Geem Duke, Medina-Contreras Oscar, Kim Wooki, Huang Clifton S, Denning Timothy L
Department of Pediatrics, Emory University.
J Vis Exp. 2012 May 21(63):e4040. doi: 10.3791/4040.
Within the intestine reside unique populations of innate and adaptive immune cells that are involved in promoting tolerance towards commensal flora and food antigens while concomitantly remaining poised to mount inflammatory responses toward invasive pathogens. Antigen presenting cells, particularly DCs and macrophages, play critical roles in maintaining intestinal immune homeostasis via their ability to sense and appropriately respond to the microbiota. Efficient isolation of intestinal DCs and macrophages is a critical step in characterizing the phenotype and function of these cells. While many effective methods of isolating intestinal immune cells, including DCs and macrophages, have been described, many rely upon long digestions times that may negatively influence cell surface antigen expression, cell viability, and/or cell yield. Here, we detail a methodology for the rapid isolation of large numbers of viable, intestinal DCs and macrophages. Phenotypic characterization of intestinal DCs and macrophages is carried out by directly staining isolated intestinal cells with specific fluorescence-labeled monoclonal antibodies for multi-color flow cytometric analysis. Furthermore, highly pure DC and macrophage populations are isolated for functional studies utilizing CD11c and CD11b magnetic-activated cell sorting beads followed by cell sorting.
在肠道内存在着独特的先天性和适应性免疫细胞群体,它们参与促进对共生菌群和食物抗原的耐受性,同时随时准备对入侵病原体发起炎症反应。抗原呈递细胞,特别是树突状细胞(DCs)和巨噬细胞,通过其感知和适当应对微生物群的能力,在维持肠道免疫稳态中发挥关键作用。高效分离肠道DCs和巨噬细胞是表征这些细胞表型和功能的关键步骤。虽然已经描述了许多分离肠道免疫细胞(包括DCs和巨噬细胞)的有效方法,但许多方法依赖于较长的消化时间,这可能会对细胞表面抗原表达、细胞活力和/或细胞产量产生负面影响。在此,我们详细介绍一种快速分离大量有活力的肠道DCs和巨噬细胞的方法。通过用特异性荧光标记单克隆抗体直接对分离的肠道细胞进行染色,以进行多色流式细胞术分析,从而对肠道DCs和巨噬细胞进行表型特征分析。此外,利用CD11c和CD11b磁激活细胞分选珠,随后进行细胞分选,分离出高度纯化的DC和巨噬细胞群体用于功能研究。