Maintaining and storing encapsulated cells for propagation of Posidonia oceanica (L.) Delile

Author:

Carrasco-Acosta M1,Garcia-Jimenez P1

Affiliation:

1. Departamento de Biologia, Facultad de Ciencias del Mar, Instituto de Estudios Ambientales y Recursos Naturales, Universidad de Las Palmas de Gran Canaria, 35017 Las Palmas de Gran Canaria, Canary Islands, Spain

Abstract

In the present study, we have developed an efficient system for regenerating Posidonia oceanica via the storage of free cells at low temperature and the initiation of cell encapsulation. This system could help in solving problems related to the intractable nature of in vitro marine phanerogam regeneration. Free cells from enzyme digestion were preserved with glycerol and DMSO at different concentrations and stored at low temperature. Cell encapsulation was performed with sodium alginate and calcium chloride. First, results showed that optimum cell culture was obtained when the initial cell concentration was 104 cells ml-1. Cell scaling allowed exponential growth to produce 2268000 cells at 13 d. Second, treatment based on cell storage with 60% glycerol plus 1.3 M DMSO was a success. The preserved cells grew and produced 1.96 more cells than the initial cell concentration (104 cells ml-1). Third, the encapsulated cells (beads) showed a survival range of 84 to 100% over 4 yr. The divided beads released cells that developed embryos or free cells depending on the culture medium. Cell encapsulation was the only method that was successful to acclimatise the cells to salinity, store artificial material for sowing and obtain embryos. We concluded that encapsulated cells could be used as a starting material for the production of embryos in the regeneration of P. oceanica.

Publisher

Inter-Research Science Center

Subject

Ecology,Aquatic Science,Ecology, Evolution, Behavior and Systematics,Oceanography

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