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使用Fluo-3监测心肌细胞内Ca2+的基本方法。

Basic methods for monitoring intracellular Ca2+ in cardiac myocytes using Fluo-3.

作者信息

Bito Virginie, Sipido Karin R, Macquaide Niall

机构信息

Division of Experimental Cardiology, Department of Cardiovascular Sciences, KU Leuven, Belgium.

出版信息

Cold Spring Harb Protoc. 2015 Apr 1;2015(4):392-7. doi: 10.1101/pdb.prot076950.

Abstract

In cardiac myocytes, the physiological increase of intracellular calcium, the [Ca(2+)]i transient, elicited during excitation-contraction coupling typically reaches a peak amplitude of up to 1 µm, from a resting value of ∼100 nm, within 50-100 msec, depending on the species. Various conditions will affect the amplitude and rise time of the [Ca(2+)]i transient and, depending on the nature of the Ca(2+) signals under study, a variety of different probes are available for monitoring changes in intracellular Ca(2+). In this protocol, we focus on Fluo-3, which exists in the cytosol in its salt form K5Fluo-3. This form is practically nonfluorescent in the absence of Ca(2+), but the fluorescence increases dramatically on Ca(2+) binding. Although Fluo-3 is a single excitation-emission dye, it has a number of advantages for investigators, including an ideal dissociation constant (Kd) value and high quantum yield, meaning that it can be used at low concentrations that introduce minimal buffering. Here, we describe the basic setup and methodology for recording the global cytosolic [Ca(2+)]i transient with this probe during simultaneous patch-clamp and whole-cell recording of membrane voltage or of ionic currents under voltage clamp.

摘要

在心肌细胞中,兴奋 - 收缩偶联过程中引发的细胞内钙生理性增加,即[Ca(2 +)]i瞬变,根据物种不同,通常在50 - 100毫秒内从约100纳米的静息值达到高达1微米的峰值幅度。各种条件会影响[Ca(2 +)]i瞬变的幅度和上升时间,并且根据所研究的Ca(2 +)信号的性质,有多种不同的探针可用于监测细胞内Ca(2 +)的变化。在本方案中,我们重点介绍Fluo - 3,它以其盐形式K5Fluo - 3存在于细胞质中。在没有Ca(2 +)的情况下,这种形式实际上是无荧光的,但在Ca(2 +)结合时荧光会急剧增加。虽然Fluo - 3是一种单一激发 - 发射染料,但它对研究人员有许多优点,包括理想的解离常数(Kd)值和高量子产率,这意味着它可以在引入最小缓冲的低浓度下使用。在这里,我们描述了在膜电压的同时膜片钳和全细胞记录或电压钳下的离子电流记录期间,用该探针记录全局细胞质[Ca(2 +)]i瞬变的基本设置和方法。

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