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人糖原合酶激酶-3α启动子的分子克隆与表达分析

Molecular cloning and expression analysis of human glycogen synthase kinase-3 alpha promoter.

作者信息

Lee K F, Chan J Y, Lau K F, Lee W C, Miller C C, Anderton B H, Shaw P C

机构信息

Department of Biochemistry, The Chinese University of Hong Kong, Shatin, N.T., Hong Kong, China.

出版信息

Brain Res Mol Brain Res. 2000 Dec 8;84(1-2):150-7. doi: 10.1016/s0169-328x(00)00238-2.

DOI:10.1016/s0169-328x(00)00238-2
PMID:11113543
Abstract

Human glycogen synthase kinase-3 alpha (GSK-3 alpha) is a serine/threonine kinase that phosphorylates a variety of cytoplasmic and nuclear proteins. It also phosphorylates components of the neuronal cytoskeleton including tau and neurofilament heavy chain. Hyperphosphorylated tau is found in neurofibrillary tangles, a hallmark of Alzheimer's disease and aberrant phosphorylation of neurofilament heavy chain is observed in motor neuron disease. Alterations in GSK-3 alpha activity may therefore contribute to the disease process in these disorders. As a first step to understand the transcriptional regulation of GSK-3 alpha, a 2-kb (p-1751/+243) DNA fragment upstream of the GSK-3 alpha initiation codon was obtained from a YAC clone and characterised. Using primer extension assays, a putative transcriptional start site was located to a G nucleotide 244 bp upstream of the ATG codon. Several transcription factor-binding sites were identified on the promoter region, but no TATA-like element was located close to the start site. Deletion mutants of the 2-kb DNA fragment were generated and fused to a promoterless chloramphenicol acetyltransferase (CAT) gene. Transfection study in a neuroblastoma cell line revealed the 1-kb (p-719/+243) fragment carried strong promoter activity, while the 2-kb construct that contains an Alu-like sequence was only 50% active.

摘要

人糖原合酶激酶-3α(GSK-3α)是一种丝氨酸/苏氨酸激酶,可磷酸化多种细胞质和核蛋白。它还能磷酸化神经元细胞骨架的成分,包括tau蛋白和神经丝重链。在神经原纤维缠结中发现了过度磷酸化的tau蛋白,这是阿尔茨海默病的一个标志,并且在运动神经元疾病中观察到神经丝重链的异常磷酸化。因此,GSK-3α活性的改变可能在这些疾病的发病过程中起作用。作为了解GSK-3α转录调控的第一步,从一个酵母人工染色体(YAC)克隆中获得了GSK-3α起始密码子上游2 kb(p-1751/+243)的DNA片段并进行了表征。使用引物延伸分析,确定了一个推定的转录起始位点位于ATG密码子上游244 bp处的一个G核苷酸。在启动子区域鉴定出了几个转录因子结合位点,但在起始位点附近未发现类似TATA的元件。构建了2 kb DNA片段的缺失突变体,并将其与无启动子的氯霉素乙酰转移酶(CAT)基因融合。在神经母细胞瘤细胞系中的转染研究表明,1 kb(p-719/+243)片段具有很强的启动子活性,而包含类Alu序列的2 kb构建体的活性仅为50%。

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