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Generation of Marker- and/or Backbone-Free Transgenic Wheat Plants via Agrobacterium-Mediated Transformation

机译:通过农杆菌介导的转化产生无标记和/或无主链的转基因小麦植物

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摘要

Horizontal transfer of antibiotic resistance genes to animals and vertical transfer of herbicide resistance genes to the weedy relatives are perceived as major biosafety concerns in genetically modified (GM) crops. In this study, five novel vectors which used gusA and bar as a reporter gene and a selection marker gene, respectively, were constructed based on the pCLEAN dual binary vector system. Among these vectors, 1G7B and 5G7B carried two T-DNAs located on two respective plasmids with 5G7B possessing an additional virGwt gene. 5LBTG154 and 5TGTB154 carried two T-DNAs in the target plasmid with either one or double right borders, and 5BTG154 carried the selectable marker gene on the backbone outside of the T-DNA left border in the target plasmid. In addition, 5BTG154, 5LBTG154, and 5TGTB154 used pAL154 as a helper plasmid which contains Komari fragment to facilitate transformation. These five dual binary vector combinations were transformed into Agrobacterium strain AGL1 and used to transform durum wheat cv Stewart 63. Evaluation of the co-transformation efficiencies, the frequencies of marker-free transgenic plants, and integration of backbone sequences in the obtained transgenic lines indicated that two vectors (5G7B and 5TGTB154) were more efficient in generating marker-free transgenic wheat plants with no or minimal integration of backbone sequences in the wheat genome. The vector series developed in this study for generation of marker- and/or backbone-free transgenic wheat plants via Agrobacterium-mediated transformation will be useful to facilitate the creation of “clean” GM wheat containing only the foreign genes of agronomic importance.
机译:抗生素抗性基因向动物的水平转移和除草剂抗性基因向杂草近缘种的垂直转移被认为是转基因作物的主要生物安全问题。在这项研究中,基于pCLEAN双二元载体系统,构建了分别使用gusA和bar作为报告基因和选择标记基因的5种新颖载体。在这些载体中,1G7B和5G7B带有两个位于两个各自质粒上的T-DNA,而5G7B具有另外的virGwt基因。 5LBTG154和5TGTB154在目标质粒中带有两个T-DNA,带有一个或两个右边界,而5BTG154在目标质粒中T-DNA左边界之外的主链上带有选择标记基因。此外,5BTG154、5LBTG154和5TGTB154使用pAL154作为辅助质粒,其中包含Komari片段以促进转化。这五种双重双元载体组合被转化到农杆菌AGL1菌株中,并用于转化硬粒小麦Stewart63。共转化效率,无标记转基因植物的频率以及获得的转基因品系中主链序列的整合评估两种载体(5G7B和5TGTB154)在生成无标记的转基因小麦植株中效率更高,而小麦基因组中的骨架序列没有或仅有极少的整合。在这项研究中开发的用于通过农杆菌介导的转化生成无标记和/或无主链的转基因小麦植物的载体系列将有助于促进仅含有农艺学重要外源基因的“清洁”转基因小麦的产生。

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