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Characterization of the human sialidase Neu4 gene promoter

机译:人唾液酸酶Neu4基因启动子的表征

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There are 4 different sialidases that have been described in humans: lysosomal (Neu1), cytoplasmic (Neu2), plasma membrane (Neu3), and lysosomal/mitochondrial (Neu4). Previously, we have shown that Neu4 has a broad substrate specificity and is active against glyco-conjugates, including G_(M2) ganglioside, at the acidic pH of 3.2. An overexpression of Neu4 in transfected neuroglia cells from a Tay–Sachs patient shows a clearance of accumulated G_(M2), indicating the biological importance of Neu4. In this paper, we aimed to characterize a minimal promoter region of the human Neu4 gene in order to understand the molecular mechanism regulating its expression. We cloned 7 different DNA fragments from the human Neu4 promoter region into luciferase expression vectors for a reporter assay and also performed an electrophoretic mobility shift assay to demonstrate the binding of transcription factors. We demonstrated that –187 bp upstream of the Neu4 gene is a minimal promoter region for controlling transcription from the human Neu4 gene. The electrophoretic mobility shift assay showed that the minimal promoter region recruits a c-myc transcription factor, which might be responsible for regulation of Neu4 gene transcription. The data we obtained might be useful to discover small molecules, which control selective high expression of the human Neu4 gene, resulting in the normal morphological phenotype in the lysosomes of Tay–Sachs patients.
机译:在人类中已描述了4种不同的唾液酸酶:溶酶体(Neu1),细胞质(Neu2),质膜(Neu3)和溶酶体/线粒体(Neu4)。以前,我们已经显示Neu4具有广泛的底物特异性,并且在3.2的酸性pH下对包括G_(M2)神经节苷脂在内的糖结合物具有活性。来自Tay-Sachs患者的转染神经胶质细胞中Neu4的过表达显示清除了累积的G_(M2),表明Neu4的生物学重要性。在本文中,我们旨在表征人类Neu4基因的最小启动子区域,以了解调节其表达的分子机制。我们从人Neu4启动子区域克隆了7种不同的DNA片段到萤光素酶表达载体中进行了报告基因分析,并且还进行了电泳迁移率迁移分析以证明转录因子的结合。我们证明,Neu4基因上游的–187 bp是控制人类Neu4基因转录的最小启动子区域。电泳迁移率变动分析表明,最小启动子区域募集了c-myc转录因子,这可能是Neu4基因转录调控的原因。我们获得的数据可能有助于发现控制人类Neu4基因选择性高表达的小分子,从而在Tay-Sachs患者的溶酶体中产生正常的形态表型。

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