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首页> 外文期刊>American Journal of Physiology >In situ calibration and (H+) sensitivity of the fluorescent Na+ indicator SBFI.
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In situ calibration and (H+) sensitivity of the fluorescent Na+ indicator SBFI.

机译:荧光Na +指示剂SBFI的原位校准和(H +)灵敏度。

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摘要

Despite the popularity of Na+-binding benzofuran isophthalate (SBFI) to measure intracellular free Na+ concentrations ([Na+](i)), the in situ calibration techniques described to date do not favor the straightforward determination of all of the constants required by the standard equation (Grynkiewicz G, Poenie M, and Tsien RY. J Biol Chem 260: 3440-3450, 1985) to convert the ratiometric signal into [Na+]. We describe a simple method in which SBFI ratio values obtained during a "full" in situ calibration are fit by a three-parameter hyperbolic equation; the apparent dissociation constant (K(d)) of SBFI for Na+ can then be resolved by means of a three-parameter hyperbolic decay equation. We also developed and tested a "one-point" technique for calibrating SBFI ratios in which the ratio value obtained in a neuron at the end of an experiment during exposure to gramicidin D and 10 mM Na+ is used as a normalization factor for ratios obtained during the experiment; each normalized ratio is converted to [Na+](i) using a modification of the standard equation and parameters obtained from a full calibration. Finally, we extended the characterization of the pH dependence of SBFI in situ. Although the K(d) of SBFI for Na+ was relatively insensitive to changes in pH in the range 6.8-7.8, acidification resulted in an apparent decrease, and alkalinization in an apparent increase, in [Na+](i) values. The magnitudes of the apparent changes in [Na+](i) varied with absolute [Na+](i), and a method was developed for correcting [Na+](i) values measured with SBFI for changes in intracellular pH.
机译:尽管结合Na +的间苯二甲酰呋喃磺酸钠(SBFI)可以测量细胞内游离Na +浓度([Na +](i)),但迄今为止描述的原位校准技术不利于直接确定标准所要求的所有常数方程(Grynkiewicz G,Poenie M和Tsien RY.J Biol Chem 260:3440-3450,1985)将比例信号转换为[Na +]。我们描述了一种简单的方法,其中在“完全”原位校准期间获得的SBFI比值通过三参数双曲方程拟合;然后可以通过三参数双曲线衰减方程来解析SBFI对Na +的表观解离常数(K(d))。我们还开发并测试了一种“单点”技术,用于校准SBFI比率,其中将实验结束时在暴露于短杆菌肽D和10 mM Na +的过程中神经元中获得的比率值用作归一化比率的标准化因子。本实验;使用标准方程式的修改和从完全校准中获得的参数,将每个归一化的比率转换为[Na +](i)。最后,我们扩展了原位SBFI的pH依赖性的表征。尽管SBFI对于Na +的K(d)对6.8-7.8范围内的pH值变化相对不敏感,但酸化导致[Na +](i)值明显降低,而碱化则明显增加。 [Na +](i)的表观变化的幅度随绝对[Na +](i)的变化而变化,并开发了一种方法来校正SBFI测得的[Na +](i)值以适应细胞内pH的变化。

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