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围产期基因表达分析:激素反应元件介导转基因小鼠肝脏中lacZ报告基因的激活。

Analysis of perinatal gene expression: hormone response elements mediate activation of a lacZ reporter gene in liver of transgenic mice.

作者信息

Montoliu L, Blendy J A, Cole T J, Schütz G

机构信息

Division Molecular Biology of the Cell I (0115), German Cancer Research Center, Heidelberg.

出版信息

Proc Natl Acad Sci U S A. 1995 May 9;92(10):4244-8. doi: 10.1073/pnas.92.10.4244.

Abstract

The transcription of genes encoding gluconeogenic enzymes is tightly regulated during the perinatal period. These genes are induced by glucagon (cAMP) and glucocorticoids and repressed by insulin. To address the role of cAMP and glucocorticoids in the physiological activation of genes encoding gluconeogenic enzymes in the perinatal period, transgenic mice have been generated with chimeric constructs containing the reporter gene lacZ under the control of hormone response elements. The activity of the transgene is restricted to the liver by the presence of the enhancers from the alpha-fetoprotein gene and its transcription is driven by a promoter that contains a TATA box linked to either cAMP response elements (CREs) or glucocorticoid response elements (GREs). We demonstrate cAMP and glucocorticoid regulation, liver-specific expression, and perinatal activation of the reporter gene. These data indicate that the CRE and GRE are, independently, necessary and sufficient to mediate perinatal gene activation. Perinatal activation was not impaired when a CRE reporter transgene was assayed in mice that contain a targeted mutation of the CRE-binding protein (CREB) gene, providing further evidence for functional redundancy among the members of the CREB/ATF gene family.

摘要

在围产期,编码糖异生酶的基因转录受到严格调控。这些基因由胰高血糖素(cAMP)和糖皮质激素诱导,并被胰岛素抑制。为了研究cAMP和糖皮质激素在围产期对编码糖异生酶基因生理激活中的作用,已构建了转基因小鼠,其嵌合构建体包含在激素反应元件控制下的报告基因lacZ。由于甲胎蛋白基因增强子的存在,转基因的活性仅限于肝脏,其转录由一个启动子驱动,该启动子包含与cAMP反应元件(CREs)或糖皮质激素反应元件(GREs)相连的TATA盒。我们证明了报告基因的cAMP和糖皮质激素调控、肝脏特异性表达以及围产期激活。这些数据表明,CRE和GRE各自独立地对于介导围产期基因激活是必要且充分的。当在含有CRE结合蛋白(CREB)基因靶向突变的小鼠中检测CRE报告转基因时,围产期激活并未受损,这为CREB/ATF基因家族成员之间的功能冗余提供了进一步证据。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/15bd/41920/46adde3e0b22/pnas01486-0181-a.jpg

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