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在缺乏白细胞介素-12和白细胞介素-4的情况下产生的人辅助性T细胞1型(Th1)和辅助性T细胞2型(Th2)中信号转导和转录激活因子(STAT)蛋白及细胞因子基因的激活。

Activation of STAT proteins and cytokine genes in human Th1 and Th2 cells generated in the absence of IL-12 and IL-4.

作者信息

Moriggl R, Kristofic C, Kinzel B, Volarevic S, Groner B, Brinkmann V

机构信息

Institute for Experimental Cancer Research, Tumor Biology Center, Freiburg, Germany.

出版信息

J Immunol. 1998 Apr 1;160(7):3385-92.

PMID:9531298
Abstract

We have shown previously that human CD4+ 45RO- T cells could be primed for a Th2 phenotype independent of IL-4 if they were activated by anti-CD28 mAb plus IL-2. If additional TCR signals were provided, the cells differentiated toward Th1 independent of IL-12. Here we show that anti-CD28/IL-2-primed Th2 cells expressed high levels of activated STAT6, but no cytokine mRNA. Moreover, both Th1 and Th2 cells expressed active STAT1 and -3, but not STAT2, -4, and -5. Restimulation of Th1 or Th2 cells via CD3 plus CD28 induced production of IFN-gamma or IL-4, respectively, but did not alter the activation status/DNA binding activity of STATs. Addition of IL-4 (or anti-IL-4 mAb) to restimulated Th2 cells did not modulate STAT6 activation or IL-4 expression, confirming the full commitment. However, Th2 cells remained responsive to IL-12, which repressed STAT6 DNA binding but activated STAT4, and this coincided with a suppression of IL-4/IL-5 and an induction of IFN-gamma. In Th1 cells, IL-12 activated both STAT6 and STAT4, and IL-4 activated STAT6, but in both cases the Th1 phenotype remained. Together the data show that CD28/IL-2-dependent Th2 priming activated STAT6 without inducing IL-4 expression. The primed Th cells resembled memory cells and produced IL-4 upon the first CD3/CD28 costimulus without detectable modulation of STATs. Th2 cells remained responsive to IL-12, which repressed STAT6 DNA binding and activated STAT4, and switched the cells to Th1. The effects of IL-12 may depend on the commitment of the cells, since IL-12 phosphorylated STAT6 in Th1 and dephosphorylated STAT6 in Th2 cells.

摘要

我们之前已经表明,如果人CD4+ 45RO- T细胞被抗CD28单克隆抗体加IL-2激活,它们可以在不依赖IL-4的情况下被诱导为Th2表型。如果提供额外的TCR信号,这些细胞会在不依赖IL-12的情况下分化为Th1细胞。在这里我们表明,抗CD28/IL-2诱导的Th2细胞表达高水平的活化STAT6,但没有细胞因子mRNA。此外,Th1和Th2细胞均表达活性STAT1和-3,但不表达STAT2、-4和-5。通过CD3加CD28再次刺激Th1或Th2细胞分别诱导IFN-γ或IL-4的产生,但不会改变STAT的激活状态/DNA结合活性。向再次刺激的Th2细胞中添加IL-4(或抗IL-4单克隆抗体)不会调节STAT6的激活或IL-4的表达,证实了其完全分化状态。然而,Th2细胞仍然对IL-12有反应,IL-12会抑制STAT6的DNA结合但激活STAT4,这与IL-4/IL-5的抑制和IFN-γ的诱导同时发生。在Th1细胞中,IL-12激活STAT6和STAT4,IL-4激活STAT6,但在这两种情况下Th1表型都保持不变。这些数据共同表明,CD28/IL-2依赖的Th2诱导激活了STAT6,但没有诱导IL-4的表达。诱导的Th细胞类似于记忆细胞,在第一次CD3/CD28共刺激时产生IL-4,而STAT没有可检测到的调节。Th2细胞仍然对IL-12有反应,IL-12会抑制STAT6的DNA结合并激活STAT4,并将细胞转变为Th1细胞。IL-12的作用可能取决于细胞的分化状态,因为IL-12在Th1细胞中使STAT6磷酸化,而在Th2细胞中使STAT6去磷酸化。

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