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利用活细胞延时高内涵显微镜成像技术对离散吞噬事件进行高分辨率定量分析。

High-resolution quantification of discrete phagocytic events by live cell time-lapse high-content microscopy imaging.

机构信息

Department of Medicine and Wilmot Cancer Institute, University of Rochester Medical Center, Rochester, NY 14642, USA

Center for Vaccine Biology & Immunology, University of Rochester Medical Center, Rochester, NY 14642, USA.

出版信息

J Cell Sci. 2020 Mar 5;133(5):jcs237883. doi: 10.1242/jcs.237883.

Abstract

Phagocytosis is a dynamic process central to immunity and tissue homeostasis. Current methods for quantification of phagocytosis largely rely on indirect or static measurements, such as target clearance or dye uptake, and thus provide limited information about engulfment rates or target processing. Improved kinetic measurements of phagocytosis could provide useful, basic insights in many areas. We present a live-cell, time-lapse and high-content microscopy imaging method based on the detection and quantification of fluorescent dye 'voids' within phagocytes that result from target internalization to quantify phagocytic events with high temporal resolution. Using this method, we measure target cell densities and antibody concentrations needed for optimal antibody-dependent cellular phagocytosis. We compare void formation and dye uptake methods for phagocytosis detection, and examine the connection between target cell engulfment and phagolysosomal processing. We demonstrate how this approach can be used to measure distinct forms of phagocytosis, and changes in macrophage morphology during phagocytosis related to both engulfment and target degradation. Our results provide a high-resolution method for quantifying phagocytosis that provides opportunities to better understand the cellular and molecular regulation of this fundamental biological process.

摘要

吞噬作用是免疫和组织动态平衡的核心过程。目前用于吞噬作用定量的方法在很大程度上依赖于间接或静态的测量,如靶清除或染料摄取,因此提供的关于吞噬率或靶处理的信息有限。吞噬作用的改进动力学测量可以在许多领域提供有用的、基本的见解。我们提出了一种基于荧光染料在吞噬细胞内的“空穴”检测和定量的活细胞、延时和高内涵显微镜成像方法,该方法可用于高时间分辨率地定量吞噬作用。使用这种方法,我们测量了用于最佳抗体依赖性细胞吞噬作用的靶细胞密度和抗体浓度。我们比较了空穴形成和染料摄取方法在吞噬作用检测中的应用,并研究了靶细胞吞噬作用与吞噬体处理之间的关系。我们展示了如何使用这种方法来测量不同形式的吞噬作用,以及在吞噬作用相关的吞噬和靶降解过程中巨噬细胞形态的变化。我们的结果提供了一种高分辨率的吞噬作用定量方法,为更好地理解这个基本生物过程的细胞和分子调控提供了机会。

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