Initiation of embryogenic cell suspensions of taro (<Emphasis Type="Italic">Colocasia esculenta</Emphasis> var. <Emphasis Type="Italic">esculenta</Emphasis>) and plant regeneration |
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| Authors: | Pradeep C Deo Mary Taylor Robert M Harding Anand P Tyagi Douglas K Becker |
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| Institution: | (1) School of Biological and Chemical Sciences, Faculty of Science, Technology and Environment, University of the South Pacific, Suva, Fiji;(2) Centre for Pacific Crops and Trees, Secretariat of the Pacific Community, Suva, Fiji;(3) Centre for Tropical Crops and Biocommodities, Faculty of Science, Queensland University of Technology, Brisbane, Queensland, Australia |
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| Abstract: | Embryogenic callus was initiated by culturing in vitro taro corm slices on agar-solidified half-strength MS medium containing
2.0 mg/L 2,4-dichlorophenoxyacetic acid (2,4-D) for 20 days followed by transfer to 1.0 mg/L thidiazuron (TDZ). Callus was
subsequently proliferated on solid medium containing 1.0 mg/L TDZ, 0.5 mg/L 2,4-D and 800 mg/L glutamine before transfer to
liquid medium containing the same components but with reduced glutamine (100 mg/L). After 3 months in liquid culture on an
orbital shaker, cytoplasmically dense cell aggregates began to form. Somatic embryogenesis was induced by plating suspension
cells onto solid media containing reduced levels of hormones (0.1 mg/L TDZ, 0.05 mg/L 2,4-D), high concentrations of sucrose
(40–50 g/L) and biotin (1.0 mg/L). Embryo maturation and germination was then induced on media containing 0.05 mg/L benzyladenine
(BA) and 0.1 mg/L indole-3-acetic acid (IAA). Histological studies of the developing embryos revealed the presence of typical
shoot and root poles suggesting that these structures were true somatic embryos. The rate of somatic embryos formation was
500–3,000 per mL settled cell volume while approximately 60% of the embryos regenerated into plants. |
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