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CD3结合的价态以及CD3细胞表面复合物的内化控制T细胞对第二信号的反应:对蛋白激酶C、细胞质游离钙和增殖影响的差异。

Valency of CD3 binding and internalization of the CD3 cell-surface complex control T cell responses to second signals: distinction between effects on protein kinase C, cytoplasmic free calcium, and proliferation.

作者信息

Ledbetter J A, June C H, Martin P J, Spooner C E, Hansen J A, Meier K E

出版信息

J Immunol. 1986 Jun 1;136(11):3945-52.

PMID:3084650
Abstract

We have studied the relationship of valency of CD3 stimulation and modulation of the CD3 receptor complex with biochemical and proliferative responses of T cells. Anti-CD3 Fab, as well as F(ab')2 and whole antibody caused rapid modulation of the CD3 antigen, whereas anti-CD3 conjugated to Sepharose did not. In the absence of monocytes, T cells stimulated with anti-CD3 Fab, F(ab')2, or F(ab')2-Sepharose showed differences in their ability to respond to second signals given by PMA, IL 1, IL 2, or antibodies to Tp67 and Tp44. None of the anti-CD3 signals alone caused resting T cells to produce IL 2, and only the Sepharose-bound anti-CD3 F(ab')2 caused T cells to express high levels of functional IL 2 receptors. Anti-CD3 F(ab')2-Sepharose-stimulated T cells produced IL 2 and proliferated in response to each of the second signals. Because anti-CD3-Sepharose did not cause modulation of the CD3 antigen, the ability of the Sepharose-bound antibody to induce T cells to express IL 2 receptors and to respond to individual second signals may be related to lack of modulation rather than valency of binding. Anti-CD3 Fab-stimulated T cells responded to PMA but required combinations of other second signals. T cells stimulated with unmodified anti-CD3 antibody or F(ab')2 fragments responded to PMA but did not respond to any other second signals alone or in combination. Stimulations that resulted in modulation (i.e., anti-CD3 whole antibody, anti-CD3 F(ab')2, or anti-CD3 Fab fragments) caused an increase in cytoplasmic calcium levels in resting T cells but blocked proliferation of T cells in response to mitogenic lectins or CD2 stimulation. Anti-CD3 F(ab')2 on Sepharose, however, did not block T cell proliferation. Whole bivalent anti-CD3 antibody or F(ab')2 fragments, but not monovalent Fab fragments, caused a rapid translation of protein kinase C activity from cytosol to membrane in the Jurkat T cell line. Because all of these modulate the receptor, these data indicate that the functional difference between monovalent and bivalent binding to CD3 is related to antibody valency and not to antigenic modulation. The use of Fab anti-CD3 stimulation that requires combinations of second signals for proliferation allowed an analysis of the functional relationships between IL 1, anti-Tp67, and anti-Tp44.

摘要

我们研究了CD3刺激的价态以及CD3受体复合物的调节与T细胞生化和增殖反应之间的关系。抗CD3 Fab以及F(ab')2和完整抗体均可导致CD3抗原的快速调节,而与琼脂糖偶联的抗CD3则不会。在没有单核细胞的情况下,用抗CD3 Fab、F(ab')2或F(ab')2 - 琼脂糖刺激的T细胞,在对PMA、IL - 1、IL - 2或针对Tp67和Tp44的抗体给出的第二信号作出反应的能力上存在差异。单独的抗CD3信号均不能使静息T细胞产生IL - 2,只有与琼脂糖结合的抗CD3 F(ab')2能使T细胞表达高水平的功能性IL - 2受体。抗CD3 F(ab')2 - 琼脂糖刺激的T细胞可产生IL - 2,并对每种第二信号作出增殖反应。由于抗CD3 - 琼脂糖不会引起CD3抗原的调节,与琼脂糖结合的抗体诱导T细胞表达IL - 2受体并对单个第二信号作出反应的能力,可能与缺乏调节有关,而非结合价态。抗CD3 Fab刺激的T细胞对PMA有反应,但需要其他第二信号的组合。用未修饰的抗CD3抗体或F(ab')2片段刺激的T细胞对PMA有反应,但单独或联合使用时对任何其他第二信号均无反应。导致调节的刺激(即抗CD3完整抗体、抗CD3 F(ab')2或抗CD3 Fab片段)会使静息T细胞的细胞质钙水平升高,但会阻断T细胞对促有丝分裂凝集素或CD2刺激的增殖反应。然而,琼脂糖上的抗CD3 F(ab')2不会阻断T细胞增殖。完整的二价抗CD3抗体或F(ab')2片段,而不是单价Fab片段,可使Jurkat T细胞系中的蛋白激酶C活性从胞质溶胶快速转移至细胞膜。由于所有这些都会调节受体,这些数据表明与CD3的单价和二价结合之间的功能差异与抗体价态有关,而非与抗原调节有关。使用需要第二信号组合才能增殖的Fab抗CD3刺激,可分析IL - 1、抗Tp67和抗Tp44之间的功能关系。

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