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Anther culture induces transposable element movement in potato

机译:花药培养诱导马铃薯中转座子的运动

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摘要

Transposon tagging is a powerful technology for studying gene function; however, somatic transposition prior to gametogenesis may result in multiple derivatives bearing the same insertion. In order to attempt to increase germinal transposition, we synthesized two novel transposon-tagging constructs. We placed the transposase gene under control of either of two microspore-specific promoters identified in Arabidopsis or Antirrhinum within the Ds element that also harbored kanamycin resistance. Both transposase and NPTII gene sequences were optimized in silico based on codon usage bias data in dicot species. Agrobacterium-mediated transformation was used to insert the constructs into diploid potato. The transgenic plants were subjected to both anther culture and outcrossing to wild type diploid potato to observe the opportunity for transposition in either gametophytic process. Green fluorescent protein screening was not efficient but kanamycin selection was able to eliminate 94 % of wild type progenies. Transposants were recovered following anther culture of two transgenic lines whereas no transposants were found among more than 250 T-1 seedlings. Anther culture provided a unique venue for the observation of the influence of gametophye specific promoters on transposition in potato.
机译:转座子标记是研究基因功能的强大技术。然而,配子发生之前的体细胞转座可能会导致多个衍生物带有相同的插入。为了尝试增加生源转座,我们合成了两个新颖的转座子标签构建体。我们将转座酶基因置于拟南芥或Antirrhinum中鉴定的两个小孢子特异性启动子的控制之下,该启动子也包含卡那霉素抗性。基于双子叶植物物种中的密码子使用偏倚数据,在计算机上优化了转座酶和NPTII基因序列。农杆菌介导的转化用于将构建体插入二倍体马铃薯。将转基因植物进行花药培养并与野生型二倍体马铃薯杂交,以观察在任一配子体过程中转座的机会。绿色荧光蛋白筛选效率不高,但卡那霉素的选择能够消除94%的野生型子代。在两个转基因品系的花药培养后回收了转座子,而在250多个T-1幼苗中未发现转座子。花药培养为观察配子体特异性启动子对马铃薯转座的影响提供了一个独特的场所。

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