Nanoparticulate systems have emerged as valuable tools in vaccine delivery through their ability to efficiently deliver cargo, including proteins, to antigen presenting cells1-5. Internalization of nanoparticles (NP) by antigen presenting cells is a critical step in generating an effective immune response to the encapsulated antigen. To determine how changes in nanoparticle formulation impact function, we sought to develop a high throughput, quantitative experimental protocol that was compatible with detecting internalized nanoparticles as well as bacteria. To date, two independent techniques, microscopy and flow cytometry, have been the methods used to study the phagocytosis of nanoparticles. The high throughput nature of flow cytometry generates robust statistical data. However, due to low resolution, it fails to accurately quantify internalized versus cell bound nanoparticles. Microscopy generates images with high spatial resolution; however, it is time consuming and involves small sample sizes6-8. Multi-spectral imaging flow cytometry (MIFC) is a new technology that incorporates aspects of both microscopy and flow cytometry that performs multi-color spectral fluorescence and bright field imaging simultaneously through a laminar core. This capability provides an accurate analysis of fluorescent signal intensities and spatial relationships between different structures and cellular features at high speed.Herein, we describe a method utilizing MIFC to characterize the cell populations that have internalized polyanhydride nanoparticles or Salmonella enterica serovar Typhimurium. We also describe the preparation of nanoparticle suspensions, cell labeling, acquisition on an ImageStreamX system and analysis of the data using the IDEAS application. We also demonstrate the application of a technique that can be used to differentiate the internalization pathways for nanoparticles and bacteria by using cytochalasin-D as an inhibitor of actin-mediated phagocytosis.
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机译:纳米颗粒系统已经能够有效地将货物(包括蛋白质)输送到抗原呈递细胞 1-5 ,从而成为疫苗输送中的重要工具。抗原呈递细胞将纳米颗粒(NP)内在化是对封装的抗原产生有效免疫应答的关键步骤。为了确定纳米颗粒配方的变化如何影响功能,我们寻求开发一种高通量,定量实验方案,该方案与检测内在化的纳米颗粒以及细菌兼容。迄今为止,显微镜和流式细胞术这两种独立的技术已经成为研究纳米颗粒吞噬作用的方法。流式细胞仪的高通量性质可生成可靠的统计数据。然而,由于分辨率低,它无法准确地量化内在的与细胞结合的纳米颗粒。显微镜产生具有高空间分辨率的图像;但是,这很耗时,并且涉及的样本量小( 6-8 )。多光谱成像流式细胞仪(MIFC)是一项结合了显微镜和流式细胞仪技术的新技术,可同时通过层流核心执行多色光谱荧光和明场成像。此功能可快速准确分析荧光信号强度以及不同结构与细胞特征之间的空间关系。在此,我们描述了一种利用MIFC表征内化聚酸酐纳米颗粒或肠炎沙门氏菌血清鼠伤寒沙门氏菌的细胞群体的方法。我们还描述了纳米颗粒悬浮液的制备,细胞标记,在ImageStream X 系统上的采集以及使用IDEAS应用程序对数据的分析。我们还展示了一种技术的应用,该技术可通过使用细胞松弛素-D作为肌动蛋白介导的吞噬作用的抑制剂来区分纳米颗粒和细菌的内在化途径。
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