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Agrobacterium: A Genome-Editing Tool-Delivery System

机译:农杆菌:一种基因组编辑工具输送系统

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With the rapidly increasing global population, it will be extremely challenging to provide food to the world without increasing food production by at least 70% over the next 30 years. As we reach the limits of expanding arable land, the responsibility of meeting this production goal will rely on increasing yields. Traditional plant breeding practices will not be able to realistically meet these expectations, thrusting plant biotechnology into the limelight to fulfill these needs. Better varieties will need to be developed faster and with the least amount of regulatory hurdles. With the need to add, delete, and substitute genes into existing genomes, the field of genome editing and gene targeting is now rapidly developing with numerous new technologies coming to the forefront. Agrobacterium-mediated crop transformation has been the most utilized method to generate transgenic varieties that are better yielding, have new traits, and are disease and pathogen resistant. Genome-editing technologies rely on the creation of double-strand breaks (DSBs) in the genomic DNA of target species to facilitate gene disruption, addition, or replacement through either non-homologous end joining or homology-dependent repair mechanisms. DSBs can be introduced through the use of zinc-finger nucleases (ZFNs), transcription activator-like effector nucleases (TALENs), or clustered regularly interspersed short palindromic repeats (CRISPR)/Cas nucleases, among others. Agrobacterium strains have been employed to deliver the reagents for genome editing to the specific target cells. Understanding the biology of transformation from the perspective not only of Agrobacterium, but also of the host, from processing of T-DNA to its integration in the host genome, has resulted in a wealth of information that has been used to engineer Agrobacterium strains having increased virulence. As more technologies are being developed, that will help overcome issues of Agrobacterium host range and random integration of DNA, combined with highly sequence-specific nucleases, a robust crop genome-editing toolkit finally seems attainable.
机译:随着全球人口迅速增加,在未来30年内向世界提供食物,为世界提供食物将是极为挑战性的。随着我们达到扩大耕地的极限,符合这一生产目标的责任将依赖于增加收益率。传统的植物育种实践将无法实现这些期望,将植物生物技术推动到敏捷者以满足这些需求。需要更快地制定更好的品种,并具有最少的监管障碍。随着需要将基因添加,删除和替换到现有基因组中,目前基因组编辑和基因靶向的领域现在与最前沿的许多新技术迅速发展。农杆菌介导的作物转化一直是产生更好的屈服的转基因品种的最具利用方法,具有新的性状,并且是疾病和病原体。基因组编辑技术依赖于靶物种基因组DNA中的双链断裂(DSB),以促进基因破坏,添加或通过非同源终端连接或同源依赖性修复机制替代。 DSB可以通过使用锌指核酸酶(ZFN),转录活化剂样效应核酸酶(TALENS),或者定期散布的短语重复(CRISPR)/ CAS核酸酶,等等。已经使用农杆菌菌株来递送对特定靶细胞的基因组的试剂。理解从透视的转化生物学,而且宿主也从宿主基因组的整合到宿主中,这导致了丰富的信息,这些信息已被用于工程株增加的土壤杆菌菌株毒力。随着正在开发更多技术的,这将有助于克服农杆菌宿主范围和DNA随机整合的问题,与高度序列特异性的核酸酶相结合,稳健的作物基因组编辑工具包最终似乎可达。

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