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1
A 275 basepair fragment at the 5' end of the interleukin 2 gene enhances expression from a heterologous promoter in response to signals from the T cell antigen receptor.白细胞介素2基因5'端的一个275个碱基对的片段,可响应来自T细胞抗原受体的信号,增强异源启动子的表达。
J Exp Med. 1987 Feb 1;165(2):395-407. doi: 10.1084/jem.165.2.395.
2
Definition of a GC-rich motif as regulatory sequence of the human IL-3 gene: coordinate regulation of the IL-3 gene by CLE2/GC box of the GM-CSF gene in T cell activation.富含鸟嘌呤-胞嘧啶(GC)的基序作为人白细胞介素-3(IL-3)基因调控序列的定义:在T细胞活化过程中,GM-CSF基因的CLE2/GC盒对IL-3基因的协同调控
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3
Expression of the type 1 human immunodeficiency virus Nef protein in T cells prevents antigen receptor-mediated induction of interleukin 2 mRNA.1型人类免疫缺陷病毒Nef蛋白在T细胞中的表达可阻止抗原受体介导的白细胞介素2信使核糖核酸的诱导。
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CD28-stimulated IL-2 gene expression in Jurkat T cells occurs in part transcriptionally and is cyclosporine-A sensitive.在Jurkat T细胞中,CD28刺激的白细胞介素-2基因表达部分发生在转录水平,且对环孢素A敏感。
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8
Role of T3 surface molecules in human T-cell activation: T3-dependent activation results in an increase in cytoplasmic free calcium.T3 表面分子在人 T 细胞活化中的作用:T3 依赖性活化导致细胞质游离钙增加。
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Multiple signals are required for function of the human granulocyte-macrophage colony-stimulating factor gene promoter in T cells.人类粒细胞-巨噬细胞集落刺激因子基因启动子在T细胞中发挥功能需要多种信号。
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Abnormal T cells from MRL/Mp-lpr/lpr mice do not respond to anti-T-cell-receptor antibody or tumor promoter and calcium ionophore A23187 despite the presence of the T-cell-receptor complex and protein kinase c.来自MRL/Mp-lpr/lpr小鼠的异常T细胞,尽管存在T细胞受体复合物和蛋白激酶c,但对抗T细胞受体抗体、肿瘤启动子和钙离子载体A23187均无反应。
Cell Immunol. 1988 Apr 15;113(1):82-94. doi: 10.1016/0008-8749(88)90008-1.

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本文引用的文献

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Antigen recognition by human T lymphocytes is linked to surface expression of the T3 molecular complex.人类T淋巴细胞对抗原的识别与T3分子复合物的表面表达相关联。
Cell. 1982 Oct;30(3):735-43. doi: 10.1016/0092-8674(82)90278-1.
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Absolute requirement for adherent cells in the production of human interleukin 2 (IL2).人白细胞介素2(IL2)生产中对贴壁细胞的绝对需求。
Cell Immunol. 1981 Sep 1;63(1):71-80. doi: 10.1016/0008-8749(81)90029-0.
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Recombinant genomes which express chloramphenicol acetyltransferase in mammalian cells.在哺乳动物细胞中表达氯霉素乙酰转移酶的重组基因组。
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Cyclosporin A inhibits T-cell growth factor gene expression at the level of mRNA transcription.环孢菌素A在信使核糖核酸转录水平抑制T细胞生长因子基因的表达。
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The role of T3 surface molecules in the activation of human T cells: a two-stimulus requirement for IL 2 production reflects events occurring at a pre-translational level.T3表面分子在人T细胞激活中的作用:白细胞介素2产生的双刺激需求反映了翻译前水平发生的事件。
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Structure of the human interleukin 2 gene.人类白细胞介素2基因的结构
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Specific factor conferring nuclease hypersensitivity at the 5' end of the chicken adult beta-globin gene.赋予鸡成年β-珠蛋白基因5'端核酸酶超敏感性的特定因子。
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Identification of two distinct regulatory regions adjacent to the human beta-interferon gene.鉴定出与人类β-干扰素基因相邻的两个不同调控区域。
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白细胞介素2基因5'端的一个275个碱基对的片段,可响应来自T细胞抗原受体的信号,增强异源启动子的表达。

A 275 basepair fragment at the 5' end of the interleukin 2 gene enhances expression from a heterologous promoter in response to signals from the T cell antigen receptor.

