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Monoclonal iNKT cell mice reveal a role for both tissue of origin and the TCR in development of iNKT functional subsets

机译:单克隆iNKT细胞小鼠揭示了iNKT功能亚型发育过程中起源组织和TCR的作用

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摘要

iNKT cell functional subsets are defined by key transcription factors and output of cytokines such as IL-4, IFNγ, IL-17, and IL-10. To examine how TCR specificity determines iNKT function, we used somatic cell nuclear transfer to generate three lines of mice, cloned from iNKT nuclei. Each line uses the invariant Vα14Jα18 TCRα, paired with unique Vβ7 or Vβ8.2 subunits. We examined tissue homing, expression of PLZF, T-bet, and RORγt, as well as cytokine profiles and found that although monoclonal iNKT cells differentiated into all functional subsets, the NKT17 lineage was reduced or expanded depending on the TCR expressed. We examined iNKT thymic development in limited dilution bone marrow chimeras and show that higher TCR avidity correlates with higher PLZF and reduced T-bet expression. iNKT functional subsets showed distinct tissue distribution patterns. Although each individual monoclonal TCR showed an inherent subset distribution preference that was evident across all tissues examined, the iNKT cytokine profile differed more by tissue of origin than by TCR specificity.
机译:iNKT细胞功能子集由关键转录因子和细胞因子(例如IL-4,IFNγ,IL-17和IL-10)的输出定义。为了检查TCR特异性如何确定iNKT功能,我们使用了体细胞核移植来生成从iNKT核克隆的三系小鼠。每条线使用不变的Vα14Jα18TCRα,与独特的Vβ7或Vβ8.2亚基配对。我们检查了组织归巢,PLZF,T-bet和RORγt的表达以及细胞因子谱,发现尽管单克隆iNKT细胞分化为所有功能亚群,但NKT17谱系根据表达的TCR有所减少或扩大。我们检查了有限稀释的骨髓嵌合体中的iNKT胸腺发育,并显示更高的TCR亲和力与更高的PLZF和降低的T-bet表达相关。 iNKT功能子集显示出不同的组织分布模式。尽管每个单独的TCR单克隆抗体都表现出固有的子集分布偏好,这一点在所有检查过的组织中均很明显,但iNKT细胞因子的分布在起源组织上的差异要大于在TCR特异性方面的差异。

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