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通过全内反射荧光检测受刺激中性粒细胞中膜近端钙瞬变。

Membrane-proximal calcium transients in stimulated neutrophils detected by total internal reflection fluorescence.

作者信息

Omann G M, Axelrod D

机构信息

Department of Surgery, University of Michigan, Ann Arbor 48105, USA.

出版信息

Biophys J. 1996 Nov;71(5):2885-91. doi: 10.1016/S0006-3495(96)79485-7.

Abstract

A novel fluorescence microscope/laser optical system was developed to measure fast transients of membrane-proximal versus bulk cytoplasmic intracellular calcium levels in cells labeled with a fluorescent calcium indicator. The method is based on the rapid chopping of illumination of the cells between optical configurations for epifluorescence, which excites predominantly the bulk intracellular region, and total internal reflection fluorescence, which excites only the region within approximately 100 nm of the cell-substrate contact. This method was applied to Fluo-3-loaded neutrophils that were activated by the chemoattractant N-formyl-met-leu-phe. Chemoattractant-activated cells showed 1) transient increases in both membrane-proximal and bulk cytosolic Ca2+ that peaked simultaneously; 2) a larger fractional change (20-60%) in membrane-proximal Ca2+ relative to bulk cytosolic Ca2+ that peaked at a time when the main Ca2+ transient was decreasing in both regions and that persisted well after the main transient was over. This method should be applicable to a wide variety of cell types and fluorescent ion indicators in which membrane-proximal ionic transients may be different from those deeper within the cytosol.

摘要

一种新型荧光显微镜/激光光学系统被开发出来,用于测量用荧光钙指示剂标记的细胞中膜近端与胞质内整体钙水平的快速瞬变。该方法基于在用于落射荧光的光学配置(主要激发胞质内整体区域)和全内反射荧光(仅激发细胞与底物接触处约100 nm范围内的区域)之间对细胞照明进行快速切换。此方法应用于被趋化因子N-甲酰基-甲硫氨酰-亮氨酰-苯丙氨酸激活的负载Fluo-3的中性粒细胞。趋化因子激活的细胞表现出:1)膜近端和胞质内整体Ca2+同时出现瞬态增加并达到峰值;2)相对于胞质内整体Ca2+,膜近端Ca2+的分数变化更大(20 - 60%),在两个区域中主要Ca2+瞬变下降时达到峰值,并且在主要瞬变结束后仍持续存在。该方法应适用于多种细胞类型和荧光离子指示剂,其中膜近端离子瞬变可能与胞质溶胶中更深区域的瞬变不同。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/9867/1233774/7ecf4291706c/biophysj00041-0649-a.jpg

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