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Transfection of plant mitochondria and in organello gene integration.

机译:植物线粒体的转染和器官的整合

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Investigation and manipulation of mitochondrial genetics in animal and plant cells remains restricted by the lack of an efficient in vivo transformation methodology. Mitochondrial transfection in whole cells and maintenance of the transfected DNA are main issues on this track. We showed earlier that isolated mitochondria from different organisms can import DNA. Exploiting this mechanism, we assessed the possibility to maintain exogenous DNA in plant organelles. Whereas homologous recombination is scarce in the higher plant nuclear compartment, recombination between large repeats generates the multipartite structure of the plant mitochondrial genome. These processes are under strict surveillance to avoid extensive genomic rearrangements. Nevertheless, following transfection of isolated organelles with constructs composed of a partial gfp gene flanked by fragments of mitochondrial DNA, we demonstrated in organello homologous recombination of the imported DNA with the resident DNA and integration of the reporter gene. Recombination yielded insertion of a continuous exogenous DNA fragment including the gfp sequence and at least 0.5 kb of flanking sequence on each side. According to our observations, transfection constructs carrying multiple sequences homologous to the mitochondrial DNA should be suitable and targeting of most regions in the organelle genome should be feasible, making the approach of general interest.
机译:由于缺乏有效的体内转化方法,动植物体内线粒体遗传学的研究和操作仍然受到限制。线粒体在全细胞中的转染和转染后的DNA的维持是该领域的主要问题。较早前我们证明,来自不同生物体的线粒体可以导入DNA。利用这种机制,我们评估了在植物细胞器中维持外源DNA的可能性。在较高的植物核区室中缺乏同源重组,而大重复序列之间的重组则产生了植物线粒体基因组的多部分结构。这些过程都受到严格监控,以避免广泛的基因组重排。然而,在用由部分 gfp 基因组成的构建体转染线粒体DNA片段后,分离的细胞器被转染后,我们证明了导入的DNA与驻留的DNA的 inorganello 同源重组。和报道基因的整合。重组产生了一个连续的外源DNA片段的插入,该片段包括 gfp 序列和每侧至少0.5kb的侧翼序列。根据我们的观察,携带与线粒体DNA同源的多个序列的转染构建体应该是合适的,并且靶向细胞器基因组中的大多数区域应该是可行的,这使该方法成为人们普遍关注的方法。

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