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首页> 外文期刊>Analytical Biochemistry: An International Journal of Analytical and Preparative Methods >Development and validation of a platelet calcium flux assay using a fluorescent imaging plate reader
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Development and validation of a platelet calcium flux assay using a fluorescent imaging plate reader

机译:使用荧光成像板读取器开发和验证血小板钙通量测定

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Calcium signaling in platelets is an important physiological response to various aggregation stimuli. Loading platelets with various fluorescent dyes and measuring the change in calcium concentration using a spectrofluorometer has been the traditional approach to studying calcium signaling. This method suffers from the need for large platelet samples and a decrease in total fluorescence signal with time due to photobleaching. Therefore, it is rarely used to measure the quantitative effect of an agonist or antagonist on calcium signaling. Adaptation of these measurements to a fluorescent imaging plate reader (FLIPR) format allows the sample size to be reduced by 5- to 10-fold, and the microplate format allows a significant increase in throughput. Addition of the agonists to all wells simultaneously serves to normalize the total response. This article describes the first use of a FLIPR to study the calcium flux in human platelets. The IC50 values showed a linear correlation with the K-i for receptor binding in washed platelets. The generality of the methodology was shown by measuring EC50 values for agonists and IC50 values for antagonists of the platelet G protein-coupled receptor P2Y(1) and for the ion channel P2X(1). (c) 2006 Elsevier Inc. All rights reserved.
机译:血小板中的钙信号传导是对各种聚集刺激的重要生理反应。研究钙信号的传统方法是用各种荧光染料加载血小板并使用分光荧光计测量钙浓度的变化。该方法需要大量的血小板样品,并且由于光漂白而使总荧光信号随时间减少。因此,很少用于测量激动剂或拮抗剂对钙信号传导的定量作用。将这些测量值调整为荧光成像板读取器(FLIPR)格式可使样品大小减少5至10倍,而微孔板格式则可显着提高通量。将激动剂同时添加到所有孔中有助于标准化总反应。本文介绍了FLIPR首次用于研究人血小板中钙通量的用途。 IC50值显示出与洗涤血小板中受体结合的K-1线性相关。通过测量激动剂的EC50值和血小板G蛋白偶联受体P2Y(1)和离子通道P2X(1)的拮抗剂的IC50值来显示该方法的通用性。 (c)2006 Elsevier Inc.保留所有权利。

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