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佛波酯/钙离子载体与植物血凝素诱导的人T淋巴细胞信号传导的比较。白细胞介素2非依赖性转铁蛋白受体基因表达的证明。

Comparison of phorbol ester/calcium ionophore and phytohemagglutinin-induced signaling in human T lymphocytes. Demonstration of interleukin 2-independent transferrin receptor gene expression.

作者信息

Kumagai N, Benedict S H, Mills G B, Gelfand E W

机构信息

Division of Immunology/Rheumatology, Hospital for Sick Children, Toronto, Ontario, Canada.

出版信息

J Immunol. 1988 Jan 1;140(1):37-43.

PMID:3121740
Abstract

The proliferation of human T lymphocytes is regulated, in part, by the coordinated expression of genes encoding T cell growth factor (interleukin 2 (IL-2), IL-2 receptors, and transferrin receptors (TFR). We examined the time course of accumulation of mRNA for these genes in T cells stimulated with the phorbol ester, phorbol 12,13-dibutyrate (PDB) and the calcium ionophore, ionomycin, and compared their expression to T cells stimulated with phytohemagglutinin. In cells treated with PDB/ionomycin, maximum expression was observed at 3 hr for IL-2 mRNA and at 6 hr for TFR mRNA, whereas the level of IL-2 receptor mRNA reached a peak 24 to 48 hr after stimulation. In phytohemagglutinin-stimulated T cells IL-2 mRNA was detectable within 3 hr but peaked later at 12 hr; the level of IL-2 receptor mRNA similarly peaked 24 to 48 hr later. Accumulation of TFR mRNA in phytohemagglutinin-stimulated T cells, however, was not detectable at 6 hr and reached a peak only between 12 to 24 hr. The early accumulation of TFR mRNA in PDB/ionomycin-stimulated T cells seemed, in part, independent of the interaction of IL-2 with its own receptor, because TFR mRNA was detectable as early as 1 hr after stimulation and addition of cycloheximide before addition of PDB/ionomycin did not abolish the PDB/ionomycin-induced accumulation of TFR mRNA. In addition, either PDB or ionomycin used alone induced the expression of TFR mRNA but not IL-2 mRNA. These results indicated that the combination of PDB/ionomycin accelerated the expression of IL-2 and TFR genes in T cells compared to phytohemagglutinin and triggered an IL-2-independent pathway for the induction of TFR mRNA.

摘要

人类T淋巴细胞的增殖部分受编码T细胞生长因子(白细胞介素2(IL-2)、IL-2受体和转铁蛋白受体(TFR))的基因的协调表达调控。我们检测了用佛波酯、佛波醇12,13 - 二丁酸酯(PDB)和钙离子载体离子霉素刺激的T细胞中这些基因的mRNA积累的时间进程,并将它们的表达与用植物血凝素刺激的T细胞进行比较。在用PDB/离子霉素处理的细胞中,IL-2 mRNA在3小时达到最大表达,TFR mRNA在6小时达到最大表达,而IL-2受体mRNA水平在刺激后24至48小时达到峰值。在植物血凝素刺激的T细胞中,IL-2 mRNA在3小时内可检测到,但在12小时后达到峰值;IL-2受体mRNA水平同样在24至48小时后达到峰值。然而,在植物血凝素刺激的T细胞中,TFR mRNA在6小时时无法检测到,仅在12至24小时之间达到峰值。PDB/离子霉素刺激的T细胞中TFR mRNA的早期积累似乎部分独立于IL-2与其自身受体的相互作用,因为早在刺激后1小时就可检测到TFR mRNA,并且在添加PDB/离子霉素之前添加环己酰亚胺并没有消除PDB/离子霉素诱导的TFR mRNA积累。此外,单独使用PDB或离子霉素均可诱导TFR mRNA的表达,但不能诱导IL-2 mRNA的表达。这些结果表明,与植物血凝素相比,PDB/离子霉素的组合加速了T细胞中IL-2和TFR基因的表达,并触发了一条独立于IL-2的TFR mRNA诱导途径。

相似文献

1
Comparison of phorbol ester/calcium ionophore and phytohemagglutinin-induced signaling in human T lymphocytes. Demonstration of interleukin 2-independent transferrin receptor gene expression.佛波酯/钙离子载体与植物血凝素诱导的人T淋巴细胞信号传导的比较。白细胞介素2非依赖性转铁蛋白受体基因表达的证明。
J Immunol. 1988 Jan 1;140(1):37-43.
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J Immunol. 1987 Sep 1;139(5):1393-9.
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The role of the accessory cell in mitogen-stimulated human T cell gene expression.辅助细胞在有丝分裂原刺激的人T细胞基因表达中的作用。
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Distinct signals are required for proliferation and lymphokine gene expression in murine T cell clones.在小鼠T细胞克隆中,增殖和淋巴因子基因表达需要不同的信号。
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Induction of competence and progression signals in human T lymphocytes by phorbol esters and calcium ionophores.佛波酯和钙离子载体对人T淋巴细胞中感受态和增殖信号的诱导作用。
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Transcriptional regulation of transferrin receptor expression by cultured lymphoblastoid T cells treated with phorbol diesters.佛波酯处理的培养淋巴母细胞样T细胞对转铁蛋白受体表达的转录调控
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Regulation of interleukin 2 and interleukin 2 receptor gene expression in human T cells: I. Effect of Ca2+-ionophore on phorbol myristate acetate co-stimulated cells.人T细胞中白细胞介素2及白细胞介素2受体基因表达的调控:I. 钙离子载体对佛波酯共刺激细胞的影响
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Signals involved in T cell activation. II. Distinct roles of intact accessory cells, phorbol esters, and interleukin 1 in activation and cell cycle progression of resting T lymphocytes.T细胞活化相关信号。II. 完整辅助细胞、佛波酯和白细胞介素1在静息T淋巴细胞活化及细胞周期进程中的不同作用。
J Immunol. 1986 May 15;136(10):3588-96.

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