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通过流入式显微镜对人T细胞免疫突触进行多参数表征

Multiparametric Characterization of Human T-Cell Immune Synapses by InFlow Microscopy.

作者信息

Wabnitz Guido H, Samstag Yvonne

机构信息

Institute of Immunology/Section Molecular Immunology, University of Heidelberg, Im Neuenheimer Feld 305, D-69120, Heidelberg, Germany.

出版信息

Methods Mol Biol. 2016;1389:155-66. doi: 10.1007/978-1-4939-3302-0_10.

Abstract

Immune cells need to communicate with each other via direct cell contact formation. The contact zone has similar functions as a neuronal synapse and is therefore named immune synapse. Supramolecular activation clusters consisting of a variety of surface receptors and cytoplasmic proteins are formed within the immune synapse, which are pivotal for T-cell activation. Thus, a malfunction of immune synapse formation has detrimental effects on the healthiness of the individual.Classical confocal microscopy to analyze the supramolecular cluster formation and maturation of the immune synapse between primary human T-cells and antigen-presenting cells is time consuming and the number of cells that can be analyzed is limited. Therefore, we have established an InFlow microscopy approach for the analysis of immune synapses. InFlow microscopy is a hybrid method combining fluorescence microscopy and flow cytometry. Our InFlow microscopy method allows quantifying protein distribution in immune synapses of several hundred or even thousand cell couples in one sample. Importantly, comparisons of different samples with a strong statistical power are possible with InFlow microcopy.

摘要

免疫细胞需要通过直接形成细胞接触来相互通信。接触区具有与神经元突触相似的功能,因此被称为免疫突触。由多种表面受体和细胞质蛋白组成的超分子激活簇在免疫突触内形成,这对T细胞激活至关重要。因此,免疫突触形成功能异常会对个体健康产生有害影响。用传统共聚焦显微镜分析原代人T细胞与抗原呈递细胞之间免疫突触的超分子簇形成和成熟过程既耗时,且可分析的细胞数量有限。因此,我们建立了一种用于分析免疫突触的流入式显微镜方法。流入式显微镜是一种将荧光显微镜和流式细胞术相结合的混合方法。我们的流入式显微镜方法能够对一个样本中数百甚至数千对细胞的免疫突触中的蛋白质分布进行定量。重要的是,使用流入式显微镜可以对不同样本进行具有强大统计效力的比较。

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