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使用空间强度分布分析(SpIDA)对G蛋白偶联受体介导的受体酪氨酸激酶激活和反式激活进行定量分析。

Quantification of receptor tyrosine kinase activation and transactivation by G-protein-coupled receptors using spatial intensity distribution analysis (SpIDA).

作者信息

Barbeau Annie, Godin Antoine G, Swift Jody L, De Koninck Yves, Wiseman Paul W, Beaulieu Jean-Martin

机构信息

Department of Psychiatry and Neuroscience, Faculty of Medicine, Laval University, Québec, QC, Canada.

出版信息

Methods Enzymol. 2013;522:109-31. doi: 10.1016/B978-0-12-407865-9.00007-8.

Abstract

This chapter presents a general approach for the application of spatial intensity distribution analysis (SpIDA) to the pharmacodynamic quantification of receptor tyrosine kinase homodimerization in response to direct ligand activation or transactivation by G-protein-coupled receptors. Intensity histograms are generated from single fluorescence microscopy images. These histograms are then fit with Poissonian distributions to obtain density maps and quantal brightness values of the labeled proteins underlying the images. This approach allows resolving monomer/oligomer protein mixtures within subcellular compartments using conventional confocal laser scanning microscopy. The application of quantitative pharmacological analysis to data obtained using SpIDA provides a universal method for comparing studies between cell lines and receptor systems. In contrast to methods based on resonance energy transfer, SpIDA is suitable not only for use in recombinant systems but also for the characterization of mechanisms involving endogenous proteins. Therefore, SpIDA enables these biological processes to be monitored directly in their native cellular environment.

摘要

本章介绍了一种将空间强度分布分析(SpIDA)应用于受体酪氨酸激酶同源二聚化药效学定量分析的通用方法,该分析用于响应直接配体激活或G蛋白偶联受体的反式激活。强度直方图由单荧光显微镜图像生成。然后将这些直方图与泊松分布拟合,以获得图像中标记蛋白质的密度图和量子亮度值。这种方法允许使用传统的共聚焦激光扫描显微镜解析亚细胞区室中的单体/寡聚体蛋白质混合物。将定量药理学分析应用于使用SpIDA获得的数据,提供了一种比较细胞系和受体系统之间研究的通用方法。与基于共振能量转移的方法相比,SpIDA不仅适用于重组系统,还适用于涉及内源性蛋白质的机制表征。因此,SpIDA能够在其天然细胞环境中直接监测这些生物过程。

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