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NF-κB 信号和 IL-4 信号通过 Th2 分化过程中的替代启动子使用调节 SATB1 的表达。

NF-κB Signaling and IL-4 Signaling Regulate SATB1 Expression via Alternative Promoter Usage During Th2 Differentiation.

机构信息

Center of Excellence in Epigenetics, Indian Institute of Science Education and Research, Pune, India.

Symbiosis School of Biological Sciences, Pune, India.

出版信息

Front Immunol. 2019 Apr 2;10:667. doi: 10.3389/fimmu.2019.00667. eCollection 2019.

DOI:10.3389/fimmu.2019.00667
PMID:31001272
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC6454056/
Abstract

SATB1 is a genome organizer protein that is expressed in a lineage specific manner in CD4 T-cells. SATB1 plays a crucial role in expression of multiple genes throughout the thymic development and peripheral differentiation of T cells. Although SATB1 function has been subjected to intense investigation, regulation of gene expression remains poorly understood. Analysis of RNA-seq data revealed multiple transcription start sites at the upstream regulatory region of . We further demonstrated that gene is expressed via alternative promoters during T-helper (Th) cell differentiation. The proximal promoter "P1" is used more by the naïve and activated CD4 T-cells whereas the middle "P2" and the distal "P3" promoters are used at a significantly higher level by polarized T-helper cells. Cytokine and TCR signaling play crucial roles toward alternative promoter usage. Under Th2 polarization conditions, transcription factor STAT6, which operates downstream of the cytokine signaling binds to the P2 and P3 promoters. Genetic perturbation by knockout and chemical inhibition of STAT6 activation resulted in the loss of P2 and P3 promoter activity. Moreover, chemical inhibition of activation of NF-B, a transcription factor that operates downstream of the TCR signaling, also resulted in reduced P2 and P3 promoter usage. Furthermore, usage of the P1 promoter correlated with lower SATB1 protein expression whereas P2 and P3 promoter usage correlated with higher SATB1 protein expression. Thus, the promoter switch might play a crucial role in fine-tuning of SATB1 protein expression in a cell type specific manner.

摘要

SATB1 是一种基因组组织蛋白,在 CD4 T 细胞中以谱系特异性方式表达。SATB1 在胸腺发育和 T 细胞外周分化过程中多个基因的表达中发挥着关键作用。尽管 SATB1 的功能已经受到了深入的研究,但基因表达的调控仍知之甚少。RNA-seq 数据分析揭示了 基因上游调控区存在多个转录起始位点。我们进一步证明,在 T 辅助(Th)细胞分化过程中,通过替代启动子表达 基因。近端启动子“P1”在幼稚和激活的 CD4 T 细胞中使用更多,而中间“P2”和远端“P3”启动子在极化的 Th 细胞中使用水平显著更高。细胞因子和 TCR 信号对替代启动子的使用起着至关重要的作用。在 Th2 极化条件下,作为细胞因子信号下游的转录因子 STAT6 结合到 P2 和 P3 启动子上。通过 knockout 和化学抑制 STAT6 激活进行遗传干扰导致 P2 和 P3 启动子活性丧失。此外,化学抑制 TCR 信号下游的转录因子 NF-B 的激活也导致 P2 和 P3 启动子使用减少。此外,P1 启动子的使用与 SATB1 蛋白表达水平降低相关,而 P2 和 P3 启动子的使用与 SATB1 蛋白表达水平升高相关。因此,启动子切换可能在以细胞类型特异性方式精细调节 SATB1 蛋白表达中发挥关键作用。

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