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氯四环素作为胰岛细胞中的一种荧光钙探针。

Chlorotetracycline as a fluorescent Ca2+ probe in pancreatic islet cells.

作者信息

Täljedal I B

出版信息

J Cell Biol. 1978 Mar;76(3):652-74. doi: 10.1083/jcb.76.3.652.

Abstract

Pancreatic islets, or suspensions of islet cells, from noninbred ob/ob-mice were incubated with chlorotetracycline and analyzed for Ca2+-dependent fluorescence in a microscope. Unless logarithmically transformed, signals from islets were asymmetrically distributed with unstable variance. Signals from cells pelleted in glass capillaries were more homogeneous and depended linearly on the thickness of the sample. The effect of sample thickness and a significant enhancement of fluorescence by alloxan suggest that beta-cells were involved in producing the signal from whole islets. The signal from dispersed cells was probably diagnostic of Ca2+ in beta-cell plasma membranes because it was suppressed by La3+ and had a spectrum indicative of an apolar micromilieu; fluorescent staining of cell surfaces was directly seen at high magnification. Fluorescence from cells was enhanced by 0.5-10 mM Ca2+ in a dose-dependent manner, whereas less than 0.5 mM Ca2+ saturated the probe alone in methanol. The signal from islets or dispersed cells was suppressed by 5 mM theophylline; that from cells was also suppressed by 0.5 mM 3-isobutyl-1-methylxanthine, 1.2 or 15 mM Mg2+, 3-20 mM D-glucose, and, to a lesser extent, 20 mM 3-O-methyl-D-glucose. D-glucose was more inhibitory in the absence than in the presence of Mg2+, as if Mg2+ and D-glucose influenced the same Ca2+ pool. L-glucose, D-mannopheptulose, or diazoxide had no noticeable effect and 20 mM bicarbonate was stimulatory. The results suggest that microscopy of chlorotetracycline-stained cells can aid in characterizing calcium pools of importance for secretion. Initiation of insulin release may be associated with an increas

摘要

将非近交系ob/ob小鼠的胰岛或胰岛细胞悬液与氯四环素一起孵育,并在显微镜下分析其钙依赖性荧光。除非进行对数转换,否则来自胰岛的信号呈不对称分布且方差不稳定。玻璃毛细管中沉淀的细胞发出的信号更均匀,并且与样品厚度呈线性相关。样品厚度的影响以及四氧嘧啶对荧光的显著增强表明β细胞参与了整个胰岛信号的产生。分散细胞发出的信号可能是β细胞质膜中钙的诊断指标,因为它被La3+抑制且具有表明非极性微环境的光谱;在高倍放大下可直接看到细胞表面的荧光染色。细胞发出的荧光在0.5 - 10 mM Ca2+作用下呈剂量依赖性增强,而在甲醇中单独使用时,低于0.5 mM Ca2+就能使探针饱和。来自胰岛或分散细胞的信号被5 mM茶碱抑制;来自细胞的信号也被0.5 mM 3 - 异丁基 - 1 - 甲基黄嘌呤、1.2或15 mM Mg2+、3 - 20 mM D - 葡萄糖以及在较小程度上被20 mM 3 - O - 甲基 - D - 葡萄糖抑制。在没有Mg2+存在时,D - 葡萄糖的抑制作用更强,就好像Mg2+和D - 葡萄糖影响同一个钙池。L - 葡萄糖、D - 甘露庚酮糖或二氮嗪没有明显影响,而20 mM碳酸氢盐具有刺激作用。结果表明,对氯四环素染色细胞进行显微镜观察有助于表征对分泌重要的钙池。胰岛素释放的起始可能与……增加有关

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