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Titlebook: Agrobacterium Protocols; Volume I Kan Wang Book 2006Latest edition Humana Press 2006 Agrobacterium tumefaciens.Arabidopsis thaliana.DNA.Flo

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https://doi.org/10.1007/978-3-030-40771-1ormation of the maize genotype Hi II. Our starting plant material is immature embryos cocultivated with an . strain carrying a standard binary vector. In addition to step-by-step laboratory transformation procedures, we include extensive details in growing donor plants and caring for transgenic plants in the greenhouse.
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https://doi.org/10.1007/978-3-476-05061-8 of other chemoorganotrophs will usually work for agrobacteria as well. Problems with culture or strain maintenance will occur more frequently because of careless technique than because of strain difficulties. Here we describe a few of the complex and defined media that have been successfully used i
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Dante and Italy in British Romanticismion as a two-component regulatory system to sense particular phenolic compounds synthesized by wounded plant tissues. Induction by these phenolic compounds, in the presence of certain neutral or acid sugars, results in activation of other . genes, leading to the processing of T-DNA from the Ti-plasm
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Introduction: A Mediterranean Comedy,sequently set seed, and transgenic plants are then selected among the progeny seedlings. Because no plant tissue culture is required, somaclonal variation is avoided, and the procedure can be performed easily by nonspecialists. Success rates are high: it is common that 1% of the progeny seedlings ar
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Conclusion: A Sea of Differencesed transformation using “flower dip” and “vacuum infiltration” protocols. However, . has also become a major system to investigate the mechanism of .-mediated transformation of somatic tissue. Such investigations require a reproducible, quantitative assay system to determine transformation frequency
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Introduction: A Mediterranean Comedy,e genotype Jemalong A17 is in progress. By using cotyledons as explants for . infection and direct shoot formation, this protocol allows for rapid production of transgenic plants from A17 and other genotypes. Transgenic plants can be regenerated and established in the greenhouse in only 3-4 mo after
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