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胶质纤维酸性蛋白(GFAP)基因的结构与转录调控

Structure and transcriptional regulation of the GFAP gene.

作者信息

Brenner M

机构信息

Stroke Branch, National Institute of Neurological Disorders and Stroke, National Institutes of Health, Bethesda, MD 20892.

出版信息

Brain Pathol. 1994 Jul;4(3):245-57. doi: 10.1111/j.1750-3639.1994.tb00840.x.

Abstract

Transcriptional regulation of the GFAP gene is intimately connected with astrocyte function: its initial activation marks the differentiation of astrocytes, and its up-regulation accompanies the reactive response to CNS injury. Studies of GFAP transcription should thus provide insights into multiple regulatory pathways operating in these cells. In addition, they should identify DNA elements that could be used to direct synthesis of other proteins to astrocytes in transgenic animals, permitting creation of disease models, and the testing of cause and effect relationships. This review describes several GFAP cDNA and genomic clones that have been isolated, including homology comparisons of the encoded RNAs and proteins. Cell transfection studies by several laboratories are summarized that have identified a DNA segment immediately upstream of the RNA start site that is essential for transcriptional activity, but which have yielded conflicting results concerning the importance of other segments located both further upstream and downstream of the RNA start site. Two procedures are recounted that have led to the successful expression of GFAP-transgenes in astrocytes in mice. One of these incorporates the transgene into the first exon of a fragment spanning the entire GFAP gene, while the other links it to a 2 kb 5'-flanking segment. Results already produced by GFAP-transgenic studies include demonstration of a neurotoxic effect of the HIV-1 gp120 coat protein, and creation of a hydrocephalic mouse model.

摘要

胶质纤维酸性蛋白(GFAP)基因的转录调控与星形胶质细胞的功能密切相关:其最初的激活标志着星形胶质细胞的分化,而其上调则伴随着对中枢神经系统损伤的反应。因此,对GFAP转录的研究应能深入了解这些细胞中多种调控途径。此外,研究还应鉴定出可用于在转基因动物中将其他蛋白质的合成导向星形胶质细胞的DNA元件,从而建立疾病模型并测试因果关系。本综述描述了已分离出的几种GFAP cDNA和基因组克隆,包括对所编码的RNA和蛋白质的同源性比较。总结了几个实验室的细胞转染研究,这些研究确定了RNA起始位点上游紧邻的一个DNA片段对转录活性至关重要,但对于位于RNA起始位点上游和下游更远位置的其他片段的重要性,研究结果存在矛盾。讲述了两种在小鼠星形胶质细胞中成功表达GFAP转基因的方法。其中一种方法是将转基因整合到跨越整个GFAP基因的一个片段的第一个外显子中,另一种方法是将其与一个2 kb的5'侧翼片段相连。GFAP转基因研究已经产生的结果包括证明了HIV-1 gp120包膜蛋白的神经毒性作用,以及建立了一个脑积水小鼠模型。

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