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Transgenic sterility in Populus: expression properties of the poplar PTLF, Agrobacterium NOS and two minimal 35S promoters in vegetative tissues

机译:杨的转基因不育:在营养组织中杨PTLF,农杆菌NOS和两个最小的35S启动子的表达特性

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Transgenic sterility is a desirable trait for containment of many kinds of transgenes and exotic species. Genetically engineered floral sterility can be imparted by expression of a cytotoxin under the control of a predominantly floral-tissue-specific promoter. However, many otherwise desirable floral promoters impart substantial non-floral expression, which can impair plant health or make it impossible to regenerate transgenic plants. We are therefore developing a floral sterility system that is capable of attenuating undesired background vegetative expression. As a first step towards this goal, we compared the vegetative expression properties of the promoter of the poplar (Populus trichocarpa Torr. & Gray) homolog of the floral homeotic gene LEAFY (PTLF), which could be used to impart male and female flower sterility, to that of three candidate attenuator-gene promoters: the cauliflower mosaic virus (CaMV) 35S basal promoter, the CaMV 35S basal promoter fused to the TMV omega element and the nopaline synthase (NOS) promoter. The promoters were evaluated via promoter::GUS gene fusions in a transgenic poplar hybrid (Populus tremula L. x P. alba L.) by both histochemical and fluorometric GUS assays. In leaves, the NOS promoter conveyed the highest activity and had a mean expression level 5-fold higher than PTLF, whereas the CaMV 35S basal promoter fused to the omega element and the CaMV 35S basal promoter alone directed mean expression levels that were 0.5x and 0.35x that of PTLF, respectively. Differential expression in shoots, leaves, stems and roots was observed only for the NOS and PTLF promoters. Strongest expression was observed in roots for the NOS promoter, whereas the PTLF promoter directed highest expression in shoots. The NOS promoter appears best suited to counteract vegetative expression of a cytotoxin driven by the PTLF promoter where 1:1 toxin:attenuator expression is required.
机译:转基因不育是遏制多种转基因和外来物种的理想特性。可以通过在主要是花组织特异性启动子的控制下表达细胞毒素来赋予基因工程的花卉无菌性。然而,许多本来希望的花卉启动子赋予大量的非花卉表达,这会损害植物健康或使其无法再生转基因植物。因此,我们正在开发一种花卉不育系统,该系统能够减弱不需要的背景营养表达。作为朝着这个目标迈出的第一步,我们比较了花卉同源基因LEAFY(PTLF)的杨树(Populus trichocarpa Torr。&Gray)同系物启动子的营养表达特性,该基因可用于赋予雄性和雌性花卉不育性到三个候选的减毒基因启动子:花椰菜花叶病毒(CaMV)35S基础启动子,融合到TMVΩ元件上的CaMV 35S基础启动子和胭脂碱合酶(NOS)启动子。通过组织化学和荧光GUS分析,通过在转基因杨树杂种(Populus tremula L. x P. alba L.)中的启动子:: GUS基因融合体评估启动子。在叶片中,NOS启动子传递的活性最高,平均表达水平比PTLF高5倍,而融合到欧米茄元件上的CaMV 35S基础启动子和单独的CaMV 35S基础启动子指导的平均表达水平为0.5x和分别是PTLF的0.35倍。仅对于NOS和PTLF启动子观察到在芽,叶,茎和根中的差异表达。在根中观察到最强的NOS启动子表达,而PTLF启动子在芽中定向最高表达。 NOS启动子似乎最适合抵消由PTLF启动子驱动的细胞毒素的营养表达,其中需要1:1毒素:衰减子表达。

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