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毛果杨PtAREB1基因启动子的克隆及功能
引用本文:王含,魏明,李成浩.毛果杨PtAREB1基因启动子的克隆及功能[J].东北林业大学学报,2016(4):18-24.
作者姓名:王含  魏明  李成浩
作者单位:1. 东北林业大学,哈尔滨,150040;2. 林木遗传育种国家重点实验室 东北林业大学
基金项目:国家“863”计划重点项目
摘    要:为了研究杨树ABF2同源基因的表达规律,从毛果杨基因组DNA中克隆出Pt AREB1基因上游一段1 800 bp序列。序列分析结果表明,该序列含有逆境胁迫响应元件TC-rich repeats、ABA应答元件ABRE和茉莉酸甲酯(Methyl Jasmonate,Me JA)应答元件TGACG-motif等胁迫相关元件。在序列分析的基础上,构建了Pt AREB1基因启动子驱动GUS报告基因的植物表达载体,利用农杆菌介导的花粉管通道法获得转基因拟南芥。结果表明Pt AREB1启动子可以在干旱、ABA、盐、Me JA和SA胁迫下,驱动GUS基因在转基因拟南芥的根、茎和叶中表达。说明Pt AREB1基因可能与干旱、高盐等胁迫应答紧密相关。

关 键 词:毛果杨  ABF转录因子  ABA  启动子  拟南芥

Cloning and Functional Identification of Promoter Region of PtAREB1 from Populus trichocarpa
Abstract:In order to study the expression and regulation of ABF homologous gene in poplar , a 1 800 bp 5’ flanking sequence of PtAREB1gene was isolated by PCR from genomic DNA of Populus trichocarpa.By promoter sequence analysis , the se-quence contained stress-response element TC-rich, ABA-response element ABRE and MeJA-response element TGACG-motif.By sequence analysis , the PtA REB1promoter was fused to the GUS reporter gene to characterize its expression pat -tern in P.trichocarpa.From the Agrobacteir um mediated transformation of Arabidopsis th aliana, the GUS gene was induced in Arabidopsis thaliana, and it expressed in roots, stems and leaves under ABA, drought, high salt, MeJA and SA, sug-gesting the PtAREB1 promoter was responsive to ABA , drought and high salt stress .
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