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    Cryopreservation of the Australian species Macropidia fuliginosa (Haemodoraceae) by vitrification

    Access Status
    Fulltext not available
    Authors
    Turner, Shane
    Tan, B.
    Senaratna, T.
    Bunn, E.
    Dixon, Kingsley
    Touchell, D.H.
    Date
    2000
    Type
    Journal Article
    
    Metadata
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    Citation
    Turner, S.R. and Tan, B. and Senaratna, T. and Bunn, E. and Dixon, K.W. and Touchell, D.H. 2000. Cryopreservation of the Australian species Macropidia fuliginosa (Haemodoraceae) by vitrification. Cryo-Letters. 21 (6): pp. 379-388.
    Source Title
    Cryo-Letters
    ISSN
    0143-2044
    Faculty
    Faculty of Science and Engineering
    School
    School of Molecular and Life Sciences (MLS)
    URI
    http://hdl.handle.net/20.500.11937/91302
    Collection
    • Curtin Research Publications
    Abstract

    Somatic embryos were used to develop a cryopreservation protocol for Macropidia fuliginosa, a commercially-important species endemic to the south-west of Western Australia. Somatic embryos were allowed to develop from embryogenic callus for three weeks on an kinetin medium prior to processing. These were transferred and cultured on a agar solidified basal medium supplemented with 0 to 0.6 M sorbitol for 2 d prior to incubation in Plant Vitrification Solution Two (PVS2). Following this, embryos were then washed in 1 M sucrose solution (treated controls) or cooled in liquid nitrogen (LN). Cooled embryos were then warmed and washed in sucrose solution. Highest survival for cooled treatments (67.3%) was achieved by preculture with 0.4 M sorbitol, then incubation in PVS2. Further experimentation varying pre-culture duration (2 or 3 d) and incubation on either glycerol (0.8 M) or sorbitol (0.4 M) indicated that very high survival (90.6%) of embryos was achievable by adopting a 2 d preculture period on 0.8 M glycerol. The phenotype and growth rates of plants obtained using this protocol were similar to those of parent plants. This optimised procedure was then applied to tissue culture-derived shoot apices of the same clone also resulting in a high survival rate (84.4%).

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