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来自用fura-2加载的肥大细胞的钙信号强烈依赖于染料加载的方法。

The Ca signal from fura-2 loaded mast cells depends strongly on the method of dye-loading.

作者信息

Almers W, Neher E

出版信息

FEBS Lett. 1985 Nov 11;192(1):13-8. doi: 10.1016/0014-5793(85)80033-8.

Abstract

The Ca concentration ([Ca2+]i) in single rat peritoneal mast cells was measured by means of the new fluorescent Ca-indicator dye fura-2. Dye-loaded cells were made to degranulate with either antigen or compound 48/80. In cells loaded with extracellularly applied, membrane-permeant fura-2 ester, degranulation was accompanied by a permanent loss of 40-60% of the fluorescence, but comparison of fluorescence at different wavelengths indicated no or only small changes in [Ca2+]i. When cells were loaded by microinjection of the impermeant potassium salt of the dye, degranulation resulted in no permanent loss of fluorescence, but instead was preceded by transient fluorescence changes that indicate a rapid, large and transient increase in [Ca2+]i. We suggest that ester-loaded fura-2 accumulates to a significant degree in the secretory granules and is lost from the cell during exocytosis.

摘要

采用新型荧光钙指示剂染料fura-2测定了单个大鼠腹膜肥大细胞内的钙浓度([Ca2+]i)。用抗原或化合物48/80使负载染料的细胞脱颗粒。在用细胞外应用的、可透过细胞膜的fura-2酯负载的细胞中,脱颗粒伴随着荧光永久性损失40%-60%,但不同波长荧光的比较表明[Ca2+]i没有变化或仅有微小变化。当通过显微注射染料的非渗透性钾盐来负载细胞时,脱颗粒并未导致荧光的永久性损失,而是在脱颗粒之前出现短暂的荧光变化,这表明[Ca2+]i迅速、大幅且短暂地增加。我们认为,负载酯的fura-2在分泌颗粒中大量积累,并在胞吐过程中从细胞中丢失。

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