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A promoter directing high level expression in pistils of transgenic plants.

机译:指导转基因植物雌蕊中高水平表达的启动子。

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摘要

The promoter of the potato (Solanum tuberosum) SK2 gene, encoding a pistil-specific basic endochitinase, was cloned. Various fragments of the SK2-promoter, from 1 kb down to 0.23 kb in length, were fused to the GUS reporter gene. Chimaeric SK2 promoter-GUS fusion constructs were transformed into potato by Agrobacterium tumefaciens-mediated transformation. The SK2-GUS transgenic potato plants exhibited a highly specific GUS activity in the pistil. Expression in the pistil was shown to be developmentally regulated. In addition to the GUS activity in pistils, transgenic plants also showed a much weaker ectopic expression in anthers. In other tissues no systematic expression was detectable. All SK2 promoter fragments analysed conferred pistil-specificexpression without significant qualitative or quantitative differences, demonstrating that the regulatory elements mediating this expression pattern are located within a 230 bp SK2 promoter fragment. The SK2 promoter may be used to engineer high levelsof expression in pistils of transgenic plants.
机译:克隆了马铃薯(Solanum tuberosum)SK2基因的启动子,该基因编码雌蕊特异性碱性内切几丁质酶。长度从1 kb到0.23 kb的各种SK2启动子片段与GUS报告基因融合。通过根癌农杆菌介导的转化将Chimaeric SK2启动子-GUS融合构建体转化为马铃薯。 SK2-GUS转基因马铃薯植株在雌蕊中表现出高度特异性的GUS活性。雌蕊中的表达显示受发育调节。除雌蕊中的GUS活性外,转基因植物在花药中的异位表达也弱得多。在其他组织中,未检测到系统表达。分析的所有SK2启动子片段均赋予雌蕊特异性表达,而没有明显的定性或定量差异,表明介导该表达模式的调控元件位于230 bp的SK2启动子片段内。 SK2启动子可用于工程化转基因植物雌蕊中的高水平表达。

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