ca2+ signalling in large groups of endothelial cells in intact rat aorta.
机译:1.用光纤激发并记录载有fura-2的大鼠主动脉或尾动脉腔表面的荧光。 2.乙酰胆碱(ACh)在两个血管中引起fura-2 340/380 nm激发比率的内皮依赖性升高。高[K +]或去氧肾上腺素引起了尾动脉中内皮依赖性比值的升高,但未能增加主动脉中的比值。这些观察结果表明,可以从完整大鼠主动脉的内皮中选择性地记录呋喃2荧光,并因此记录胞浆钙浓度([Ca2 +] i)。 3.在主动脉内皮中,静止的[Ca2 +] i为95 +/- 8 nM(n = 44)。 ACh引起[Ca2 +] i单相上升,这在时间上与膜超极化相吻合。 4.多数(22/35)制剂中的ATP引起[Ca2 +] i升高,然后趋于静止,随后出现第二次升高。双相[Ca2 +] i响应伴随着双相电响应,即初始超极化,然后在静息电位以上进行去极化,随后恢复为静息。在高[K +]或K +离子载体缬氨霉素存在的情况下,ATP不会引起膜电位的变化,并且仅观察到[Ca2 +] i的单相升高。在某些(7/35)制剂中,ATP引起[Ca2 +] i的振荡,而膜电势呈反相振荡。 5.这些数据表明在天然内皮中激动剂引起的反应中[Ca2 +] i和膜电位之间存在相互作用。观察到的[Ca2 +] i振荡表明完整大鼠主动脉中大量内皮细胞中Ca2 +信号的时空同步。

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