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Cloning and tissue-specific functional characterization of the promoter of the rat diazepam binding inhibitor, a peptide with multiple biological actions.

机译:大鼠地西epa结合抑制剂(具有多种生物学作用的肽)启动子的克隆和组织特异性功能表征。

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摘要

Diazepam binding inhibitor (DBI) is a 10-kDa polypeptide that regulates mitochondrial steroidogenesis, glucose-induced insulin secretion, metabolism of acyl-CoA esters, and the action of gamma-aminobutyrate on GABAA receptors. To investigate the regulation of DBI gene expression, three positive clones were isolated from a rat genomic library. One of them contained a DBI genomic DNA fragment encompassing 4 kb of the 5' untranslated region, the first two exons, and part of the second intron of the DBI gene. Two other overlapping clones contained a processed DBI pseudogene. Several transcription initiation sites were detected by RNase protection and primer extension assays. Different tissues exhibited clear differences in the efficiencies of transcription startpoint usage. Transient expression experiments using DNA fragments of different length from the 5' untranslated region of the DBI gene showed that basal promoter activity required 146 bp of the proximal DBI sequence, whereas full activation was achieved with 423 bp of the 5' untranslated region. DNase I protection experiments with liver nuclear proteins demonstrated three protected regions at nt -387 to -333, -295 to -271, and -176 to -139 relative to the ATG initiation codon; in other tissues the pattern of protection was different. In gel shift assays the most proximal region (-176 to -139) was found to bind several general transcription factors as well as cell type-restricted nuclear proteins which may be related to specific regulatory patterns in different tissues. Thus, the DBI gene possesses some features of a housekeeping gene but also includes a variable regulation which appears to change with the function that it subserves in different cell types.
机译:地西p结合抑制剂(DBI)是一种10 kDa的多肽,可调节线粒体的类固醇生成,葡萄糖诱导的胰岛素分泌,酰基辅酶A酯的代谢以及γ-氨基丁酸酯对GABAA受体的作用。为了研究DBI基因表达的调控,从大鼠基因组文库中分离了三个阳性克隆。其中一个包含一个DBI基因组DNA片段,该片段包含4 kb的5'非翻译区,前两个外显子和DBI基因第二个内含子的一部分。其他两个重叠克隆包含一个经过处理的DBI假基因。通过RNA酶保护和引物延伸测定法检测到几个转录起始位点。不同的组织在转录起点使用效率上表现出明显的差异。使用与DBI基因5'非翻译区长度不同的DNA片段进行的瞬时表达实验表明,基础启动子活性需要近端DBI序列的146 bp,而5'非翻译区的423 bp则可以完全激活。用肝核蛋白进行的DNase I保护实验表明,相对于ATG起始密码子,在nt -387至-333,-295至-271和-176至-139处有三个保护区。在其他组织中,保护方式不同。在凝胶迁移分析中,发现最接近的区域(-176至-139)结合了几种通用转录因子以及细胞类型受限的核蛋白,这些蛋白可能与不同组织中的特定调控模式有关。因此,DBI基因具有管家基因的某些特征,但也包括可变调节,该调节似乎随其在不同细胞类型中所具有的功能而改变。

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