Michelle L Niese, Nicole Glosson-Byers, Ana Paula Moreira Serezani, Nada S Alakhras, Mark H Kaplan
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引用次数: 0
Abstract
The polarization of naive Th cells into differentiated subsets in vitro was a powerful approach to define the development and function of Th cells in vivo. Th cell cultures identified cytokines that promote polarization and defined the phenotype and stability of differentiated cells. One of the limitations of this approach is the heterogeneity of the differentiated culture, essentially with regard to what proportion of the culture is secreting the hallmark cytokine of interest. This heterogeneity has always been puzzling because all cells in the culture have been exposed to identical culture conditions. We examined this phenomenon using an Il17f lineage-tracing allele (Cost, Cre on seventeen transcript) crossed to stop-flox Rosa-YFP (yellow fluorescent protein) mice. We found that less than half of the cells in a Th17 culture become lineage-positive during a differentiation culture and that it is primarily cells that are lineage-positive that produce cytokines when cultures are restimulated after differentiation. We sorted and analyzed YFP-positive and YFP-negative cells and found similar expression of many Th17 transcription factors, although YFP-negative cells had increased expression of other lineage-defining transcription factors. We observed that YFP-negative cells had diminished expression of Stat3 and Il6ra, as well as decreased STAT3 activation. YFP-negative cells transduced with active STAT3 had significant increases in IL-17A expression, without increases in Th17 transcription factors. Taken together, these data suggest that there is a threshold of STAT3 activation that is required for efficient Th17 differentiation, and that even in a culture of homogeneous naive T cells there is heterogeneity in the receipt of early cytokine signals.
在体外将幼稚Th细胞极化为分化的亚群是确定体内Th细胞发育和功能的有力方法。Th细胞培养物鉴定了促进极化的细胞因子,并确定了分化细胞的表型和稳定性。这种方法的局限性之一是分化培养物的异质性,本质上是关于培养物中分泌感兴趣的标志性细胞因子的比例。这种异质性一直令人困惑,因为培养物中的所有细胞都暴露在相同的培养条件下。我们使用Il17f谱系追踪等位基因(Cost,Cre on seventeen转录物)杂交来阻止荧光蛋白(黄色荧光蛋白)小鼠来检测这种现象。我们发现,Th17培养物中不到一半的细胞在分化培养过程中成为谱系阳性,并且当分化后重新刺激培养物时,主要是谱系阳性细胞产生细胞因子。我们对YFP阳性和YFP阴性细胞进行了分类和分析,发现许多Th17转录因子表达相似,尽管YFP阴性的细胞增加了其他谱系定义转录因子的表达。我们观察到YFP阴性细胞的Stat3和Il6ra表达减少,Stat3激活减少。用活性STAT3转导的YFP阴性细胞的IL-17A表达显著增加,而Th17转录因子没有增加。总之,这些数据表明,存在有效Th17分化所需的STAT3激活阈值,并且即使在同质幼稚T细胞的培养中,早期细胞因子信号的接收也存在异质性。