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Planta Med 1982; 46(10): 82-87
DOI: 10.1055/s-2007-970026
Research Articles

© Hippokrates Verlag Stuttgart

Cryopreservation of Digitalis lanata Cell Cultures

B. Diettrich1 , A. S. Popov2 , B. Pfeiffer1 , D. Neumann3 , R. Butenko2 , M. Luckner1
  • 1Section of Pharmacy of the Martin-Luther-University, DDR-402 Halle, Weinbergweg 15, GDR
  • 2Timirjazev Institute of Plant Physiology of the Academy of Sciences of USSR, Moscow 127273, Botanicheskaja ul. 35, USSR
  • 3Institute of Plant Biochemistry of the Academy of Sciences of GDR, DDR-402 Halle, Weinbergweg 3, GDR
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Publication History

1982

Publication Date:
29 March 2007 (online)

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Abstract

Suspension cultures of Digitalis lanata strain I were grown in a medium containing 3% mannitol. For cryopreservation cell suspensions were treated with a mixture of sucrose-glycerol (20%/20 V%), cooled slowly (about 1° C/min) till -100° C and then were transferred to liquid nitrogen. After storage in liquid nitrogen the cells were thawed rapidly in a water bath of 40° C and spread on the surface of a solidified nutrient medium. After 7 days of regrowth the cells were suspended in liquid nutrient medium for further cultivation. About 50% of the cells survived freezing and thawing. However, also the apparently surviving cells showed signs of injury (membrane vesicles outside the plasmalemma, dilated ER cisternae and separation of the nuclear membranes). The cultures derived from the surviving cells had the same growth rate and biochemical activity relative to the transformation of cardenolides, e.g., digitoxin, as the parent cultures. The frequency distribution of the nuclear DNA content in the cell cultures was the same before and after cryopreservation. These results indicate that there is no selection of a special cell type during freezing and thawing.

Key Word Index

Digitalis lanata - Scrophulariaceae - Cell Cultures - Cryopreservation - Cardenolides - Digitoxin

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