Time-lapse 3D Imaging of Phagocytosis by Mouse Macrophages

吞噬作用 调理素 受体 补体受体 细胞生物学 巨噬细胞 吞噬细胞 肌动蛋白 肌动蛋白细胞骨架 细胞骨架 内化 生物 抗体调理 活体细胞成像 传出细胞增多 补体系统 化学 小胶质细胞 细胞 荧光显微镜 炎症 先天免疫系统 免疫学 抗体 生物化学
作者
Markus Horsthemke,Janine J. Wilden,Anne C. Bachg,Peter J. Hanley
出处
期刊:Journal of Visualized Experiments [MyJoVE Corporation]
卷期号: (140) 被引量:3
标识
DOI:10.3791/57566
摘要

Phagocytosis plays a key role in host defense, as well as in tissue development and maintenance, and involves rapid, receptor-mediated rearrangements of the actin cytoskeleton to capture, envelop and engulf large particles. Although phagocytic receptors, downstream signaling pathways, and effectors, such as Rho GTPases, have been identified, the dynamic cytoskeletal remodeling of specific receptor-mediated phagocytic events remain unclear. Four decades ago, two distinct mechanisms of phagocytosis, exemplified by Fcγ receptor (FcγR)- and complement receptor (CR)-mediated phagocytosis, were identified using scanning electron microscopy. Binding of immunoglobulin G (IgG)-opsonized particles to FcγRs triggers the protrusion of thin membrane extensions, which initially form a so-called phagocytic cup around the particle before it becomes completely enclosed and retracted into the cell. In contrast, complement opsonized particles appear to sink into the phagocyte following binding to complement receptors. These two modes of phagocytosis, phagocytic cup formation and sinking in, have become well established in the literature. However, the distinctions between the two modes have become blurred by reports that complement receptor-mediated phagocytosis may induce various membrane protrusions. With the availability of high resolution imaging techniques, phagocytosis assays are required that allow real-time 3D (three dimensional) visualization of how specific phagocytic receptors mediate the uptake of individual particles. More commonly used approaches for the study of phagocytosis, such as end-point assays, miss the opportunity to understand what is happening at the interface of particles and phagocytes. Here we describe phagocytic assays, using time-lapse spinning disk confocal microscopy, that allow 3D imaging of single phagocytic events. In addition, we describe assays to unambiguously image Fcγ receptor- or complement receptor-mediated phagocytosis.
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