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Handling culture medium composition for optimizing plant cell suspension culture in shake flasks
Authors:Tiago Fidemann  Gabriela Aparecida de Araujo Pereira  Tárik Reis Heluy  Rodrigo Boccoli Gallego  Mônica Rosa Bertão  Regildo Márcio Gonçalves da Silva  Eutimio Gustavo Fernández Núñez
Institution:1.INRA, UR 0588, Amélioration, Génétique et Physiologie Forestière,Orléans Cedex 2,France;2.Université de Limoges, Laboratoire de Chimie des Substances Naturelles,Limoges,France;3.Institute of Experimental Botany CAS,Praha 6-Lysolaje,Czech Republic;4.Université de Bordeaux, Centre de Génomique Fonctionnelle, Plateforme Protéome,Bordeaux,France;5.Scion,Rotorua,New Zealand;6.FCBA, P?le Biotechnologie et Sylviculture Avancée,Cestas,France
Abstract:Douglas-fir is a conifer species of major economic importance worldwide, including Western Europe and New Zealand. Herein we describe some characterization and significant refinement of somatic embryogenesis in Douglas-fir, with focus on maturation. The most typical structures observed in the embryonal masses were large polyembryogenic centres (up to 800–1500 µm) with a broad meristem, creating a compact cell “package” with suspensor cells. Singulated somatic embryos composed of both a embryonal head (300–400 µm) and long, tightly arranged suspensor were also frequent. Embryo development was enhanced following embryonal mass dispersion on filter paper discs at low density (50–100 mg fresh mass). Moreover, increasing gellan gum concentration in maturation medium (up to 10 g L?1) improved both the quantity and quality of cotyledonary somatic embryos (SEs), which were subsequently able to germinate and develop into plantlets at high frequency. Embryogenic yield was highly variable among the seven embryogenic lines tested (27–1544 SE g?1 fresh mass). Interestingly secondary somatic embryogenesis could be induced from cotyledonary SEs of both low- and highly-productive lines with some useful practical outcomes: secondary lines from low-performance lines (30–478 SE g?1 fresh mass) displayed significantly higher embryogenic yield (148–1343 SE g?1 fresh mass). In our best conditions, the total protein content in cotyledonary SEs increased significantly with maturation duration (up to 150 µg mg?1 fresh mass after 7 weeks) but remained below that of mature zygotic embryos (300 µg mg?1). The protein pattern was similar in both somatic and zygotic embryos, with major storage proteins identified as 7S-vicilin- and legumin-like proteins.
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