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A study of intracellular calcium oscillations in sheep cardiac Purkinje fibres measured at the single cell level.

机译:在单细胞水平上对绵羊心脏浦肯野纤维中细胞内钙振荡的研究。

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摘要

Previous work has shown that an elevation of intracellular calcium concentration [( Ca2+]i) produces spontaneous oscillations of [Ca2+]i. However the fact that the oscillations are unsynchronized between different cells has made it difficult to study them. We have therefore injected only one cell in a Purkinje fibre with aequorin in order to avoid these problems. The addition of strophanthidin (10 microM) produced an increase of mean aequorin light over the course of several minutes. During this period spontaneous oscillations of light developed and, with time, their frequency and magnitude increased. The oscillations could first be seen at levels of [Ca2+]i of less than 1 microM. The amplitude of the oscillations of [Ca2+]i could be up to 10 microM and was modulated at a slow rate (about 0.3-0.5 Hz). This suggests that, even within one cell, different regions may oscillate at different frequencies. Elevating [Ca+]o, removing extracellular Na+, or depolarization increased the magnitude of the aequorin light oscillations. Converting the records to [Ca2+]i showed that this increase in the magnitude of the aequorin oscillations was accompanied by a real increase of mean [Ca2+]i and of the magnitude of the oscillations [Ca2+]i. The frequency of the oscillations increased up to a point but saturated at a maximum value of 3-4 Hz. Since previous experiments have used the mean aequorin light to estimate mean [Ca2+]i, we have calculated the error produced in this calculation by the presence of [Ca2+]i oscillations. We estimate that the error is greatest at low levels of Ca2+ loading when the frequency of the oscillations is low. However, at higher Ca2+ loads, when the frequency is above 2 Hz, the error is probably less than 10%. If oscillations were produced by removal of external Na+ after the application of strophanthidin, then either ryanodine or caffeine abolished the oscillations. Furthermore, in both cases, the resulting steady level of [Ca2+]i was similar to the mean level before the addition of the drugs. In another series of experiments we examined the effects of these drugs on oscillations produced by the application of strophanthidin. Caffeine produced a transient increase in both the frequency of the oscillations and mean [Ca2+]i before abolishing the oscillations and decreasing [Ca2+]i to below the level in the absence of caffeine. In contrast ryanodine gradually decreased both the mean [Ca2+]i and the frequency until the oscillations were abolished. During this period of slowing of the oscillations their magnitude was often increased.
机译:先前的工作表明,细胞内钙浓度[(Ca2 +] i)升高会产生[Ca2 +] i的自发振荡。然而,振荡在不同单元之间是不同步的,这使得研究它们变得困难。因此,为了避免这些问题,我们仅在浦肯野纤维中注入了水母发光蛋白一个细胞。在数分钟的过程中,加入鸟嘌呤(10 microM)会使平均水母发光蛋白光增加。在此期间,光自发产生振荡,并且随着时间的流逝,它们的频率和强度增加。首先可以在[Ca2 +] i小于1 microM的水平上看到振荡。 [Ca2 +] i的振荡幅度可能高达10 microM,并以较慢的速率(约0.3-0.5 Hz)进行调制。这表明,即使在一个小区内,不同的区域也可能以不同的频率振荡。升高[Ca +] o,去除细胞外Na +或去极化会增加水母发光蛋白光振荡的幅度。将记录转换为[Ca2 +] i表明,水母发光蛋白振荡幅度的这种增加伴随着平均[Ca2 +] i和振荡幅度[Ca2 +] i的真实增加。振荡频率增加到一个点,但以3-4 Hz的最大值饱和。由于先前的实验已使用均值水母发光来估计均值[Ca2 +] i,因此我们计算了由于[Ca2 +] i振荡而在此计算中产生的误差。我们估计,当振荡频率较低时,在Ca2 +含量较低的情况下,误差最大。但是,在较高的Ca2 +负载下,当频率高于2 Hz时,误差可能小于10%。如果在施用鸟嘌呤后,通过去除外部Na +产生振荡,则无论是雷诺丁还是咖啡因都可以消除振荡。此外,在两种情况下,所得的[Ca2 +] i稳定水平均与添加药物前的平均水平相似。在另一系列的实验中,我们检查了这些药物对应用鸟草磷脂所产生的振荡的影响。咖啡因使振荡频率和平均[Ca2 +] i瞬时增加,然后消除振荡,并使[Ca2 +] i降低到不存在咖啡因的水平以下。相反,ryanodine逐渐降低平均[Ca2 +] i和频率,直到消除振荡为止。在振荡减慢的这段时间内,其幅度通常会增加。

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