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挖掘微阵列数据以识别在未活化的静息T淋巴细胞而非活化T淋巴细胞中表达的转录因子。

Mining microarray data to identify transcription factors expressed in naïve resting but not activated T lymphocytes.

作者信息

Argyropoulos C, Nikiforidis G C, Theodoropoulou M, Adamopoulos P, Boubali S, Georgakopoulos T N, Paliogianni F, Papavassiliou A G, Mouzaki A

机构信息

Laboratory of Hematology and Transfusion Medicine, University of Patras, Patras, Greece.

出版信息

Genes Immun. 2004 Jan;5(1):16-25. doi: 10.1038/sj.gene.6364034.

DOI:10.1038/sj.gene.6364034
PMID:14735145
Abstract

Transcriptional repressors controlling the expression of cytokine genes have been implicated in a variety of physiological and pathological phenomena. An unknown repressor that binds to the distal NFAT element of the interleukin-2 (IL-2) gene promoter in naive T-helper lymphocytes has been implicated in autoimmune phenomena and has emerged as a potentially important factor controlling the latency of HIV-1. The aim of this paper was the identification of this repressor. We resorted to public microarray databases looking for DNA-binding proteins that are present in naïve resting T cells but are downregulated when the cells are activated. A Bayesian data mining statistical analysis uncovered 25 candidate factors. Of the 25, NFAT4 and the oncogene ets-2 bind to the common motif AAGGAG found in the HIV-1 LTR and IL-2 probes. Ets-2 binding site contains the three G's that have been shown to be important for binding of the unknown factor; hence, we considered it the likeliest candidate. Electrophoretic mobility shift assays confirmed cross-reactivity between the unknown repressor and anti-ets-2 antibodies, and cotransfection experiments demonstrated the direct involvement of Ets-2 in silencing the IL-2 promoter. Designing experiments for transcription factor analysis using microarrays and Bayesian statistical methodologies provides a novel way toward elucidation of gene control networks.

摘要

控制细胞因子基因表达的转录抑制因子与多种生理和病理现象有关。一种未知的抑制因子可与初始辅助性T淋巴细胞中白细胞介素-2(IL-2)基因启动子的远端核因子活化T细胞(NFAT)元件结合,与自身免疫现象有关,并且已成为控制HIV-1潜伏期的一个潜在重要因素。本文的目的是鉴定这种抑制因子。我们借助公共微阵列数据库寻找在初始静止T细胞中存在但在细胞被激活时表达下调的DNA结合蛋白。贝叶斯数据挖掘统计分析揭示了25个候选因子。在这25个因子中,NFAT4和癌基因ets-2与在HIV-1长末端重复序列(LTR)和IL-2探针中发现的共同基序AAGGAG结合。Ets-2结合位点包含已被证明对未知因子结合很重要的三个G;因此,我们认为它是最有可能的候选因子。电泳迁移率变动分析证实了未知抑制因子与抗ets-2抗体之间的交叉反应性,共转染实验证明了Ets-2直接参与沉默IL-2启动子。利用微阵列和贝叶斯统计方法设计转录因子分析实验为阐明基因控制网络提供了一种新方法。

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