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A Versatile ΦC31 Based Reporter System for Measuring AP-1 and Nrf2 Signaling in Drosophila and in Tissue Culture

机译:基于多功能ΦC31的报告系统,用于测量果蝇和组织培养物中的AP-1和Nrf2信号

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摘要

This paper describes the construction and characterization of a system of transcriptional reporter genes for monitoring the activity of signaling pathways and gene regulation mechanisms in intact Drosophila, dissected tissues or cultured cells. Transgenic integration of the reporters into the Drosophila germline was performed in a site-directed manner, using ΦC31 integrase. This strategy avoids variable position effects and assures low base level activity and high signal responsiveness. Defined integration sites furthermore enable the experimenter to compare the activity of different reporters in one organism. The reporter constructs have a modular design to facilitate the combination of promoter elements (synthetic transcription factor binding sites or natural regulatory sequences), reporter genes (eGFP, or DsRed.T4), and genomic integration sites. The system was used to analyze and compare the activity and signal response profiles of two stress inducible transcription factors, AP-1 and Nrf2. To complement the transgenic reporter fly lines, tissue culture assays were developed in which the same synthetic ARE and TRE elements control the expression of firefly luciferase.
机译:本文描述了转录报告基因系统的构建和表征,该系统用于监测完整果蝇,解剖组织或培养细胞中信号传导途径的活性和基因调控机制。使用ΦC31整合酶以定点方式将报告基因转入果蝇种系。这种策略避免了位置变化的影响,并确保了较低的碱基水平活性和较高的信号响应能力。明确的整合位点还使实验人员能够比较一种生物体中不同报告基因的活性。报告基因构建体具有模块化设计,可促进启动子元件(合成转录因子结合位点或天然调控序列),报告基因(eGFP或DsRed.T4)和基因组整合位点的组合。该系统用于分析和比较两种应激诱导转录因子AP-1和Nrf2的活性和信号响应谱。为了补充转基因报告基因蝇系,开发了组织培养测定法,其中相同的合成ARE和TRE元件控制萤火虫荧光素酶的表达。

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  • 年度 2012
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  • 原文格式 PDF
  • 正文语种 {"code":"en","name":"English","id":9}
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