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拟南芥中基因表达的时空可控诱导

Temporally and spatially controlled induction of gene expression in Arabidopsis thaliana.

作者信息

Maizel Alexis, Weigel Detlef

机构信息

Department of Molecular Biology, Max Planck Institute for Developmental Biology, Spemannstrasse 37-39, D-72076 Tübingen, Germany.

出版信息

Plant J. 2004 Apr;38(1):164-71. doi: 10.1111/j.1365-313X.2004.02027.x.

DOI:10.1111/j.1365-313X.2004.02027.x
PMID:15053769
Abstract

Temporally and spatially regulated induction of gene expression is an important tool of genetic analysis. In plants, several systems are available for spatially unregulated induction of gene expression, or for spatially regulated expression. Here, we describe a new system that provides both temporal and spatial control for transgene expression. It combines the advantages of its two constituent components: temporally regulated activity of the ethanol-dependent AlcR transcription factor, and tissue specificity of a plant promoter. As a proof of principle, transgenic lines were developed in which the promoter of the meristem identity gene LEAFY (LFY) provided flower-specific expression of the AlcR activator. Tissue-specific activity of AlcR was confirmed with a responder in which the beta-glucuronidase (GUS) reporter was under the control of the alcA response element. As expected, reporter activity in a pattern typical for the LFY promoter was ethanol dependent. Next, we placed the LFY coding sequenced under control of the AlcA response element. In a strong lfy-12 background, this construct in combination with the LFY:AlcR driver provided complete, ethanol-dependent rescue of the lfy phenotype, including restoration of fertility. Apart from facilitating the investigation of temporal and spatial requirements of gene activity, this technology will permit new types of genetic modifier screens starting with mutations that otherwise confer lethality or sterility.

摘要

基因表达在时间和空间上的调控诱导是遗传分析的重要工具。在植物中,有几种系统可用于基因表达的空间非调控诱导或空间调控表达。在此,我们描述了一种新系统,它能对转基因表达提供时间和空间控制。它结合了其两个组成部分的优点:乙醇依赖性AlcR转录因子的时间调控活性以及植物启动子的组织特异性。作为原理验证,构建了转基因株系,其中分生组织特性基因LEAFY(LFY)的启动子提供AlcR激活剂的花特异性表达。用一个响应载体证实了AlcR的组织特异性活性,该载体中β-葡萄糖醛酸酶(GUS)报告基因受alcA响应元件控制。正如预期的那样,LFY启动子典型模式下的报告基因活性依赖于乙醇。接下来,我们将LFY编码序列置于AlcA响应元件的控制之下。在强lfy - 12背景下,该构建体与LFY:AlcR驱动子结合,能完全依赖乙醇拯救lfy表型,包括恢复育性。除了便于研究基因活性的时间和空间需求外,这项技术还将允许开展新型的遗传修饰筛选,起始于那些否则会导致致死性或不育性的突变。

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