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An Improved pPZP Vector for Agrobacterium-mediated Plant Transformation

机译:用于农杆菌介导的植物转化的改良pPZP载体

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We report a new and improved pPZP vector (pPZP3425) for efficient plant transformation. This vector is derived from the widely used pPZP100 series of binary Agrobacterium vectors. One disadvantage of these vectors is the use of chloramphenicol resistance for selection in Escherichia coli and Agrobacteria. We have therefore included a kanamycin resistance gene for selection in Agrobacterium. Furthermore, the strong 35S CaMV promoter driving the plant resistance gene has been replaced by the weaker nospromoter because it has been shown that the 35S promoter driving the plant resistance marker can lead to ectopic expression of the transgene. During replacement of the 35S promoter, the Ncol site within the plant resistance gene has been removed, and Ncol can now be used for cloning purposes within the expression cassette which consists of an intron-containing gus gene driven by a strong constitutive promoter (35S promoter with doubled enhancer plus omega-element as translational enhancer). Thus, a single vector can conveniently be used for two purposes: (1) for overexpression of proteins by replacing the gus gene by the coding sequence of choice and (2) for creation of promoter:gus fusions by substituting the constitutive promoter by any other promoter. We demonstrate the usefulness of this vector for cloning a promoter:gus fusion and in planta transformation of Arabidopsis.
机译:我们报告了一种新的和改进的pPZP载体(pPZP3425),用于有效的植物转化。该载体衍生自广泛使用的pPZP100系列双农杆菌载体。这些载体的一个缺点是在氯霉素和农杆菌中使用氯霉素抗性进行选择。因此,我们包括了一种卡那霉素抗性基因供在农杆菌中选择。此外,驱动植物抗性基因的强35S CaMV启动子已被较弱的启动子所取代,因为已显示驱动植物抗性标记的35S启动子可导致转基因的异位表达。在替换35S启动子的过程中,植物抗性基因中的Ncol位点已被去除,Ncol现在可用于表达盒内的克隆目的,该表达盒由由强组成型启动子(35S启动子)驱动的含内含子的gus基因组成加倍的增强剂加上欧米茄元素作为翻译增强剂)。因此,单个载体可方便地用于两个目的:(1)通过用选择的编码序列替换gus基因来过表达蛋白质,以及(2)通过用任何其他组成型启动子取代来创建启动子:gus融合体启动子。我们证明了此载体的克隆启动子:gus融合和拟南芥植物转化的有用性。

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