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Analysis of the Agrobacterium tumefaciens pTiChry5 6b promoter

机译:根癌农杆菌pTiChry5 6b启动子的分析

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The 6b gene of Agrobacterium tumefaciens has evolved to become transcriptionally active in plant cells and has been postulated to modify the activity of plant growth regulators, auxins and cytokinins. To delimit the region that is necessary for expression and is responsible for auxin inducibility, we have constructed a series of 5' deletions and duplications of the A. tumefaciens strain Chry5 6b gene promoter. These deletions and duplications of the 6b gene promoter were fused to the GUS reporter gene and transformed into tobacco (Nicotiana tabacum L cv KY160) to monitor levels and tissue specificity of expression. The -284 bp region upstream of 6b gene translational start site was enough for basal expression and was inducible by auxins, 2,4-D andNAA and to a lesser extent by cytokinin. However, the -438 bp fragment showed higher auxin inducibility. The auxin inducibility was increased by duplication of the upstream region fragments of the promoter. GUS expression was mostly confined to the vascular tissue and the meristem region.
机译:根癌农杆菌的6b基因已经进化为在植物细胞中具有转录活性,并被认为可修饰植物生长调节剂,植物生长素和细胞分裂素的活性。为了界定表达所需的区域并负责植物生长素的诱导,我们构建了根癌农杆菌Chry5 6b基因启动子的5'缺失和重复序列。将6b基因启动子的这些缺失和重复与GUS报告基因融合,并转化到烟草(Nicotiana tabacum L cv KY160)中,以监测表达的水平和组织特异性。 6b基因翻译起始位点上游的-284 bp区域足以进行基础表达,并且可以被生长素,2,4-D和NAA诱导,而被细胞分裂素诱导的程度较小。但是,-438 bp片段显示出较高的生长素诱导性。通过重复启动子的上游区域片段来增加植物生长素的诱导能力。 GUS的表达主要局限于血管组织和分生组织区域。

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