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通过细胞内掺入对活化蛋白-1转录复合物具有特异性的多克隆抗体来抑制CD28/CD3介导的天然和记忆性人T淋巴细胞的共刺激。

Inhibition of CD28/CD3-mediated costimulation of naive and memory human T lymphocytes by intracellular incorporation of polyclonal antibodies specific for the activator protein-1 transcriptional complex.

作者信息

Woodside D G, McIntyre B W

机构信息

Department of Immunology, University of Texas M. D. Anderson Cancer Center, Houston 77030, USA.

出版信息

J Immunol. 1998 Jul 15;161(2):649-58.

PMID:9670939
Abstract

A number of indirect methods have been utilized in demonstrating activator protein-1 transcription factor function in IL-2 promoter activity. However, there has been no direct demonstration that activator protein-1 is involved in CD28-dependent costimulation of IL-2 gene transcription in freshly isolated naive and memory human T lymphocytes. To address this issue, the method of scrape loading was applied to purified peripheral blood T lymphocytes. Since scrape loading relies on adherent cells, peripheral blood human T (PB-T) cells were immobilized on the nonspecific cell attachment factor poly-L-lysine. Cells scraped off poly-L-lysine in the presence of Ig FITC efficiently incorporated Ig, with relatively uniform fluorescence. T cells retained their physical parameters as measured by forward and side light scatter, and functional activity as measured by costimulation of proliferation and IL-2 production after being scraped off this substrate. CD28/CD3-costimulated T cells produced intracellular IL-2 from all subsets measured (CD4+, CD4-, CD45RO+, and CD45RO-). IL-2 production and intracellular accumulation in nonscraped PB-T cells activated with CD28/CD3 coligation were skewed favoring CD45RO+ and CD4+ subsets, as was IL-2 production in scraped PB-T cells. The intracellular incorporation of Abs specific for c-Fos and c-Jun family members by scrape loading inhibited the production and intracellular accumulation of IL-2 within 6 h of costimulation with PMA/ionomycin, or costimulation by CD28 and CD3 ligation. Scrape loading thus provides an efficient mechanism for intracellular incorporation of macromolecules, and the first direct evidence that c-Fos and c-Jun are involved in transcription of the IL-2 gene within its correct chromosomal context, in resting human T lymphocyte subpopulations.

摘要

已经使用了多种间接方法来证明激活蛋白-1转录因子在白细胞介素-2启动子活性中的功能。然而,尚无直接证据表明激活蛋白-1参与新鲜分离的天然和记忆性人T淋巴细胞中白细胞介素-2基因转录的CD28依赖性共刺激。为了解决这个问题,将刮擦加载方法应用于纯化的外周血T淋巴细胞。由于刮擦加载依赖于贴壁细胞,因此外周血人T(PB-T)细胞固定在非特异性细胞附着因子聚-L-赖氨酸上。在Ig FITC存在下从聚-L-赖氨酸上刮下的细胞有效地掺入了Ig,荧光相对均匀。T细胞在从该底物上刮下后,通过前向和侧向光散射测量保留了其物理参数,并通过增殖共刺激和白细胞介素-2产生测量保留了功能活性。CD28/CD3共刺激的T细胞从所有测量的亚群(CD4+、CD4-、CD45RO+和CD45RO-)产生细胞内白细胞介素-2。用CD28/CD3共连接激活的未刮擦PB-T细胞中的白细胞介素-2产生和细胞内积累偏向于CD45RO+和CD4+亚群,刮擦PB-T细胞中的白细胞介素-2产生也是如此。通过刮擦加载细胞内掺入针对c-Fos和c-Jun家族成员的抗体,在与佛波酯/离子霉素共刺激或CD28和CD3连接共刺激的6小时内抑制了白细胞介素-2的产生和细胞内积累。因此,刮擦加载为大分子的细胞内掺入提供了一种有效机制,并且首次直接证明c-Fos和c-Jun在静息人T淋巴细胞亚群中白细胞介素-2基因在其正确染色体背景下的转录中起作用。

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