Lynch F, Shevach E M
Laboratory of Immunology, National Institutes of Allergy and Infectious Diseases, National Institutes of Health, Bethesda, MD 20892.
J Immunol. 1992 Oct 1;149(7):2307-14.
We have analyzed the requirements for the induction of proliferative responses by thymic CD4-CD8- gamma delta T cells. Enriched populations of CD4-CD8- thymocytes from newborn mice, purified by negative selection with anti-CD4, anti-CD8, and anti-TCR alpha beta mAbs were found to contain approximately 20% gamma delta T cells that were p55IL-2R-. When these cells were cultured with a panel of lymphokines (IL-1, -2, -4, and -7), a small response was observed to some of the cytokines tested individually; however, combinations of certain lymphokines (IL-1 + 2, IL-1 + 7, and IL-2 + 7) were found to induce significant proliferation and the selective outgrowth (75-90%) of gamma delta T cells. These cells were IL-2R+, remained CD4-, yet expressed variable levels of CD8. A limited analysis with specific anti-V gamma and V delta mAb suggested that there had not been a selective expansion of preexisting V gamma 2, V gamma 3, or V delta 4 populations in response to the stimulatory lymphokine combinations. Thymic CD4-CD8- gamma delta T cells were unresponsive to stimulation with immobilized anti-pan gamma delta mAb alone. However, in the presence of immobilized anti-pan gamma delta mAb and IL-1, IL-2, or IL-7, but not IL-4, a vigorous proliferative response was observed. Phenotypic analysis showed that 80 to 95% of the proliferating cells were polyclonally expanded gamma delta T cells, expressed the p55IL-2R, and the majority remained CD4-CD8-. Blocking studies with anti-IL-2R mAb showed that stimulation with anti-pan gamma delta + IL-1, but not anti-pan gamma delta + IL-7 was dependent on endogenously produced IL-2. Collectively, these studies suggest that the activation requirements of newborn thymic gamma delta T cells differ markedly from alpha beta T cells in that gamma delta T cells 1) respond to combinations of cytokines in the absence of TCR cross-linking, 2) can respond to TCR cross-linking in the presence of exogenous cytokines, 3) but are unable to activate endogenous cytokine production solely in the presence of TCR cross-linking.
我们分析了胸腺CD4-CD8-γδT细胞诱导增殖反应的条件。通过用抗CD4、抗CD8和抗TCRαβ单克隆抗体进行阴性选择纯化的新生小鼠胸腺CD4-CD8-胸腺细胞富集群体中,发现约20%的γδT细胞为p55IL-2R-。当这些细胞与一组淋巴因子(IL-1、-2、-4和-7)一起培养时,单独检测某些细胞因子时观察到轻微反应;然而,某些淋巴因子组合(IL-1 + 2、IL-1 + 7和IL-2 + 7)被发现可诱导显著增殖以及γδT细胞的选择性生长(75-90%)。这些细胞为IL-2R+,仍为CD4-,但CD8表达水平可变。用特异性抗Vγ和Vδ单克隆抗体进行的有限分析表明,针对刺激的淋巴因子组合,预先存在的Vγ2、Vγ3或Vδ4群体未出现选择性扩增。胸腺CD4-CD8-γδT细胞对单独固定的抗泛γδ单克隆抗体刺激无反应。然而,在固定的抗泛γδ单克隆抗体和IL-1、IL-2或IL-7存在的情况下,但不是IL-4,观察到强烈的增殖反应。表型分析表明,80%至95%的增殖细胞为多克隆扩增的γδT细胞,表达p55IL-2R,且大多数仍为CD4-CD8-。用抗IL-2R单克隆抗体进行的阻断研究表明,抗泛γδ + IL-1刺激,但不是抗泛γδ + IL-7刺激,依赖于内源性产生的IL-2。总体而言,这些研究表明,新生胸腺γδT细胞的激活条件与αβT细胞明显不同,即γδT细胞1)在没有TCR交联的情况下对细胞因子组合有反应,2)在存在外源性细胞因子的情况下可对TCR交联有反应,3)但仅在存在TCR交联时无法激活内源性细胞因子产生。
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