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Mechanisms Regulating GLUT4 Transcription in Skeletal Muscle Cells Are Highly Conserved across Vertebrates

机译:调节骨骼肌细胞中GLUT4转录的机制在整个脊椎动物中高度保守。

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摘要

The glucose transporter 4 (GLUT4) plays a key role in glucose uptake in insulin target tissues. This transporter has been extensively studied in many species in terms of its function, expression and cellular traffic and complex mechanisms are involved in its regulation at many different levels. However, studies investigating the transcription of the GLUT4 gene and its regulation are scarce. In this study, we have identified the GLUT4 gene in a teleost fish, the Fugu (Takifugu rubripes), and have cloned and characterized a functional promoter of this gene for the first time in a non-mammalian vertebrate. In silico analysis of the Fugu GLUT4 promoter identified potential binding sites for transcription factors such as SP1, C/EBP, MEF2, KLF, SREBP-1c and GC-boxes, as well as a CpG island, but failed to identify a TATA box. In vitro analysis revealed three transcription start sites, with the main residing 307 bp upstream of the ATG codon. Deletion analysis determined that the core promoter was located between nucleotides -132/+94. By transfecting a variety of 5´deletion constructs into L6 muscle cells we have determined that Fugu GLUT4 promoter transcription is regulated by insulin, PG-J2, a PPARγ agonist, and electrical pulse stimulation. Furthermore, our results suggest the implication of motifs such as PPARγ/RXR and HIF-1α in the regulation of Fugu GLUT4 promoter activity by PPARγ and contractile activity, respectively. These data suggest that the characteristics and regulation of the GLUT4 promoter have been remarkably conserved during the evolution from fish to mammals, further evidencing the important role of GLUT4 in metabolic regulation in vertebrates.
机译:葡萄糖转运蛋白4(GLUT4)在胰岛素靶组织中的葡萄糖摄取中起关键作用。已经对该转运蛋白的功能,表达和细胞运输进行了广泛的研究,复杂的机制参与了许多不同水平的调控。但是,缺乏关于GLUT4基因的转录及其调控的研究。在这项研究中,我们已经确定了硬骨鱼类Fugu(Takifugu rubripes)中的GLUT4基因,并首次在非哺乳动物脊椎动物中克隆并表征了该基因的功能启动子。在对Fugu GLUT4启动子进行的计算机分析中,确定了转录因子(例如SP1,C / EBP,MEF2,KLF,SREBP-1c和GC-boxes)以及CpG岛的潜在结合位点,但未能识别TATA盒。体外分析显示三个转录起始位点,主要位于ATG密码子上游307 bp。缺失分析确定核心启动子位于核苷酸-132 / + 94之间。通过将多种5'缺失构建体转染到L6肌肉细胞中,我们已经确定了Fugu GLUT4启动子的转录受胰岛素,PG-J2,PPARγ激动剂和电脉冲刺激的调节。此外,我们的结果表明,例如PPARγ/ RXR和HIF-1α等基序分别通过PPARγ和收缩活性调节Fugu GLUT4启动子活性。这些数据表明,GLUT4启动子的特征和调控在从鱼类到哺乳动物的进化过程中已经得到了显着的保守,进一步证明了GLUT4在脊椎动物代谢调控中的重要作用。

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