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Structural and functional characterization of mouse glutamate decarboxylase 67 gene promoter

机译:小鼠谷氨酸脱羧酶67基因启动子的结构和功能表征

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Neuronal expression of the mouse glutamate decarboxylase 67 (mGAD67) gene occurs exclusively in neurons that synthesize and release GABA (GABAergic neurons). This gene is also expressed in pancreatic islet cells and testicular spermatocytes. In order to elucindate the molecular mechanisms underlying the regulation of mGAD67 gene expression, we isolated and characterized the 5'-flanking region of this gene. Sequence analysis of a 10.2-kb DNA fragment of this gene containing a promoter region (8.4 kb) and noncoding exons 0A and 0B revealed the presence of numerous potential neuron-specific cis-regulatory elements. Functional analysis of the 5'-flaking region of exons 0A and 0B by transient transfection into cultured cells revealed that the region -98 to -52 close to exon 0A is important for the transcriptional activity of both exons 0A and 0B. In addition, we used transgenic mice to examine the expression pattern conferred by the 10.2 kb DNA fragment of the mGAD67 gene fused to the bacterial lacZ reporter gene. Transgene expression was observed in neurons of particular brain regions containing abundant GABAergic neurons such as the basal ganglia, in pancreatic islet cells and in testicular spermatocytes and spermatogonia. These results suggest that the 10.2 kb DNA fragment of the mGAD67 gene contains regulatory elements essential for its targeted expression in GABAergic neurons, islet cells and spermatocytes.
机译:小鼠谷氨酸脱羧酶67(mGAD67)基因的神经元表达仅发生在合成和释放GABA(GABA能神经元)的神经元中。该基因还在胰岛细胞和睾丸精母细胞中表达。为了阐明调控mGAD67基因表达的分子机制,我们分离并表征了该基因的5'侧翼区域。对该基因的10.2kb DNA片段的序列分析,其含有启动子区(8.4kb)和非编码外显子0A和0B,表明存在许多潜在的神经元特异性顺式调控元件。通过瞬时转染到培养的细胞中对外显子0A和0B的5'剥落区域进行功能分析,发现靠近外显子0A的-98至-52区域对于外显子0A和0B的转录活性都很重要。此外,我们使用转基因小鼠检查了与细菌lacZ报告基因融合的mGAD67基因的10.2 kb DNA片段所赋予的表达模式。在含有丰富的GABA能神经元的特定大脑区域的神经元(如基底神经节),胰岛细胞,睾丸精细胞和精原细胞中观察到转基因表达。这些结果表明,mGAD67基因的10.2 kb DNA片段包含其在GABA能神经元,胰岛细胞和精母细胞中靶向表达所必需的调控元件。

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