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影响静止雪貂心室肌细胞内游离钙浓度的因素

Factors influencing free intracellular calcium concentration in quiescent ferret ventricular muscle.

作者信息

Allen D G, Eisner D A, Orchard C H

出版信息

J Physiol. 1984 May;350:615-30. doi: 10.1113/jphysiol.1984.sp015221.

Abstract

The photoprotein aequorin was injected into cells of ferret papillary muscles to monitor the resting intracellular free Ca concentration [( Ca2+]i). Increasing the external Ca concentration [( Ca2+]o) increased both resting [Ca2+]i and resting tension. The tension and [Ca2+]i both rose to a peak and then declined to a steady-state level which was higher than the control. Qualitatively similar, but larger, effects were observed if [Ca2+]i was first elevated with strophanthidin. The increase of [Ca2+]i was accompanied by the development of spontaneous oscillations of [Ca2+]i. When a steady level of [Ca2+]i had been reached in high [Ca2+]o, [Ca2+]o was reduced back to the control level for a brief period. A subsequent increase of [Ca2+]o produced a rise of [Ca2+]i to the same steady level as that previously found in the high [Ca2+]o but the initial peak and subsequent decline were absent. It is suggested that the decline of [Ca2+]i from the initial peak is mediated by a fall of intracellular Na concentration [( Na+]i) limiting Ca entry on a Na-Ca exchange. Increasing external K concentration [( K+]o) from 5 to 30 mmol/l had no detectable effect on [Ca2+]i under control conditions. However, if [Ca2+]i was first increased either by applying strophanthidin or by increasing [Ca2+]o, increasing [K+]o produced a transient rise of [Ca2+]i and tension. This rise was unaffected by D600. It is suggested that the secondary decline of [Ca2+]i after the initial rise may, again, be produced by a fall of [Na+]i acting on an Na-Ca exchange. Acidification produced by increasing [CO2] had no detectable effect on [Ca2+]i under control conditions. However, if [Ca2+]i was increased by strophanthidin, acidification produced a rise of [Ca2+]i. This rise of [Ca2+]i was partly transient even when the intracellular acidification was presumably maintained (raising CO2 at constant [HCO3-]). Acidification in Na-free solutions had qualitatively similar effects to those in Na-containing solutions. In Na-free solutions (Na replaced by K) the [Ca2+]i could be maintained at a low level for at least several hours. Increases of [Ca2+]o in Na-free solutions led to a decrease of [Ca2+]i, and similarly decreasing [Ca2+]o led to an increase in [Ca2+]i. These anomalous effects of [Ca2+]o on [Ca2+]i could be abolished by Mn ions or D600. It is suggested that changes in [Ca2+]o may have reciprocal effects on Ca permeability and hence on [Ca2+]i. The application of the mitochondrial uncoupler FCCP in Na-free solutions led to an increase of resting tension followed, after a substantial delay, by an increase of [Ca2+]i.(ABSTRACT TRUNCATED AT 400 WORDS)

摘要

将光蛋白水母发光蛋白注入雪貂乳头肌细胞,以监测静息状态下细胞内游离钙浓度[(Ca2+]i)。增加细胞外钙浓度[(Ca2+]o)会使静息[Ca2+]i和静息张力均升高。张力和[Ca2+]i均先升至峰值,然后降至高于对照的稳态水平。如果先用毒毛花苷使[Ca2+]i升高,则会观察到定性相似但幅度更大的效应。[Ca2+]i的升高伴随着[Ca2+]i的自发振荡。当在高[Ca2+]o中达到[Ca2+]i的稳定水平后,将[Ca2+]o短暂降至对照水平。随后[Ca2+]o的增加会使[Ca2+]i升至与先前在高[Ca2+]o中发现的相同稳定水平,但没有初始峰值和随后的下降。提示[Ca2+]i从初始峰值下降是由细胞内钠浓度[(Na+]i)降低介导的,这限制了钠钙交换时的钙内流。在对照条件下,将细胞外钾浓度[(K+]o)从5 mmol/L增加到30 mmol/L对[Ca2+]i没有可检测到的影响。然而,如果先用毒毛花苷或增加[Ca2+]o使[Ca2+]i升高,增加[K+]o会使[Ca2+]i和张力短暂升高。这种升高不受D600的影响。提示初始升高后[Ca2+]i的二次下降可能再次是由作用于钠钙交换的[Na+]i下降引起的。在对照条件下,增加[CO2]导致的酸化对[Ca2+]i没有可检测到的影响。然而,如果用毒毛花苷使[Ca2+]i升高,酸化会使[Ca2+]i升高。即使细胞内酸化可能持续存在(在恒定[HCO3-]下升高CO2),[Ca2+]i的这种升高也部分是短暂的。无钠溶液中的酸化与含钠溶液中的酸化具有定性相似的效应。在无钠溶液(用K取代Na)中,[Ca2+]i可维持在低水平至少数小时。无钠溶液中[Ca2+]o的增加导致[Ca2+]i降低,类似地,降低[Ca2+]o导致[Ca2+]i增加。[Ca2+]o对[Ca2+]i的这些异常效应可被Mn离子或D600消除。提示[Ca2+]o的变化可能对钙通透性进而对[Ca2+]i有相互影响。在无钠溶液中应用线粒体解偶联剂FCCP会导致静息张力增加,在相当长的延迟后,[Ca2+]i增加。(摘要截取自400字)

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