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Quantitative label-free single cell tracking in 3D biomimetic matrices

机译:在3D仿生矩阵中进行无标记的定量单细胞跟踪

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摘要

Live cell imaging enables an observation of cell behavior over a period of time and is a growing field in modern cell biology. Quantitative analysis of the spatio-temporal dynamics of heterogeneous cell populations in three-dimensional (3D) microenvironments contributes a better understanding of cell-cell and cell-matrix interactions for many biomedical questions of physiological and pathological processes. However, current live cell imaging and analysis techniques are frequently limited by non-physiological 2D settings. Furthermore, they often rely on cell labelling by fluorescent dyes or expression of fluorescent proteins to enhance contrast of cells, which frequently affects cell viability and behavior of cells. In this work, we present a quantitative, label-free 3D single cell tracking technique using standard bright-field microscopy and affordable computational resources for data analysis. We demonstrate the efficacy of the automated method by studying migratory behavior of a large number of primary human macrophages over long time periods of several days in a biomimetic 3D microenvironment. The new technology provides a highly affordable platform for long-term studies of single cell behavior in 3D settings with minimal cell manipulation and can be implemented for various studies regarding cell-matrix interactions, cell-cell interactions as well as drug screening platform for primary and heterogeneous cell populations.
机译:活细胞成像可以观察一段时间内的细胞行为,并且是现代细胞生物学中一个不断发展的领域。三维(3D)微环境中的异质细胞群体的时空动态的定量分析有助于更好地了解许多细胞和细胞-基质相互作用的生理和病理过程的许多生物医学问题。但是,当前的活细胞成像和分析技术通常受到非生理2D设置的限制。此外,它们通常依靠荧光染料对细胞进行标记或荧光蛋白的表达来增强细胞的对比度,这经常影响细胞的活力和行为。在这项工作中,我们提出了一种使用标准明场显微镜和可负担的计算资源进行数据分析的定量无标签3D单细胞跟踪技术。我们通过在仿生3D微环境中研究数天的长时间内大量初级人类巨噬细胞的迁徙行为,证明了自动化方法的功效。这项新技术为3D设置下的单细胞行为的长期研究提供了一种价格低廉的平台,并且只需极少的细胞操作,就可以用于有关细胞-基质相互作用,细胞-细胞相互作用的各种研究,以及用于原发性和中性的药物筛选平台异质细胞群。

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