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Two adjacent E box elements and a M-CAT box are involved in the muscle-specific regulation of the rat acetylcholine receptor β subunit gene

机译:两个相邻的E盒元件和一个m-CaT盒参与大鼠乙酰胆碱受体β亚基基因的肌肉特异性调节

摘要

We have isolated and analysed the 5' flanking region of the rat acetylcholine receptor (AChR) beta subunit gene and determined regulatory elements that confer muscle specificity. Deletion mapping revealed a minimal TATA-box-less promoter region containing an initiator motif. An 85-bp fragment has been shown to promote high muscle-specific expression of a chloramphenicol acetyltransferase (CAT) reporter construct upon transfection in primary muscle cells. This sequence can be functionally dissected in a basal muscle-specific promoter element carrying a M-CAT box that is flanked at the 5' end by an enhancer element with two binding sites for myogenic factors. Point mutations in the M-CAT box cause the loss of transcriptional activity of the basal promoter fragment. The enhancer activity depends on the presence of both E boxes that cooperate in a synergistic fashion. We therefore conclude that the control of muscle-specific and developmental expression of the rat AChR beta subunit gene requires both regulatory elements, the M-CAT box and two adjacent E boxes, located in close proximity to each other. Cotransfection experiments in NIH3T3 cells demonstrate that the rat AChR beta subunit gene can be transactivated by myogenic factors displaying a preference for myogenin, as well as MRF4 and myf5 compared to a clearly weaker responsiveness to MyoD1.
机译:我们已经分离并分析了大鼠乙酰胆碱受体(AChR)β亚基基因的5'侧翼区域,并确定了赋予肌肉特异性的调控元件。缺失作图揭示了含有启动子基序的最小的TATA-box-less启动子区域。已显示一个85 bp的片段在原代肌肉细胞中转染后能促进氯霉素乙酰转移酶(CAT)报告基因构建体的高肌肉特异性表达。该序列可以在带有M-CAT盒的基底肌特异性启动子元件中进行功能切割,所述M-CAT盒在5'端侧接具有两个生肌因子结合位点的增强子元件。 M-CAT盒中的点突变导致基础启动子片段的转录活性丧失。增强子活性取决于以协同方式协同作用的两个E盒的存在。因此,我们得出结论,对大鼠AChRβ亚基基因的肌肉特异性和发育性表达的控制需要两个调节元件,即M-CAT盒和两个彼此紧邻的E盒。在NIH3T3细胞中进行的共转染实验表明,与对MyoD1的响应性明显较弱相比,大鼠AChRβ亚基基因可以被显示出对肌原蛋白以及MRF4和myf5偏爱的成肌因子反式激活。

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