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在装载高浓度乙二醇双四乙酸(EGTA)的骨骼肌纤维中的荧光比率型钙离子指示剂Fura-2钙信号

Fura-2 calcium signals in skeletal muscle fibres loaded with high concentrations of EGTA.

作者信息

Struk A, Szücs G, Kemmer H, Melzer W

机构信息

Department of Applied Physiology, University of Ulm, Germany.

出版信息

Cell Calcium. 1998 Jan;23(1):23-32. doi: 10.1016/s0143-4160(98)90071-9.

Abstract

Fura-2 is one of the most frequently used fluorescent Ca indicator dyes; yet it has limitations in tracking large intracellular Ca transients due to its high affinity for Ca. Since high affinity is of advantage when small Ca changes are to be detected, we tried the application of Fura-2 in skeletal muscle fibres which had been loaded with 15 mM internal EGTA to eliminate contractile artifacts. Under these conditions, the free Ca transients are considerably reduced in amplitude and strong saturation of Fura-2 is avoided. Cut segments of isolated muscle fibres were voltage-clamped in a double vaseline gap set-up. In the presence of high internal EGTA, free Ca (as measured with the rapid metallochromic indicator antipyrylazo III) drops rapidly from one value to a lower quasi steady-state value at the end of a depolarizing voltage pulse. This property allowed inspection of the dissociation kinetics of Ca from Fura-2 in the myoplasmic environment. The dissociation rate constant koff in the fibre was determined from the time constant of the exponential decay of the Fura-2 signal as a function of the final level of free Ca. We obtained a value of 26 s-1 at the experimental temperature of 12 degrees C. Knowledge of koff in the cell is essential for reconstructing the time course of free Ca from indicator bound Ca and for estimating the time course of the rate of release from the sarcoplasmic reticulum. The described combination of high EGTA buffering with Fura-2 fluorescence recording may be particularly useful for the determination of Ca release in small muscle cells.

摘要

呋喃-2是最常用的荧光钙指示剂染料之一;然而,由于其对钙的高亲和力,它在追踪大的细胞内钙瞬变方面存在局限性。由于在检测小的钙变化时高亲和力具有优势,我们尝试在已加载15 mM内部乙二醇双四乙酸(EGTA)以消除收缩伪迹的骨骼肌纤维中应用呋喃-2。在这些条件下,游离钙瞬变的幅度显著降低,并且避免了呋喃-2的强烈饱和。分离的肌纤维切段在双凡士林间隙装置中进行电压钳制。在高内部EGTA存在的情况下,游离钙(用快速金属显色指示剂安替比拉宗III测量)在去极化电压脉冲结束时从一个值迅速下降到一个较低的准稳态值。这一特性使得能够在肌浆环境中检测钙从呋喃-2的解离动力学。纤维中的解离速率常数koff是根据呋喃-2信号指数衰减的时间常数作为游离钙最终水平的函数来确定的。在12摄氏度的实验温度下,我们得到的值为26 s-1。了解细胞中的koff对于从指示剂结合的钙重建游离钙的时间进程以及估计从肌浆网释放速率的时间进程至关重要。所描述的高EGTA缓冲与呋喃-2荧光记录的结合对于确定小肌肉细胞中的钙释放可能特别有用。

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