Lécine P, Algarté M, Rameil P, Beadling C, Bucher P, Nabholz M, Imbert J
INSERM U119, Marseille, France.
Mol Cell Biol. 1996 Dec;16(12):6829-40. doi: 10.1128/MCB.16.12.6829.
The interleukin 2 receptor alpha-chain (IL-2R alpha) gene is a key regulator of lymphocyte proliferation. IL-2R alpha is rapidly and potently induced in T cells in response to mitogenic stimuli. Interleukin 2 (IL-2) stimulates IL-2R alpha. transcription, thereby amplifying expression of its own high-affinity receptor. IL-2R alpha transcription is at least in part controlled by two positive regulatory regions, PRRI and PRRII. PRRI is an inducible proximal enhancer, located between nucleotides -276 and -244, which contains NF-kappaB and SRE/CArG motifs. PRRII is a T-cell-specific enhancer, located between nucleotides -137 and -64, which binds the T-cell-specific Ets protein Elf-1 and HMG-I(Y) proteins. However, none of these proximal regions account for the induction of IL-2R alpha transcription by IL-2. To find new regulatory regions of the IL-2R alpha gene, 8.5 kb of the 5' end noncoding sequence of the IL-2R alpha gene have been sequenced. We identified an 86-nucleotide fragment that is 90% identical to the recently characterized murine IL-2-responsive element (mIL-2rE). This putative human IL-2rE, designated PRRIII, confers IL-2 responsiveness on a heterologous promoter. PRRIII contains a Stat protein binding site that overlaps with an EBS motif (GASd/EBSd). These are essential for IL-2 inducibility of PRRIII/CAT reporter constructs. IL-2 induced the binding of Stat5a and b proteins to the human GASd element. To confirm the physiological relevance of these findings, we carried out in vivo footprinting experiments which showed that stimulation of IL-2R alpha expression correlated with occupancy of the GASd element. Our data demonstrate a major role of the GASd/EBSd element in IL-2R alpha regulation and suggest that the T-cell-specific Elf-1 factor can serve as a transcriptional repressor.
白细胞介素2受体α链(IL-2Rα)基因是淋巴细胞增殖的关键调节因子。IL-2Rα在有丝分裂原刺激下可在T细胞中迅速且强烈地被诱导。白细胞介素2(IL-2)刺激IL-2Rα转录,从而放大其自身高亲和力受体的表达。IL-2Rα转录至少部分受两个正调控区域PRRI和PRRII的控制。PRRI是一个可诱导的近端增强子,位于核苷酸-276至-244之间,包含NF-κB和SRE/CArG基序。PRRII是一个T细胞特异性增强子,位于核苷酸-137至-64之间,可结合T细胞特异性Ets蛋白Elf-1和HMG-I(Y)蛋白。然而,这些近端区域均不能解释IL-2对IL-2Rα转录的诱导作用。为了寻找IL-2Rα基因的新调控区域,我们对IL-2Rα基因5'端非编码序列的8.5 kb进行了测序。我们鉴定出一个86个核苷酸的片段,它与最近鉴定的小鼠IL-2反应元件(mIL-2rE)有90%的同源性。这个假定的人类IL-2rE,命名为PRRIII,可赋予异源启动子IL-2反应性。PRRIII包含一个与EBS基序(GASd/EBSd)重叠的Stat蛋白结合位点。这些对于PRRIII/CAT报告基因构建体的IL-2诱导性至关重要。IL-2诱导Stat5a和b蛋白与人GASd元件结合。为了证实这些发现的生理相关性,我们进行了体内足迹实验,结果表明IL-2Rα表达的刺激与GASd元件的占据相关。我们的数据证明了GASd/EBSd元件在IL-2Rα调控中的主要作用,并表明T细胞特异性Elf-1因子可作为转录抑制因子。