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Transient gene expression in transformed banana (Musa cv. Bluggoe) protoplasts and embryogenic cell suspensions
Authors:  szló    gi, Serge Remy, Bert Verelst, Bart Panis, Bruno P. A. Cammue, Guido Volckaert  Rony Swennen
Affiliation:(1) Laboratory of Tropical Crop Husbandry, Catholic University of Leuven, Belgium;(2) F.A. Janssens Laboratory of Genetics, Catholic University of Leuven, Belgium;(3) Laboratory of Gene Technology, Catholic University of Leuven, Belgium
Abstract:
Summary In order to introduce currently-available genes with agronomical value into banana, two genetic transformation protocols have been optimized.Firstly, regenerable protoplasts isolated from embryogenic cell suspensions of the cultivar Bluggoe have been used for the introduction of several chimaeric uidA gene constructs by electroporation. With the inclusion of polyethylene glycol and heat shock, the frequency of transiently expressing protoplasts reached 1.8% as shown by an in situ beta-glucuronidase assay. A duplicated 35S promoter with an alfalfa mosaic virus leader sequence (pBI-426) induced the highest expression rate among the constructs tested.Embryogenic cell suspensions of cv. Bluggoe have also been bombarded with accelerated particles coated with a high expression uidA gene construct (pEmuGN) using a biolistic gun. After a partial optimization of the procedure, transient GUS assays reproducibly demonstrated the presence of 400 blue foci in 30 mgrl of settled cell volume (approximately 25 mg cells). Selection and characterization of antibiotic-resistant transformed cultures is in progress.Abbreviations AMV alfalfa mosaic virus - GUS beta-glucuronidase - TGE transient GUS expression - uidA gene for beta-glucuronidase
Keywords:banana  biolistic transformation  electroporation  embryogenic cell suspension  Musa spp.  protoplast
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