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A phased strategy to differentiate human CD14(+) monocytes into classically and alternatively activated macrophages and dendritic cells

机译:一种将人CD14(+)单核细胞分化为经典或替代活化巨噬细胞和树突状细胞的分阶段策略

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摘要

There are currently several in vitro strategies to differentiate human CD14(+) monocytes isolated from peripheral blood mononuclear cells (PBMCs) into the M1 or M2 macrophage cell types. Each cell type is then verified using flow cytometric analysis of cell-surface markers. Human CD14(+) monocytes have the potential to differentiate into M1 and M2 macrophages, both of which demonstrate varying degrees of cell-surface antigen overlap. Using multiple surface markers with current macrophage polarization protocols, our data reveal several limitations of currently used methods, such as highly ambiguous cell types that possess cell-surface marker overlap and functional similarities. Utilizing interleukin-6 (IL-6) and two phases of cytokine exposure, we have developed a protocol to differentiate human monocytes into M1, M2, or dendritic cells (DCs) with greater efficiency and fidelity relative to macrophages and DCs that are produced by commonly used methods. This is achieved via alterations in cytokine composition, dosing, and incubation times, as well as improvements in verification methodology. Our method reliably reproduces human in vitro monocyte-derived DCs and macrophage models that will aid in better defining and understanding innate and adaptive immunity, as well as pathologic states.
机译:当前,有几种体外策略可将从外周血单核细胞(PBMC)分离的人CD14(+)单核细胞区分为M1或M2巨噬细胞类型。然后使用细胞表面标记的流式细胞仪分析验证每种细胞类型。人CD14(+)单核细胞具有分化为M1和M2巨噬细胞的潜力,这两个都显示出不同程度的细胞表面抗原重叠。使用具有当前巨噬细胞极化方案的多个表面标记,我们的数据揭示了当前使用的方法的一些局限性,例如具有细胞表面标记重叠和功能相似性的高度模糊的细胞类型。利用白细胞介素6(IL-6)和细胞因子暴露的两个阶段,我们已经开发出一种协议,可以将人单核细胞分化为M1,M2或树突状细胞(DC),相对于由巨噬细胞和DC产生的树突状细胞和DC,它们具有更高的效率和保真度。常用方法。这是通过改变细胞因子组成,剂量和孵育时间以及改进验证方法来实现的。我们的方法能够可靠地复制人体外单核细胞衍生的DC和巨噬细胞模型,这将有助于更好地定义和理解先天免疫和适应性免疫以及病理状态。

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