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Obtainment of Macrophages from Human Monocytes to Assess <em>Leishmania braziliensis</em> Infection Rate and Innate Host Immune Response

免疫系统 生物 巨噬细胞 免疫学 外周血单个核细胞 先天免疫系统 抗原 微生物学 体外 生物化学
作者
Ícaro Bonyek-Silva,Sara Nunes,Rana Bastos,Reinan Lima,Leilane Barbosa,G. Grimaldi,Vinícius Pinto Costa Rocha,Milena Botelho Pereira Soares,Patrícia Sampaio Tavares Veras,Juliana de Menezes,Cláudia Brodskyn,Natália Machado Tavares
出处
期刊:Journal of Visualized Experiments [MyJoVE Corporation]
卷期号: (174) 被引量:3
标识
DOI:10.3791/62555
摘要

Macrophages are multifunctional cells essential to the immune system function, and the primary host cell in Leishmania braziliensis (Lb) infection. These cells are specialized in microorganism recognition and phagocytosis, but also activate other immune cells and present antigens, as well as promote inflammation and tissue repair. Here, we describe a protocol to obtain mononuclear cells from peripheral blood (PBMC) of healthy donors to separate monocytes that then differentiate into macrophages. These cells can then be infected in vitro at different Lb concentrations to evaluate the ability to control infection, as well as evaluate host cell immune response, which can be measured by several methods. PBMCs were first isolated by centrifuging with Ficoll-Hypaque gradient and then plated to allow monocytes to adhere to culture plates; non-adherent cells were removed by washing. Next, adherent cells were cultured with macrophage-colony stimulating factor (M-CSF) for 7 days to induce macrophage differentiation. We suggest plating 2 x 106 cells per well on 24-well plates in order to obtain 2 x 105 macrophages. Fully differentiated macrophages can then be infected with Lb for 4 or 24 hours. This protocol results in a significant percentage of infected cells, which can be assessed by optical or fluorescence microscopy. In addition to infection index, parasite load can be measured by counting the numbers of parasites inside each cell. Further molecular and functional assays can also be performed in culture supernatants or within the macrophages themselves, which allows this protocol to be applied in a variety of contexts and also adapted to other intracellular parasite species.

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