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Efforts to Initiate Construction of a Disease Resistance Package on a Designer Chromosome in Tobacco

机译:在烟草的设计染色体上启动构建抗病包装的努力

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Gene cloning and transformation can be used to circumvent linkage drag effects that can plague conventional interspecific gene transfers. These techniques can also be used to create desirable genetic linkages. Use of Nicotiana glutinosa L. N-gene mediated TMV (tobacco mosaic virus) resistance in flue-cured tobacco, N tabacum L., has been limited due to linkage drag effects. Transformation was used to introduce the cloned N-gene into NC152, a chromosome addition line possessing a chromosome pair from N africana. This chromosome has been proposed to be used as a a€?designer chromosomea€? into which numerous transgenes could be inserted to form a desirable linkage package. The system could be used to shuttle a large number of transgenes from genotype to genotype. One hundred thirty-six primary transformants possessing the N transgene were produced and hybridized with TMV-susceptible a€?Petite Havana.a€? These may serve as valuable TMV-resistant breeding materials. For each independent transformant, BC1F1 families which segregated for TMV resistance and the addition chromosome were generated. Data from cosegregation, transmission, and molecular analyses were used to conclude that one transformant possessed an insertion of the N-gene in the addition chromosome. By inserting N in the chromosome, we initiated construction of a disease resistance package by linking the TMV resistance gene with a potyvirus resistance gene(s) native to the chromosome. Occasional loss of the transgene, however, may be evidence of previously undetected interchromosomal recombination, and may have implications for use of this system in cultivar development.
机译:基因克隆和转化可用于规避可能困扰常规种间基因转移的连锁拖曳效应。这些技术也可以用来建立理想的遗传联系。由于连锁拖曳效应,限制了烟谷烟草N基因介导的TMV(烟草花叶病毒)抗性在烤烟N. Tabacum L.中的应用。使用转化将克隆的N基因引入到NC152中,NC152是具有来自非洲种的染色体对的染色体添加系。有人建议将该染色体用作“设计染色体”。可以将许多转基因插入其中以形成所需的连接包装。该系统可用于将大量转基因从基因型穿梭到基因型。产生了136个具有N转基因的初级转化体,并与易受TMV感染的α-PetiteHavana杂交。这些可以作为有价值的抗TMV的育种材料。对于每个独立的转化体,产生了针对TMV抗性和附加染色体分离的BC1F1家族。来自共同分离,传播和分子分析的数据用于得出结论,即一个转化子在附加染色体中具有N基因的插入。通过将N插入染色体中,我们通过将TMV抗性基因与染色体固有的马铃薯病毒抗性基因连接起来,开始了抗病包装的构建。但是,偶尔发生转基因丢失可能是以前未发现的染色体间重组的证据,并且可能对该系统在栽培品种开发中的使用有影响。

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