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荧光钙指示剂Fura-2的细胞内校准。

Intracellular calibration of the fluorescent calcium indicator Fura-2.

作者信息

Williams D A, Fay F S

机构信息

Department of Physiology, University of Melbourne, Parkville, Victoria, Australia.

出版信息

Cell Calcium. 1990 Feb-Mar;11(2-3):75-83. doi: 10.1016/0143-4160(90)90061-x.

Abstract

We present the techniques we have used and the problems we have encountered in our laboratories in the in vivo calibration of the fluorescent Ca2(+)-indicator Fura-2. These techniques include the use of potentiometric methods for the precise control and determination of Ca2+ levels in bathing solutions, in association with methods for the equilibration of internal and external solutions with ionophores (Br-A23187, ionomycin, monensin and nigericin). A by-product of these techniques has been the development of a simple procedure that utilizes Fura-2 as a general indicator of ionized Ca2+ concentrations within the physiological range (pCa 7.5 to 5.5), in other experimental solutions. The major advantages of this relatively simple procedure are that it is (i) rapidly performed, (ii) independent of the total EGTA concentration within each experimental solution, (iii) independent of the absolute EGTA purity, and (iv) unaffected by a large number of potentially interfering cations (i.e. Mg2+, H+, K+, Na+) within the test solutions.

摘要

我们介绍了在我们实验室中对荧光Ca2+指示剂Fura-2进行体内校准所使用的技术以及遇到的问题。这些技术包括使用电位测定法精确控制和测定浴液中的Ca2+水平,并结合使用离子载体(溴-A23187、离子霉素、莫能菌素和尼日利亚菌素)使内部和外部溶液达到平衡的方法。这些技术的一个附带成果是开发了一种简单的程序,该程序利用Fura-2作为其他实验溶液中生理范围内(pCa 7.5至5.5)游离Ca2+浓度的通用指示剂。这个相对简单的程序的主要优点是:(i)执行速度快;(ii)与每个实验溶液中的总EGTA浓度无关;(iii)与EGTA的绝对纯度无关;(iv)不受测试溶液中大量潜在干扰阳离子(即Mg2+、H+、K+、Na+)的影响。

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