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核心结合因子与相邻启动子元件之间的协同作用有助于白细胞介素-3的组织特异性表达。

Cooperation between core binding factor and adjacent promoter elements contributes to the tissue-specific expression of interleukin-3.

作者信息

Taylor D S, Laubach J P, Nathan D G, Mathey-Prevot B

机构信息

Divisions of Pediatric Hematology and Oncology, Dana Farber Cancer Institute, Boston, Massachusetts 02115, USA.

出版信息

J Biol Chem. 1996 Jun 14;271(24):14020-7. doi: 10.1074/jbc.271.24.14020.

DOI:10.1074/jbc.271.24.14020
PMID:8662845
Abstract

Tissue-specific expression of interleukin-3 (IL-3) is mediated via cis-acting elements located within 315 base pairs of the transcription start. This is achieved in part through the positive activities of the AP-1 and Elf-1 sites in the IL-3 promoter. The contribution to T cell-specific expression by other promoter sites was assessed in a transient expression assay with IL-3 promoter constructs linked to a luciferase gene, focusing initially on the core binding factor (CBF) site, which is footprinted in vivo upon T cell activation. Activity of the CBF site is shown to be critically dependent on the adjacent activator site Act-1. Together the Act-1 and CBF sites form a functional unit (AC unit) with dual activity. The AC unit is demonstrated to enhance basal activity of promoters both in fibroblasts and T cells. This activity is further inducible in activated T cells, but not in fibroblasts. In addition to the already identified NIP repressor site, evidence is presented for a second repressor region that restricts promoter activity in fibroblasts. Finally, a novel positive regulatory element has been mapped in the IL-3 promoter between nucleotide -180 and -210 that leads to increased expression in T cells. Together these results demonstrate that T cell expression of IL-3 is not specified by the activity of a single tissue-specific element, but instead involves multiple interacting elements that provide both specific positive regulation in T cells and specific negative regulation in fibroblasts.

摘要

白细胞介素-3(IL-3)的组织特异性表达是通过位于转录起始点315个碱基对内的顺式作用元件介导的。这部分是通过IL-3启动子中AP-1和Elf-1位点的正向活性实现的。在与荧光素酶基因相连的IL-3启动子构建体的瞬时表达测定中,评估了其他启动子位点对T细胞特异性表达的贡献,最初重点关注核心结合因子(CBF)位点,该位点在T细胞活化时在体内被足迹化。结果表明,CBF位点的活性严重依赖于相邻的激活位点Act-1。Act-1和CBF位点共同形成了一个具有双重活性的功能单元(AC单元)。AC单元被证明可增强成纤维细胞和T细胞中启动子的基础活性。这种活性在活化的T细胞中进一步诱导,但在成纤维细胞中不诱导。除了已经确定的NIP抑制位点外,还提供了证据表明存在第二个抑制区域,该区域限制了成纤维细胞中的启动子活性。最后,在IL-3启动子中已定位了一个新的正向调节元件,位于核苷酸-180和-210之间,可导致T细胞中表达增加。这些结果共同表明,IL-3的T细胞表达不是由单个组织特异性元件的活性决定的,而是涉及多个相互作用的元件,这些元件在T细胞中提供特异性正向调节,在成纤维细胞中提供特异性负向调节。

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Cooperation between core binding factor and adjacent promoter elements contributes to the tissue-specific expression of interleukin-3.核心结合因子与相邻启动子元件之间的协同作用有助于白细胞介素-3的组织特异性表达。
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