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新型DNA结合蛋白参与人类神经丝蛋白H基因表达的调控。

Novel DNA binding proteins participate in the regulation of human neurofilament H gene expression.

作者信息

Elder G A, Liang Z, Lee N, Friedrich V L, Lazzarini R A

机构信息

Brookdale Center for Molecular Biology, Mount Sinai School of Medicine, New York, NY 10029.

出版信息

Brain Res Mol Brain Res. 1992 Sep;15(1-2):85-98. doi: 10.1016/0169-328x(92)90155-5.

Abstract

By a combination of DNase I footprinting, methylation interference, and gel shift analyses we have identified multiple binding sites for nuclear proteins within the promoter region of the human neurofilament H gene. Two sites likely bind the transcription factor Sp1 while two others may be targets for previously unrecognized DNA binding proteins. One site, PAL, occurs within the 10 bp sequence GGGGAGGAGG. Two copies of the PAL sequence form an interrupted palindrome around one of the Sp1 sites. A second site, PROX, is found within the sequence GGTTGGACC. Nuclear extracts prepared from both neural and non-neural cell lines, mouse brain, and mouse liver contain proteins that recognize and bind to the PROX and PAL sequences indicating that proteins which bind to these target sequences are widespread. The appearance of these target sequences in the 5' upstream region of several neuron specific genes suggests that they play key roles in the transcription of neuron specific genes. The functional activity of these target DNA sequences was demonstrated by transfection assays using a reporter gene fused to nested deletions of the NF(H) promoter region. Interestingly, these assays revealed that maximal transient expression was obtained with DNA fusion genes containing the PAL, PROX and TATA sequences. Inclusion of the Sp1 sites into the fusion genes failed to enhance the expression of the reporter gene. To determine if the NF(H) promoter can be activated in a tissue specific manner during development transgenic mice containing the promoter region linked to a beta-galactosidase reporter gene were generated. In one line sporadic expression of the transgene occurred in the CNS and testis while in four other lines no expression occurred. Collectively these results suggest that the NF(H) gene promoter is active in a tissue specific manner only by interactions with regulatory elements that lie further upstream or downstream of the start site of initiation.

摘要

通过DNA酶I足迹法、甲基化干扰法和凝胶迁移分析相结合的方法,我们在人神经丝H基因启动子区域内鉴定出了多个核蛋白结合位点。两个位点可能结合转录因子Sp1,而另外两个位点可能是以前未识别的DNA结合蛋白的作用靶点。一个位点,PAL,位于10bp序列GGGGAGGAGG内。PAL序列的两个拷贝围绕其中一个Sp1位点形成一个间断的回文结构。另一个位点,PROX,位于序列GGTTGGACC内。从神经和非神经细胞系、小鼠脑和小鼠肝脏制备的核提取物中都含有能识别并结合PROX和PAL序列的蛋白质,这表明与这些靶序列结合的蛋白质广泛存在。这些靶序列出现在几个神经元特异性基因的5'上游区域,表明它们在神经元特异性基因的转录中起关键作用。使用与NF(H)启动子区域嵌套缺失片段融合的报告基因进行转染实验,证明了这些靶DNA序列的功能活性。有趣的是,这些实验表明,含有PAL、PROX和TATA序列的DNA融合基因能获得最大的瞬时表达。将Sp1位点纳入融合基因未能增强报告基因的表达。为了确定NF(H)启动子在发育过程中是否能以组织特异性方式被激活,我们构建了含有与β-半乳糖苷酶报告基因相连的启动子区域的转基因小鼠。在一个品系中,转基因在中枢神经系统和睾丸中呈散在表达,而在其他四个品系中没有表达。这些结果共同表明,NF(H)基因启动子仅通过与起始位点上游或下游更远的调控元件相互作用,以组织特异性方式发挥活性。

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