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成年哺乳动物单个心肌细胞内游离镁离子的调节与收缩

Regulation of intracellular free Mg2+ and contraction in single adult mammalian cardiac myocytes.

作者信息

Silverman H S, Di Lisa F, Hui R C, Miyata H, Sollott S J, Hanford R G, Lakatta E G, Stern M D

机构信息

Laboratory of Cardiovascular Science, National Institute on Aging, National Institutes of Health, Baltimore 21224.

出版信息

Am J Physiol. 1994 Jan;266(1 Pt 1):C222-33. doi: 10.1152/ajpcell.1994.266.1.C222.

Abstract

Studies in isolated cardiac myocytes have increased our understanding of intracellular Ca2+ regulation. Because less is known about Mg2+ regulation, adult rat ventricular myocytes were loaded with the Mg(2+)-sensitive fluorescent probe mag-indo 1, and changes in intracellular Mg2+ concentration ([Mg2+]i) and cell length were examined under a variety of conditions. The fluorescent signal was calibrated intracellularly and found to differ slightly from that for the probe in solution. Roughly 40% of the signal was intramitochondrial; the remainder was localized in the cytosol. Basal [Mg2+]i averaged 1.02 +/- 0.03 mM (n = 53 cells). No change in [Mg2+]i was observed during a single electrically stimulated contraction, and only a minor increase was seen during rapid electrical stimulation, which was expected to raise intracellular Ca2+ concentration ([Ca2+]i) to approximately 1 microM. An acid shift in intracellular pH of approximately 1 pH unit was accompanied by a small change in [Mg2+]i (0.34 +/- 0.03 mM, n = 6, P < 0.05). No change in [Mg2+]i was observed when cells were superfused with 15 mM Mg2+, despite marked changes in contraction. [Mg2+]i more than doubled when cells were depleted of ATP by exposure to hypoxia or metabolic inhibitors. The increase in [Mg2+]i was abrupt and occurred at the time of the failure of contraction, plateauing as rigor contracture developed. Reoxygenation was accompanied by a gradual fall in [Mg2+]i in cells that recovered mechanical function, and in a subset of cells that underwent hypercontracture. Studies in cell suspensions confirmed that rapid cellular energy depletion was accompanied by increases in [Mg2+]i and parallel decreases in ATP. Thus [Mg2+]i was largely insensitive to changes in [Ca2+]i or pHi and extracellular [Mg2+] but was rapidly altered by changes in energy state in a manner that was related to specific changes in cell morphology and contractile function.

摘要

对分离的心肌细胞的研究增进了我们对细胞内钙离子调节的理解。由于对镁离子调节的了解较少,我们将成年大鼠心室肌细胞用镁离子敏感荧光探针mag-indo 1进行负载,并在多种条件下检测细胞内镁离子浓度([Mg2+]i)和细胞长度的变化。荧光信号在细胞内进行校准,发现与溶液中探针的信号略有不同。大约40%的信号位于线粒体内;其余部分位于细胞质中。基础[Mg2+]i平均为1.02±0.03 mM(n = 53个细胞)。在单次电刺激收缩期间未观察到[Mg2+]i的变化,在快速电刺激期间仅观察到轻微增加,快速电刺激预计会使细胞内钙离子浓度([Ca2+]i)升高至约1 microM。细胞内pH值约1个pH单位的酸性变化伴随着[Mg2+]i的小变化(0.34±0.03 mM,n = 6,P < 0.05)。当用15 mM镁离子对细胞进行灌流时,尽管收缩有明显变化,但未观察到[Mg2+]i的变化。当细胞通过暴露于缺氧或代谢抑制剂而耗尽ATP时,[Mg2+]i增加了一倍多。[Mg2+]i的增加是突然的,发生在收缩失败时,并随着强直收缩的发展而达到平台期。复氧伴随着恢复机械功能的细胞以及经历过度收缩的一部分细胞中[Mg2+]i的逐渐下降。对细胞悬液的研究证实,细胞能量的快速耗尽伴随着[Mg2+]i的增加和ATP的平行减少。因此,[Mg2+]i在很大程度上对[Ca2+]i、细胞内pH值或细胞外[Mg2+]的变化不敏感,但会因能量状态的变化而迅速改变,这种改变方式与细胞形态和收缩功能的特定变化有关。

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