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克隆于酵母人工染色体载体上的人神经生长因子 - 荧光素酶报告基因的位置独立表达。

Position-independent expression of a human nerve growth factor-luciferase reporter gene cloned on a yeast artificial chromosome vector.

作者信息

Asselbergs F A, Grossenbacher R, Ortmann R, Hengerer B, McMaster G K, Sutter E, Widmer R, Buxton F

机构信息

Pharma Research Department, Novartis Pharma Inc., CH-4002 Basel, Switzerland.

出版信息

Nucleic Acids Res. 1998 Apr 1;26(7):1826-33. doi: 10.1093/nar/26.7.1826.

Abstract

Two yeast artificial chromosomes containing the entire human nerve growth factor gene were isolated and mapped. By homologous recombination a luciferase gene was precisely engineered into the coding portion of the NGF gene and a neomycin selection marker was placed adjacent to one of the YAC telomeres. Expression of the YAC-based NGF reporter gene and a plasmid-based NGF reporter gene were compared with the regulation of endogenous mouse NGF protein in mouse L929 fibroblasts. In contrast to the plasmid-based reporter gene, expression and regulation of the YAC-based reporter gene was independent of the site of integration of the transgene. Basic fibroblast growth factor and okadaic acid stimulated expression of the YAC transgene, whereas transforming growth factor-beta and dexamethasone inhibited it. Although cyclic AMP strongly stimulated production of the endogenous mouse NGF, no effect was seen on the human NGF reporter genes. Downregulation of the secretion of endogenous mouse NGF already occurred at an EC50 of 1-2 nM dexamethasone, but downregulation of the expression of NGF reporter genes occurred only at EC50 of 10 nM. This higher concentration was also required for upregulation of luciferase genes driven by the dexamethasone-inducible promoter of the mouse mammary tumor virus in L929 fibroblasts.

摘要

分离并定位了两个包含完整人类神经生长因子基因的酵母人工染色体。通过同源重组,将一个荧光素酶基因精确地构建到NGF基因的编码部分,并在其中一个YAC端粒附近放置了一个新霉素选择标记。将基于YAC的NGF报告基因和基于质粒的NGF报告基因的表达与小鼠L929成纤维细胞中内源性小鼠NGF蛋白的调控进行了比较。与基于质粒的报告基因不同,基于YAC的报告基因的表达和调控与转基因的整合位点无关。碱性成纤维细胞生长因子和冈田酸刺激YAC转基因的表达,而转化生长因子-β和地塞米松则抑制其表达。尽管环磷酸腺苷强烈刺激内源性小鼠NGF的产生,但对人类NGF报告基因没有影响。地塞米松的半数有效浓度(EC50)为1-2 nM时,内源性小鼠NGF的分泌就已经下调,但NGF报告基因的表达下调仅在地塞米松的EC50为10 nM时才出现。在L929成纤维细胞中,由小鼠乳腺肿瘤病毒的地塞米松诱导型启动子驱动的荧光素酶基因上调也需要更高的浓度。

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