作者信息

Durand D B, Bush M R, Morgan J G, Weiss A, Crabtree G R

出版信息

J Exp Med. 1987 Feb 1;165(2):395-407. doi: 10.1084/jem.165.2.395.

DOI:10.1084/jem.165.2.395
PMID:3102668
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2188523/
Abstract

Using a transient transfection assay, we have defined the sequences required for the activation of the IL-2 gene in response to signals from the T cell antigen receptor. To do so we have transfected the human T cell line Jurkat with hybrid DNA constructs in which fragments from the IL-2 gene are linked to an indicator gene. The indicator gene product, as well as IL-2 production from the endogenous IL-2 gene were assayed after activation of the transfected Jurkat cells by various stimuli. We have demonstrated that a 275 bp fragment stretching from 52 to 326 bp upstream of the IL-2 gene transcription initiation site is required for expression of the linked indicator gene. This IL-2 gene fragment has several of the characteristics of a transcriptional enhancer element, in that it functions in both orientations and will enhance the expression from the promoter of an unrelated gene. Such enhancement occurred only after activation of Jurkat cells through the T cell antigen receptor. More specifically, this 275 bp fragment activated the expression of a linked gene after binding of a monoclonal antibody to the Jurkat T cell antigen receptor in the presence of PMA. In addition, calcium ionophore, which circumvents antigen receptor binding in T cell activation, induced the expression of the linked gene through this 275 bp sequence, in the presence of PMA. Finally, in a mutant Jurkat cell line lacking T3/antigen receptor complexes at the cell surface, no expression due to the IL-2 5' flanking region was seen after exposure to antibody to the T cell antigen receptor plus PMA or to PHA plus PMA. In contrast, calcium ionophore plus PMA did induce the expression of a linked gene through the IL-2 5' flanking region in the mutant Jurkat cell line. The responsiveness of the transfected hybrid genes containing the IL-2 regulatory region paralleled the expression of the endogenous IL-2 gene, as determined by IL-2 bioassays. We conclude that the 275 bp IL-2 sequence (-326 to -52 bp) is a target for the signal pathway originating at the T cell antigen receptor. Definition of this 275 bp target sequence should now permit the isolation of the molecules that bind to and activate the IL-2 gene.

摘要

利用瞬时转染分析,我们确定了白介素-2(IL-2)基因在响应来自T细胞抗原受体的信号时被激活所需的序列。为此,我们用杂交DNA构建体转染了人T细胞系Jurkat,其中来自IL-2基因的片段与一个指示基因相连。在用各种刺激激活转染的Jurkat细胞后,检测指示基因产物以及内源性IL-2基因产生的IL-2。我们已经证明,在IL-2基因转录起始位点上游从52到326 bp延伸的一个275 bp片段是连接的指示基因表达所必需的。这个IL-2基因片段具有转录增强子元件的几个特征,即它在两个方向上都起作用,并且会增强来自无关基因启动子的表达。这种增强仅在通过T细胞抗原受体激活Jurkat细胞后发生。更具体地说,在存在佛波酯(PMA)的情况下,单克隆抗体与Jurkat T细胞抗原受体结合后,这个275 bp片段激活了连接基因的表达。此外,在存在PMA的情况下,钙离子载体绕过T细胞激活中抗原受体的结合,通过这个275 bp序列诱导连接基因的表达。最后,在细胞表面缺乏T3/抗原受体复合物的突变Jurkat细胞系中,在用抗T细胞抗原受体抗体加PMA或用植物血凝素(PHA)加PMA处理后,未观察到由于IL-2 5'侧翼区域导致的表达。相反,钙离子载体加PMA确实通过IL-2 5'侧翼区域在突变Jurkat细胞系中诱导了连接基因的表达。通过IL-2生物测定确定,含有IL-2调控区域的转染杂交基因的反应性与内源性IL-2基因的表达平行。我们得出结论,275 bp的IL-2序列(-326至-52 bp)是源自T细胞抗原受体的信号通路的靶点。现在对这个275 bp靶序列的定义应该允许分离与IL-2基因结合并激活它的分子。