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对位于拟南芥中控制水杨酸诱导的NIMIN-1表达的启动子区域的一个TGA因子结合位点的功能分析。

Functional analysis of a TGA factor-binding site located in the promoter region controlling salicylic acid-induced NIMIN-1 expression in Arabidopsis.

作者信息

Fonseca J P, Menossi M, Thibaud-Nissen F, Town C D

机构信息

Departamento de Genética, Evolução e Bioagentes, Universidade Estadual de Campinas, Campinas, SP, Brasil.

出版信息

Genet Mol Res. 2010 Feb 2;9(1):167-75. doi: 10.4238/vol9-1gmr704.

DOI:10.4238/vol9-1gmr704
PMID:20198573
Abstract

TGA factors play a key role in plant defense by binding to the promoter region of defense genes, inducing expression. Salicylic acid (SA) induces the expression of the gene encoding NIMIN-1, which interacts with NPR1/NIM1, a key regulator of systemic acquired resistance. We investigated whether the TGA2-binding motif TGACG located upstream of the NIMIN-1 gene is necessary for SA induction of NIMIN-1 expression. A mutated version of the NIMIN-1 promoter was created by site-directed mutagenesis. We generated T-DNA constructs in which native NIMIN-1 and mutated promoters were fused to green fluorescent protein and beta-glucuronidase reporters. We produced transgenic Arabidopsis plants and observed NIMIN-1 promoter-driven green fluorescent protein expression in the roots, petiole and leaves. Constructs were agroinfiltrated into the leaves for transient quantitative assays of gene expression. Using quantitative real-time RT-PCR, we characterized the normal gene response to SA and compared it to the response of the mutant version of the NIMIN-1 promoter. Both the native NIMIN-1 construct and an endogenous copy of NIMIN-1 were induced by SA. However, the mutated promoter construct was much less sensitive to SA than the native NIMIN-1 promoter, indicating that this TGA2-binding motif is directly involved in the modulation of SA-induced NIMIN-1 expression in Arabidopsis.

摘要

TGA因子通过与防御基因的启动子区域结合来诱导表达,从而在植物防御中发挥关键作用。水杨酸(SA)可诱导编码NIMIN-1的基因表达,NIMIN-1与系统获得性抗性的关键调节因子NPR1/NIM1相互作用。我们研究了位于NIMIN-1基因上游的TGA2结合基序TGACG对于SA诱导NIMIN-1表达是否必要。通过定点诱变创建了NIMIN-1启动子的突变版本。我们构建了T-DNA载体,其中天然NIMIN-1和突变启动子与绿色荧光蛋白和β-葡萄糖醛酸酶报告基因融合。我们培育了转基因拟南芥植株,并观察了NIMIN-1启动子驱动的绿色荧光蛋白在根、叶柄和叶片中的表达。将构建体通过农杆菌浸润法导入叶片进行基因表达的瞬时定量分析。使用定量实时RT-PCR,我们表征了正常基因对SA的反应,并将其与NIMIN-1启动子突变体版本的反应进行比较。天然NIMIN-1构建体和NIMIN-1的内源拷贝均受SA诱导。然而,突变启动子构建体对SA的敏感性远低于天然NIMIN-1启动子,表明该TGA2结合基序直接参与了拟南芥中SA诱导的NIMIN-1表达的调控。

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