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将来自Foxc2报告基因敲入小鼠的体外分化脂肪细胞作为筛选工具。

In vitro differentiated adipocytes from a Foxc2 reporter knock-in mouse as screening tool.

作者信息

Cederberg Anna, Grände Mats, Rhedin Magdalena, Peng Xiao-Rong, Enerbäck Sven

机构信息

Department of Medical and Clinical Genetics, Institute of Biomedicine, Sahlgrenska Academy, Göteborg University, Box 440, 405 30 Göteborg, Sweden.

出版信息

Transgenic Res. 2009 Dec;18(6):889-97. doi: 10.1007/s11248-009-9280-1. Epub 2009 May 28.

Abstract

We have developed a generic model for in vitro high-throughput screening for agents regulating transcription of genes in the mouse genome here exemplified by Foxc2, a forkhead transcription factor involved in regulation of adipocyte metabolism. We made a Foxc2-LacZ reporter "knock-in" mouse in which one of the two Foxc2 alleles has been inactivated and replaced by a LacZ reporter gene. Mouse embryonic fibroblasts, derived from such mice, were differentiated in vitro to adipocytes and used in cell-based screens. Forskolin as well as 12-O-tetradecanoylphorbol-13-acetate (TPA) increased levels of Foxc2nLacZ fusion protein. We could also demonstrate that this was paralleled by an increase in Foxc2 mRNA, transcribed from the wild type allele. This generic method offers a novel way of identifying both positive and negative upstream regulators of a gene, using high-throughput screening methodology. In a cell-based screen using such methodology we demonstrate efficacy by identifying NKH477 as a Foxc2 activating compound.

摘要

我们开发了一种通用模型,用于体外高通量筛选调节小鼠基因组中基因转录的因子,此处以Foxc2为例,Foxc2是一种参与脂肪细胞代谢调节的叉头转录因子。我们构建了一个Foxc2-LacZ报告基因“敲入”小鼠,其中两个Foxc2等位基因中的一个已失活,并被LacZ报告基因取代。从这类小鼠中获取的小鼠胚胎成纤维细胞在体外分化为脂肪细胞,并用于基于细胞的筛选。福斯高林以及12-O-十四酰佛波醇-13-乙酸酯(TPA)可提高Foxc2nLacZ融合蛋白的水平。我们还能证明,这与野生型等位基因转录的Foxc2 mRNA水平升高同时发生。这种通用方法提供了一种利用高通量筛选方法鉴定基因正负上游调节因子的新途径。在使用这种方法的基于细胞的筛选中,我们通过鉴定NKH477为一种Foxc2激活化合物来证明其有效性。

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