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Comparison of bone marrow-derived and mucosal mast cells in controlling intramacrophage Francisella tularensis replication

机译:骨髓衍生和粘液肥粘土细胞控制控制肠道颅骨菌骨髓复制的比较

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摘要

Although the importance of mast cells (MCs) in response to allergens has been characterized extensively, the contribution of these cells in host defense against bacterial pathogens is not well understood. Previously, we have demonstrated that the release of interleukin-4 by bone marrow-derived MCs inhibits intramacrophage replication of Francisella tularensis live vaccine strain (LVS). Because pneumonic tularemia is one of the several manifestations of infection by Francisella, it is important to determine whether MCs present in mucosal tissues, i.e. the lung, exhibit similar effects on LVS replication. On the basis of this rationale, we phenotypically compared mucosal mast cells (MMCs) to traditional bone marrow-derived MCs. Both cell types exhibited similar levels of cell surface expression of fragment crystal epsilon receptor I (FcεRI), mast/ stem cell growth factor receptor (c-Kit) and major histocompatibility complex I (MHCI), as well as patterns of granulation. MMCs exhibited a comparable, but somewhat greater uptake of fluorescent-labeled beads compared with MCs, suggesting an increased phagocytic ability. MCs and MMCs co-cultured with primary macrophages exhibited comparable significant decreases in LVS replication compared with macrophages cultured alone. Collectively, these results suggest that MMCs are phenotypically similar to MCs and appear equally effective in the control of intramacrophage F. tularensis LVS replication.
机译:虽然肥大细胞(MCS)对过敏原的重要性已经广泛表征,但是对细菌病原体的宿主防御这些细胞对细菌病原体的贡献并不了解。以前,我们已经证明,通过骨髓衍生的MCS释放白细胞介素-4抑制了Francisella Tularentsis活疫苗菌株(LVS)的肠道畏缩复制。由于肺炎术术是弗朗西亚感染的几种表现之一,重要的是要确定粘膜组织中是否存在MCS,即肺部,对LVS复制表现出类似的效果。基于该理由,我们将粘膜肥大细胞(MMC)与传统的骨髓衍生的MCs进行了表型。两种细胞类型表现出类似水平的片段晶体ε受体I(FcεRI)的细胞表面表达水平,肥大/干细胞生长因子受体(C-KIT)和主要的组织相容性络合物I(MHCI)以及造粒的图案。与MCS相比,MMCS表现出可比较,但有点更大吸收荧光标记的珠子,表明吞噬能力增加。与单独培养的巨噬细胞相比,与初级巨噬细胞共同培养的MCS和MMCs在LVS复制中表现出相当的显着降低。总的来说,这些结果表明MMCS与MCS相似,并且在肠道噬菌体F.Tularensis LVS复制的控制中表现出同样有效。

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