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本文引用的文献

1
Human profilin 1 is a negative regulator of CTL mediated cell-killing and migration.人原肌球蛋白1是细胞毒性T淋巴细胞介导的细胞杀伤和迁移的负调节因子。
Eur J Immunol. 2017 Sep;47(9):1562-1572. doi: 10.1002/eji.201747124. Epub 2017 Jul 31.
2
Three-Dimensional Cell Cultures in Drug Discovery and Development.三维细胞培养在药物发现和开发中的应用。
SLAS Discov. 2017 Jun;22(5):456-472. doi: 10.1177/1087057117696795.
3
A guide to light-sheet fluorescence microscopy for multiscale imaging.多尺度成像的光片荧光显微镜指南。
Nat Methods. 2017 Mar 31;14(4):360-373. doi: 10.1038/nmeth.4224.
4
Bystander cells enhance NK cytotoxic efficiency by reducing search time.旁观者细胞通过减少搜索时间来提高 NK 细胞的细胞毒性效率。
Sci Rep. 2017 Mar 13;7:44357. doi: 10.1038/srep44357.
5
T cell migration, search strategies and mechanisms.T细胞迁移、搜索策略与机制。
Nat Rev Immunol. 2016 Mar;16(3):193-201. doi: 10.1038/nri.2015.16. Epub 2016 Feb 8.
6
Comparison of 2D- and 3D-culture models as drug-testing platforms in breast cancer.二维和三维培养模型作为乳腺癌药物测试平台的比较
Oncol Rep. 2015 Apr;33(4):1837-43. doi: 10.3892/or.2015.3767. Epub 2015 Jan 29.
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Three-dimensional organotypic culture: experimental models of mammalian biology and disease.三维器官型培养:哺乳动物生物学与疾病的实验模型
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3D cell culture systems: advantages and applications.3D细胞培养系统:优势与应用
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9
Dimensions in cell migration.细胞迁移的维度。
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10
Impact of the 3D microenvironment on phenotype, gene expression, and EGFR inhibition of colorectal cancer cell lines.3D 微环境对结直肠癌细胞系表型、基因表达和 EGFR 抑制的影响。
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用于人类免疫细胞三维可视化的光片显微镜技术

Light-sheet Microscopy for Three-dimensional Visualization of Human Immune Cells.

作者信息

Schoppmeyer Rouven, Zhao Renping, Hoth Markus, Qu Bin

机构信息

Department of Biophysics, Center for Integrative Physiology and Molecular Medicine (CIPMM), School of Medicine, Saarland University.

Department of Biophysics, Center for Integrative Physiology and Molecular Medicine (CIPMM), School of Medicine, Saarland University;

出版信息

J Vis Exp. 2018 Jun 13(136):57651. doi: 10.3791/57651.

DOI:10.3791/57651
PMID:29985362
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC6101706/
Abstract

In vivo, activation, proliferation, and function of immune cells all occur in a three-dimensional (3D) environment, for instance in lymph nodes or tissues. Up to date, most in vitro systems rely on two-dimensional (2D) surfaces, such as cell-culture plates or coverslips. To optimally mimic physiological conditions in vitro, we utilize a simple 3D collagen matrix. Collagen is one of the major components of extracellular matrix (ECM) and has been widely used to constitute 3D matrices. For 3D imaging, the recently developed light-sheet microscopy technology (also referred to as single plane illumination microscopy) is featured with high acquisition speed, large penetration depth, low bleaching, and photocytotoxicity. Furthermore, light-sheet microscopy is particularly advantageous for long-term measurement. Here we describe an optimized protocol how to set up and handle human immune cells, e.g. primary human cytotoxic T lymphocytes (CTL) and natural killer (NK) cells in the 3D collagen matrix for usage with the light-sheet microscopy for live cell imaging and fixed samples. The procedure for image acquisition and analysis of cell migration are presented. A particular focus is given to highlight critical steps and factors for sample preparation and data analysis. This protocol can be employed for other types of suspension cells in a 3D collagen matrix and is not limited to immune cells.

摘要

在体内,免疫细胞的激活、增殖和功能均发生在三维(3D)环境中,例如在淋巴结或组织中。迄今为止,大多数体外系统依赖于二维(2D)表面,如细胞培养板或盖玻片。为了在体外最佳地模拟生理条件,我们使用了一种简单的3D胶原基质。胶原蛋白是细胞外基质(ECM)的主要成分之一,已被广泛用于构建3D基质。对于3D成像,最近开发的光片显微镜技术(也称为单平面照明显微镜)具有采集速度快、穿透深度大、漂白低和光细胞毒性低的特点。此外,光片显微镜对于长期测量特别有利。在这里,我们描述了一种优化的方案,如何在3D胶原基质中建立和处理人类免疫细胞,例如原代人类细胞毒性T淋巴细胞(CTL)和自然杀伤(NK)细胞,以便与光片显微镜一起用于活细胞成像和固定样本。介绍了细胞迁移的图像采集和分析过程。特别关注突出样本制备和数据分析的关键步骤和因素。该方案可用于3D胶原基质中的其他类型悬浮细胞,不限于免疫细胞。