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Infection of Embryonic Callus with Agrobacterium Enables High-Speed Transformation of Maize

机译:农杆菌感染胚性愈伤组织可实现玉米的高速转化

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摘要

Several approaches have recently been adopted to improve Agrobacterium-mediated transformation of maize; however, about eight months of in vitro culture are still required to isolate transgenic plants. Furthermore, genetic transformation of maize depends on immature embryos, which greatly increases costs. Here, we report a method that ensures the competency of an embryogenic callus secondary culture under laboratory conditions for Agrobacterium-mediated transformation. Moreover, pretreatment of the cell wall with a mixed lytic enzyme solution prior to Agrobacterium infection, significantly improved transformation efficiency and stability. Average stable transformation efficiency was approximately 30.39%, with peaks of 94.46%. Expression and phenotypic analysis of the Rsc reporter gene were tested in the T0 generation of transgenic plants. Using this system, we successfully regenerated transgenic maize plantlets within three months of the emergence of the embryogenic callus. Additionally, we reduced somaclonal variation accompanying prolonged culture of maize cells in the dedifferentiated state, thus facilitating the molecular breeding of maize.
机译:最近已经采用了几种方法来改善土壤杆菌介导的玉米转化。然而,分离转基因植物仍需要大约八个月的体外培养。此外,玉米的遗传转化依赖于未成熟的胚,这大大增加了成本。在这里,我们报告一种方法,可确保在实验室条件下农杆菌介导的转化的胚性愈伤组织继代培养的能力。而且,在农杆菌感染之前用混合的裂解酶溶液预处理细胞壁,显着提高了转化效率和稳定性。平均稳定转化效率约为30.39%,峰值为94.46%。在转基因植物的T0代中测试了Rsc报道基因的表达和表型分析。使用该系统,我们在胚性愈伤组织出现后的三个月内成功地再生了转基因玉米苗。此外,我们减少了在去分化状态下长时间培养玉米细胞伴随的体细胞克隆变异,从而促进了玉米的分子育种。

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