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首页> 外文期刊>Maydica >Improving in vitro culture and regeneration conditions for Agrobacterium-mediated maize transformation.
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Improving in vitro culture and regeneration conditions for Agrobacterium-mediated maize transformation.

机译:改善农杆菌介导的玉米转化的体外培养和再生条件。

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Experimental conditions for improving the tissue culture regenerative potential and embryogenic capability of maize cultures after Agrobacterium-mediated transformation have been investigated. The parameters were investigated in five elite inbreds per se and in their crosses with A188. Embryogenic calli obtained from the inbreds spanned in a range of values from hardly responsive (11.5%) to highly responsive (79.1%) cultures. Immature embryos explanted from crosses of each inbred with A188 were all enhanced in their embryogenic and regenerative capability, with values ranging from 72.7 to 79.6%. The same genotypes, were subjected to Agrobacterium-mediated transformation, considering as target tissue either freshly explanted or five days-precultured immature embryos. Tissues were transformed with the Agrobacterium strain EHA105 with a standard binary vector based on pCAMBIA3301. The addition of 400mg/l L-cysteine in the co-cultivation step, as antioxidant to reduce callus necrosis, was also tested. Results indicated that addition of L-cys in the infection step with non pre-cultured embryos in general reduces regenerative capability, inhibiting the embryogenic development of the infected embryos. Conversely, the adoption of a pre-culture period of five days on callus induction medium, largely overcomes the inhibition. Calli treated and non-treated with L-cys exhibited comparable embryogenic potential; in addition, the regenerative capability was significantly enhanced. The protocol described is discussed as an improvement in Agrobacterium-mediated maize transformation.
机译:研究了提高农杆菌介导的转化后玉米培养物的组织培养物再生潜力和胚发生能力的实验条件。在五个自交系和与A188杂交的自交系中研究了这些参数。从近交系获得的胚性愈伤组织的值范围很广,从几乎不响应(11.5%)到高度响应(79.1%)培养。从每只自交系A188的杂交中移出的未成熟胚的胚发生和再生能力均得到增强,其值在72.7至79.6%之间。将相同基因型进行农杆菌介导的转化,将新鲜移植或五天预培养的未成熟胚视为目标组织。用农杆菌菌株EHA105和基于pCAMBIA3301的标准二元载体转化组织。还测试了在共培养步骤中添加400mg / l L-半胱氨酸作为抗氧化剂,以减少愈伤组织坏死。结果表明,在非预培养胚胎的感染步骤中添加L-cys通常会降低再生能力,从而抑制了受感染胚胎的胚胎发生发育。相反地​​,在愈伤组织诱导培养基上采用五天的预培养期大大克服了抑制作用。用L-cys处理和未处理的愈伤组织均具有可比的胚发生潜能。此外,再生能力也大大增强。所描述的方案被讨论为对农杆菌介导的玉米转化的改进。

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