首页> 外文OA文献 >Selectable marker independent transformation of recalcitrant maize inbred B73 and sorghum P898012 mediated by morphogenic regulators \u3ci\u3eBABY BOOM\u3c/i\u3e and \u3ci\u3eWUSCHEL2\u3c/i\u3e
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Selectable marker independent transformation of recalcitrant maize inbred B73 and sorghum P898012 mediated by morphogenic regulators \u3ci\u3eBABY BOOM\u3c/i\u3e and \u3ci\u3eWUSCHEL2\u3c/i\u3e

机译:由形态发生调节子调控的顽固玉米近交自交系B73和高粱P898012的选择性标记独立转化BAUM BOOM \ u3c / i \ u3e和\ u3ci \ u3eWUSCHEL2 \ u3c / i \ u3e

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摘要

The use of morphogenic regulators to overcome barriers in plant transformation is a revolutionary breakthrough for basic plant science and crop applications. Current standard plant transformation systems are bottlenecks for genetic, genomic, and crop improvement studies. We investigated the differential use of co-expression of maize transcription factors BABY BOOM and WUSCHEL2 coupled with a desiccation inducible CRE/lox excision system to enable regeneration of stable transgenic recalcitrant maize inbred B73 and sorghum P898012 without a chemical selectable marker. The PHP78891 expression cassette contains CRE driven by the drought inducible maize RAB17M promoter with lox P sites which bracket the CRE, WUS, and BBM genes. A constitutive maize UBIM promoter directs a ZsGreen GFP expression cassette as a reporter outside of the excision sites and provides transient, transgenic, and developmental analysis. This was coupled with evidence for molecular integration and analysis of stable integration and desiccation inducible CRE-mediated excision. Agrobacterium-mediated transgenic introduction of this vector showed transient expression of GFP and induced somatic embryogenesis in maize B73 and sorghum P898012 explants. Subjection to desiccation stress in tissue culture enabled the excision of CRE, WUS, and BBM, leaving the UBIM::GFP cassette and allowing subsequent plant regeneration and GFP expression analysis. Stable GFP expression was observed in the early and late somatic embryos, young shoots, vegetative plant organs, and pollen. Transgene integration and expression of GFP positive T0 plants were also analyzed using PCR and Southern blots. Progeny segregation analysis of primary events confirmed correlation between functional GFP expression and presence of the GFP transgene in T1 plants generated from self pollinations, indicating good transgene inheritance. This study confirms and extends the use of morphogenic regulators to overcome transformation barriers.
机译:使用形态发生调节剂克服植物转化中的障碍是基础植物科学和作物应用的一项革命性突破。当前的标准植物转化系统是遗传,基因组和作物改良研究的瓶颈。我们研究了玉米转录因子BABY BOOM和WUSCHEL2共表达与干燥诱导型CRE / lox切除系统结合使用的差异性,以使稳定的转基因顽固玉米自交系B73和高粱P898012再生,而无需化学选择标记。 PHP78891表达盒包含受干旱诱导的玉米RAB17M启动子驱动的CRE,该启动子的lox P位点包围着CRE,WUS和BBM基因。组成型玉米UBIM启动子指导ZsGreen GFP表达盒作为报告基因位于切除位点之外,并提供瞬时,转基因和发育分析。这与分子整合的证据以及稳定整合和干燥诱导的CRE介导的切除的分析有关。农杆菌介导的该载体的转基因导入显示了玉米B73和高粱P898012外植体中GFP的瞬时表达和诱导的体细胞胚发生。在组织培养中经受干燥压力使得能够切除CRE,WUS和BBM,留下UBIM :: GFP盒,并允许随后的植物再生和GFP表达分析。在早期和晚期的体细胞胚,幼芽,植物性植物器官和花粉中观察到稳定的GFP表达。还使用PCR和Southern印迹分析了GFP阳性T0植物的转基因整合和表达。对主要事件的后代隔离分析证实了功能性GFP表达与自花授粉产生的T1植物中GFP转基因的存在之间的相关性,表明良好的转基因遗传。这项研究证实并扩展了形态发生调节剂的使用,以克服转化障碍。

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