Preservation of viable biological samples for experiments in space laboratories

Standard viable preservation methods for biological samples using low temperatures have been investigated concerning their storage capabilities under higher temperature levels than usual. For a representative set of organism classes (plants, mammalian cells, arthropods and aquatic invertebrates), th...

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Bibliographic Details
Published in:Journal of biotechnology 1996-06, Vol.47 (2), p.377-393
Main Authors: Anthony, P., Ausseil, J., Bechler, B., Benguría, A., Blackhall, N., Briarty, L.G., Cogoli, A., Davey, M.R., Garesse, R., Hager, R., Loddenkemper, R., Marchant, R., Marco, R., Marthy, H.J., Perry, M., Power, J.B., Schiller, P., Ugalde, C., Volkmann, D., Wardrop, J.
Format: Article
Language:English
Subjects:
Animals
Biotechnology
Cells, Cultured
Cryopreservation - methods
Evaluation Studies as Topic
Female
Humans
Male
Preservation capabilities
Preservation, Biological - methods
Space and ground application
Space Flight
Space life sciences
Standard preservation methods
Survival screening
Temperature
Thermal conditioning requirements
Time Factors
Viability
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Summary:Standard viable preservation methods for biological samples using low temperatures have been investigated concerning their storage capabilities under higher temperature levels than usual. For a representative set of organism classes (plants, mammalian cells, arthropods and aquatic invertebrates), the minimum appropriate storage conditions have been identified by screening storage temperatures at − 196 °, −80 °, −20 °, +4 °, + 20 °/25 °C for periods from 2 days to 4 weeks. For storage below 0 °C, as a typical cryopreservative, dimethylsulfoxide (DMSO) was used. For some samples, the addition of trehalose (as cryopreservative) and the use of a nitrogen atmosphere were investigated. After storage, the material was tested for vitality. The findings demonstrated that acceptable preservation can be achieved under higher storage temperatures than are typically applied. Small, dense cultured plant cells survive for 21 d when moderately cooled (+4 ° to − 20 °C); addition of trehalose enhances viability at − 20 °C. For mammalian cells, the results show that human lymphocytes can be preserved for 3 d at 25 °C, 7 d at 4 °C and 28 d at − 80 °C. Friend leukaemia virus transformed cells can be stored for 3 d at 25 °C, 14 d at 4 °C and 28 d at − 80 °C. Hybridoma cells can be kept 7 d at 4 °C and 28 d at − 20 dgC or − 80 °C. Model arthropod systems are well preserved for 2 weeks if maintained at lower temperatures that vary depending on the species and/or stage of development; e.g., 12 °C for Drosophila imagoes and 4–6 °C for Artemia nauplii. For aquatic invertebrates such as sea urchins, embryonic and larval stages can be preserved for several weeks at +6 °C, whereas sperm and eggs can best be stored at +4 °C for up to 5 d at maximum.These results enhance the range of feasible space experiments with biological systems. Moreover, for typical terrestrial preservation methods, considerable modification potential is identified.
ISSN:0168-1656
1873-4863
DOI:10.1016/0168-1656(96)01363-6