Giese T, Allison J P, Davidson W F
Laboratory of Genetics, National Cancer Institute, National Institutes of Health, Bethesda, MD 20892.
J Immunol. 1993 Jul 15;151(2):597-609.
Mice homozygous for lpr and gld develop lymphadenopathy characterized by the progressive accumulation of an unusual population of CD4-, CD8-, CD2-, IL-2R- double-negative (DN) T cells that express reduced levels of TCR-alpha/beta, high levels of CD45 (B220) and Ly-6C and variable levels of CD69. These cells are refractory to most stimuli, including staphylococcal entertoxins and cross-linking of the TCR, Ly-6C, and CD69. For normal T cells, the binding of ligand to the TCR alone is insufficient to induce a proliferative response and can result in the induction of a state of prolonged anergy. Efficient stimulation is dependent on the delivery of a second or costimulatory signal. Recently it was reported that CD28 can provide costimulatory signals to T cells and, that these signals can prevent anergy induction in T cell clones. We investigated the possibility that lpr and gld DN T cells are unresponsive because they fail to transduce signals via CD28. These studies showed that highly purified B220+ TCR-alpha/beta+ DN T cells expressed high levels of CD28, responded weakly to stimulation with PMA and anti-CD28 mAb and quite strongly to PMA, anti-CD28 antibody and high concentrations of immobilized anti-TCR-alpha/beta antibodies. The latter stimulus also induced low levels of expression of CD2 and IL-2R and secretion of modest amounts of IL-2. Although DN T cells proliferated and secreted IL-2, these responses differed qualitatively and quantitatively from those of +/+ and lprB220- T cells. Consistent with its effects on normal T cells, cyclosporin A partially inhibited the response of DN T cells to TCR cross-linking and CD28 ligation. Studies of synergism between CD28-, Ly-6C-, and CD69-mediated signals revealed that ligation of CD28 enhanced the proliferative response induced by cross-linking of Ly-6C or CD69 on +/+, lpr and gld B220- T cells but had no effect on the unresponsiveness of DN T cells to these stimuli. Ligation of CD28 did not reverse the unresponsiveness of DN T cells to SEB and had only a weak synergistic effect on the response of B220- T cells. Together, these observations suggest that the mechanisms leading to immunosuppression of DN T cells are complex and appear to involve abnormalities in signal transduction via the TCR and CD28 and possibly via Ly-6C and CD69 as well.
lpr和gld基因纯合的小鼠会出现淋巴结病,其特征是一种异常的CD4-、CD8-、CD2-、IL-2R-双阴性(DN)T细胞群体逐渐积累,这些细胞表达的TCR-α/β水平降低,CD45(B220)和Ly-6C水平升高,CD69水平可变。这些细胞对大多数刺激具有抗性,包括葡萄球菌肠毒素以及TCR、Ly-6C和CD69的交联。对于正常T细胞,单独配体与TCR的结合不足以诱导增殖反应,反而可能导致长期无反应状态的诱导。有效的刺激依赖于第二个或共刺激信号的传递。最近有报道称,CD28可以为T细胞提供共刺激信号,并且这些信号可以防止T细胞克隆中的无反应诱导。我们研究了lpr和gld DN T细胞无反应是因为它们无法通过CD28转导信号的可能性。这些研究表明,高度纯化的B220+ TCR-α/β+ DN T细胞表达高水平的CD28,对PMA和抗CD28单克隆抗体的刺激反应较弱,而对PMA、抗CD28抗体和高浓度固定化抗TCR-α/β抗体反应较强。后一种刺激还诱导了低水平的CD2和IL-2R表达以及少量IL-2的分泌。尽管DN T细胞增殖并分泌IL-2,但这些反应在质量和数量上与+/+和lprB220- T细胞的反应不同。与其对正常T细胞的作用一致,环孢素A部分抑制了DN T细胞对TCR交联和CD28连接的反应。对CD28、Ly-6C和CD69介导信号之间协同作用的研究表明,CD28的连接增强了+/+、lpr和gld B220- T细胞上Ly-6C或CD69交联诱导的增殖反应,但对DN T细胞对这些刺激的无反应性没有影响。CD28的连接并没有逆转DN T细胞对SEB的无反应性,对B220- T细胞的反应只有微弱的协同作用。总之,这些观察结果表明,导致DN T细胞免疫抑制的机制很复杂,似乎涉及通过TCR和CD28以及可能通过Ly-6C和CD69的信号转导异常。
