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CD28共刺激与无反应性对白介素-2表达的分子调控

Molecular regulation of interleukin-2 expression by CD28 co-stimulation and anergy.

作者信息

Powell J D, Ragheb J A, Kitagawa-Sakakida S, Schwartz R H

机构信息

Laboratory of Cellular and Molecular Immunology, National Institutes of Health, Bethesda, MD 20892-0420, USA.

出版信息

Immunol Rev. 1998 Oct;165:287-300. doi: 10.1111/j.1600-065x.1998.tb01246.x.

DOI:10.1111/j.1600-065x.1998.tb01246.x
PMID:9850868
Abstract

The consequences of T-cell receptor engagement (signal 1) are profoundly affected by the presence or absence of co-stimulation (signal 2). T-cell receptor (TCR) stimulation in the absence of CD28-mediated co-stimulation not only results in little interleukin (IL)-2 production, but induces a long lasting hyporesponsive state known as T-cell clonal anergy. The addition of CD28 ligation to signal 1, on the other hand, results in the production of copious amounts of IL-2. Our laboratory has utilized CD4+ Th 1 clones in an effort to understand the molecular events resulting in enhanced IL-2 production by co-stimulation and the inhibition of IL-2 production in anergy. Our current studies have focused on defining the post-transcriptional effects of CD28-enhanced IL-2 production. The data suggest that a major component of CD28's ability to regulate IL-2 production occurs at the level of message stability and involves the 3'-untranslated region of the message. In terms of anergy, our recent studies support the notion that it is not the result of TCR engagement in the absence of co-stimulation, but rather signal 1 in the absence of IL-2 receptor signaling and proliferation. Furthermore, T-cell anergy appears to be an active negative state in which IL-2 production is inhibited both at the level of signal transduction and by cis-dominant repression at the level of the IL-2 promoter.

摘要

T细胞受体激活(信号1)的后果会受到共刺激(信号2)存在与否的深刻影响。在缺乏CD28介导的共刺激情况下进行T细胞受体(TCR)刺激,不仅导致白细胞介素(IL)-2产生极少,还会诱导一种持久的低反应状态,即T细胞克隆无能。另一方面,在信号1基础上添加CD28连接会导致产生大量IL-2。我们实验室利用CD4+ Th1克隆来试图理解通过共刺激增强IL-2产生以及在无能状态下抑制IL-2产生所涉及的分子事件。我们目前的研究聚焦于确定CD28增强IL-2产生的转录后效应。数据表明,CD28调节IL-2产生的能力的一个主要成分发生在信使稳定性水平,并且涉及信使的3'非翻译区。就无能状态而言,我们最近的研究支持这样一种观点,即它不是在缺乏共刺激时TCR激活的结果,而是在缺乏IL-2受体信号传导和增殖时信号1的结果。此外,T细胞无能似乎是一种活跃的负性状态,其中IL-2产生在信号转导水平以及在IL-2启动子水平通过顺式显性抑制均受到抑制。

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