Please use this identifier to cite or link to this item: http://repositorio.ufla.br/jspui/handle/1/41409
Title: Genetic transformation of Eucalyptus calmadulensis by agrobalistic method
Other Titles: Transformação genética de Eucalyptus camaldulensis via agrobiobalistica
Keywords: A. tumefasciens EHA 105
pCambia 3301 vetor
Tissue culture
Transient expression
EHA 105 strain
EHA101 strain
Agrobacterium tumefaciens
Cultura de tecidos
Expressão transiente
Cepa EHA 105
Cepa EHA 101
Vetor pCambia 3301
Issue Date: Jun-2013
Publisher: Sociedade de Investigações Florestais (SIF)
Citation: MENDONÇA, E. G. et al. Genetic transformation of Eucalyptus calmadulensis by agrobalistic method. Revista Árvore, Viçosa, MG, v. 37, n. 3, p. 419-429, May/June 2013. DOI: 10.1590/S0100-67622013000300005.
Abstract: Eucalyptus stands in the setting of worldwide forestry due to its adaptability, rapid growth, production of high-quality and low cost of wood pulp fibers. The eucalyptus convetional breeding is impaired mainlly by the long life cycle making the genetic transformation systems an important tool for this purpose. However, this system requires in vitro eficient protocols for plant induction, regeneration and seletion, that allow to obtain transgenic plants from the transformed cell groups. The aim of this work was to evaluate the callus formation and to optimize the leaves and callus genetic transformation protocol by using the Agrobacterium tumefaciens system. Concerning callus formation, two different culture media were evaluated: MS medium supplemented with auxin, cytokinin (M1) and the MS medium with reduced nitrogen concentration and supplemented with auxin, cytokinin coconut water (M2). To establish the leave genetic transformation, those were exposed to agrobiolistics technique (gene gun), to tissue injury, and A. tumesfasciens EHA 105 contening the vetor pCambia 3301 (35S::GUS::NOS), for gene transference and to establish the callus transformation thoses were exposed only to A. tumefasciens. For both experiments, the influence of different infection periods was evaluated. The M2 medium provided the best values for callus sizea and fresh and dry weight. The leaves genetic transformation using the agrobiolistics technique was effective, the gus gene transient expression could be observed. No significant differences were obtained in the infection periods (4, 6 and 8 minutes). The callus genetic transformation with A. tumefaciens also promotend the gus gene transient expression on the callus co-cultiveted for 15 e 30 minutes. The transformed callus was transfered to a regeneration and selection medium and transformed plants were obtained.
URI: http://repositorio.ufla.br/jspui/handle/1/41409
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