首页> 外文期刊>Archives of Biochemistry and Biophysics >Promoter analysis and transcriptional regulation of human carbonic anhydrase VIII gene in a MERRF disease cell model
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Promoter analysis and transcriptional regulation of human carbonic anhydrase VIII gene in a MERRF disease cell model

机译:Merrf疾病细胞模型中人碳酸酐酶VIII基因的启动子分析及转录调控

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Myoclonic epilepsy with ragged-red fibers (MERRF) is a maternally inherited mitochondria] neuromuscular disease. We previously reported a significant decrease of mRNA and protein levels of nuclear DNA-encoded carbonic anhydrase VIII (CA8) in MERRF cybrids harboring A8344G mutation in mitochondrial DNA (mtDNA). In this study, we established a reporter construct of luciferase gene-carrying hCA8 promoter containing several putative transcription factor-binding sites, including GC-box, AP-2 and TATA-binding element in the 5'flanldng region of the hCA8 gene. Using a series of mutated hCA8 promoter constructs, we demonstrated that a proximal GC-box, recognized by Spl and other Sp family members, may be a key cis-element functioning at the promoter. Additionally, a significant increase of the hCA8 promoter activity was observed in the wild-type and mutant cybrids with over-expression of eGFP-Spl, but no detectable increase in the CA8 protein expression. In contrast, over-expression of Flag-Spl and Flag-Sp4 significantly increased the hCA8 promoter activity as well as endogenous CA8 protein expression in neuron like HEK-293 T cells. However, down-regulation of Spl, but not Sp4, in 293 T cells revealed a significant reduction of CA8 expression, suggesting that Sp1 is a predominant transcription factor for regulation of CA8 activity. Furthermore, our data indicate that chromatin structure may be involved in the expression of hCA8 gene in MERRF cybrids. Taken together, these results suggest that Spl transactivates hCA8 gene through the proximal GC box element in the promoter region. The key modulator-responsive factor to the mtDNA mutation and how it may affect nuclear hCA8 gene transcription need further investigations.
机译:肌阵挛性癫痫与衣衫红纤维(MERRF)是一种母体遗传性的线粒体。神经肌肉疾病。我们之前据报道,Merrf糖蛋白酶VIII(CA8)的mRNA和蛋白质水平的显着降低,含有线粒体DNA(MTDNA)中的A8344G突变。在该研究中,我们建立了含有几种推定转录因子结合位点的荧光素酶基因携带HCA8启动子的报告构建体,包括HCA8基因的5'FlaNDngng区域中的GC盒,AP-2和TATA结合元件。使用一系列突变的HCA8启动子构建体,我们证明了由SPL和其他SP系列成员识别的近端GC盒,可以是在启动子上运行的关键顺式元素。另外,在野生型和突变体胞胎中观察到HCA8启动子活性的显着增加,具有eGFP-SPL的过表达,但没有可检测的CA8蛋白表达增加。相反,FLAG-SPL和FLAG-SP4的过表达显着增加了HCA8启动子活性以及神经元中的内源CA8蛋白表达,如HEK-293 T细胞。然而,在293T细胞中,SPL的下调但不是SP4,显示CA8表达的显着降低,表明SP1是用于调节CA8活性的主要转录因子。此外,我们的数据表明染色质结构可以参与Merrf胞胎中HCA8基因的表达。总之,这些结果表明,SPL通过启动子区域中的近端GC盒元件转移HCA8基因。对MTDNA突变的关键调节剂响应因子及其如何影响核HCA8基因转录需要进一步调查。

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