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胰腺β细胞中刺激诱导基因表达的在线监测

Online monitoring of stimulus-induced gene expression in pancreatic beta-cells.

作者信息

Moede T, Leibiger B, Berggren P O, Leibiger I B

机构信息

Department of Molecular Medicine, Rolf Luft Center for Diabetes Research, Karolinska Institute, Stockholm, Sweden.

出版信息

Diabetes. 2001 Feb;50 Suppl 1:S15-9. doi: 10.2337/diabetes.50.2007.s15.

Abstract

Fluorescent proteins have been extensively used as protein "tags" to study the subcellular localization of proteins and/or their translocation upon stimulation or as markers for transfection in transient and stable expression systems. However, they have not been frequently used as reporter genes to monitor stimulus-induced gene expression in mammalian cells. Here we demonstrate the use of fluorescent proteins to study stimulus-induced gene transcription. The general applicability of the approach is exemplified by doxycyclin-(Tet-On) and phorbol 12-myristate 13-acetate-induced (c-fos) promoter activation, with green fluorescent protein (GFP) and red fluorescent protein (DsRed) as semiquantitative and immediate reporters, of transcription activation. Under the control of beta-cell-specific promoters, such as the rat insulin 1 promoter or the rat upstream glucokinase promoter, this approach allowed us to monitor online glucose-induced gene transcription in primary beta-cells at the single-cell level as well as in the context of the islet of Langerhans. Applying discretely detectable fluorescent proteins, for example GFP and DsRed, enabled us to simultaneously monitor stimulus-induced transcription by two different promoters in the same cell.

摘要

荧光蛋白已被广泛用作蛋白质“标签”,以研究蛋白质的亚细胞定位和/或其在刺激后的转位,或作为瞬时和稳定表达系统中转染的标记物。然而,它们尚未被频繁用作报告基因来监测哺乳动物细胞中刺激诱导的基因表达。在此,我们展示了使用荧光蛋白来研究刺激诱导的基因转录。强力霉素(Tet-On)和佛波酯12-肉豆蔻酸酯13-乙酸酯诱导的(c-fos)启动子激活以绿色荧光蛋白(GFP)和红色荧光蛋白(DsRed)作为转录激活的半定量和即时报告基因,例证了该方法的普遍适用性。在β细胞特异性启动子(如大鼠胰岛素1启动子或大鼠上游葡萄糖激酶启动子)的控制下,该方法使我们能够在单细胞水平以及在胰岛的背景下在线监测原代β细胞中葡萄糖诱导的基因转录。应用可离散检测的荧光蛋白,例如GFP和DsRed,使我们能够在同一细胞中同时监测由两个不同启动子诱导的刺激转录。

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