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通过共定位分析追踪药物诱导的内化后受体转运变化

Tracking Drug-induced Changes in Receptor Post-internalization Trafficking by Colocalizational Analysis.

作者信息

Ong Edmund, Cahill Catherine

机构信息

Department of Anesthesiology and Perioperative Care, University of California Irvine; Department of Biomedical and Molecular Sciences, Queen's University;

Department of Anesthesiology and Perioperative Care, University of California Irvine; Department of Biomedical and Molecular Sciences, Queen's University; Department of Pharmacology, University of California Irvine.

出版信息

J Vis Exp. 2015 Jul 3(101):e52824. doi: 10.3791/52824.

Abstract

The intracellular trafficking of receptors is a collection of complex and highly controlled processes. Receptor trafficking modulates signaling and overall cell responsiveness to ligands and is, itself, influenced by intra- and extracellular conditions, including ligand-induced signaling. Optimized for use with monolayer-plated cultured cells, but extendable to free-floating tissue slices, this protocol uses immunolabelling and colocalizational analysis to track changes in intracellular receptor trafficking following both chronic/prolonged and acute interventions, including exogenous drug treatment. After drug treatment, cells are double-immunolabelled for the receptor and for markers for the intracellular compartments of interest. Sequential confocal microscopy is then used to capture two-channel photomicrographs of individual cells, which are subjected to computerized colocalizational analysis to yield quantitative colocalization scores. These scores are normalized to permit pooling of independent replicates prior to statistical analysis. Representative photomicrographs may also be processed to generate illustrative figures. Here, we describe a powerful and flexible technique for quantitatively assessing induced receptor trafficking.

摘要

受体的细胞内运输是一系列复杂且高度受控的过程。受体运输调节信号传导以及细胞对配体的整体反应性,并且其本身受细胞内和细胞外条件的影响,包括配体诱导的信号传导。该方案针对单层培养的细胞进行了优化,但也可扩展至游离的组织切片,它利用免疫标记和共定位分析来追踪慢性/长期和急性干预(包括外源性药物处理)后细胞内受体运输的变化。药物处理后,对细胞进行双重免疫标记,分别标记受体和感兴趣的细胞内区室的标志物。然后使用顺序共聚焦显微镜拍摄单个细胞的双通道显微照片,并对其进行计算机化共定位分析以得出定量共定位分数。这些分数经过归一化处理,以便在统计分析之前合并独立重复实验的数据。代表性的显微照片也可进行处理以生成说明性图表。在这里,我们描述了一种用于定量评估诱导的受体运输的强大且灵活的技术。

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