首页> 美国卫生研究院文献>Plant Physiology >Focus Issue on Plastid Biology: High Levels of Bioplastic Are Produced in Fertile Transplastomic Tobacco Plants Engineered with a Synthetic Operon for the Production of Polyhydroxybutyrate
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Focus Issue on Plastid Biology: High Levels of Bioplastic Are Produced in Fertile Transplastomic Tobacco Plants Engineered with a Synthetic Operon for the Production of Polyhydroxybutyrate

机译:质体生物学的重点问题:用合成操纵子生产多羟基丁酸酯的可改造转基因烟草植物中高水平的生物可塑性

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摘要

An optimized genetic construct for plastid transformation of tobacco (Nicotiana tabacum) for the production of the renewable, biodegradable plastic polyhydroxybutyrate (PHB) was designed using an operon extension strategy. Bacterial genes encoding the PHB pathway enzymes were selected for use in this construct based on their similarity to the codon usage and GC content of the tobacco plastome. Regulatory elements with limited homology to the host plastome yet known to yield high levels of plastidial recombinant protein production were used to enhance the expression of the transgenes. A partial transcriptional unit, containing genes of the PHB pathway and a selectable marker gene encoding spectinomycin resistance, was flanked at the 5′ end by the host plant’s psbA coding sequence and at the 3′ end by the host plant’s 3′ psbA untranslated region. This design allowed insertion of the transgenes into the plastome as an extension of the psbA operon, rendering the addition of a promoter to drive the expression of the transgenes unnecessary. Transformation of the optimized construct into tobacco and subsequent spectinomycin selection of transgenic plants yielded T0 plants that were capable of producing up to 18.8% dry weight PHB in samples of leaf tissue. These plants were fertile and produced viable seed. T1 plants producing up to 17.3% dry weight PHB in samples of leaf tissue and 8.8% dry weight PHB in the total biomass of the plant were also isolated.
机译:使用操纵子延伸策略设计了用于烟草(烟草)质体转化的优化遗传构建体,以生产可再生的,可生物降解的塑料聚羟基丁酸酯(PHB)。根据编码PHB途径酶的细菌基因与烟草质体组的密码子使用和GC含量的相似性,选择用于该构建体的细菌基因。与宿主质体组同源性有限的调节元件但已知可产生高水平的质体重组蛋白生产的调节元件用于增强转基因的表达。包含PHB途径的基因和编码壮观霉素抗性的选择标记基因的部分转录单位,在宿主植物的psbA编码序列的5'末端和宿主植物的3'psbA非翻译区的3'末端。这种设计允许将转基因作为psbA操纵子的延伸插入质体组,从而无需添加启动子来驱动转基因的表达。将优化的构建体转化为烟草并随后选择转基因植物的壮观霉素,可生产出能够在叶片组织样品中产生高达18.8%干重PHB的TO植物。这些植物是可育的,并产生了可行的种子。还分离出在叶片组织样品中产生高达17.3%干重PHB的T1植物和在植物总生物量中产生8.8%干重PHB的T1植物。

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