1. Investigations on gel forming media for use in low gravity bioseparations research.
- Author
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Todd P, Szlag DC, Plank LD, Delcourt SG, Kunze ME, Kirkpatrick FH, and Pike RG
- Subjects
- Animals, Chickens, Culture Media, Electrophoresis methods, Gelatin, Humans, Polysaccharides, Rabbits, Rats, Sepharose, Cell Separation methods, Erythrocytes cytology, Gels, Weightlessness Simulation
- Abstract
Microgravity research includes investigations designed to gain insight on methods of separating living cells. During a typical separation certain real-time measurements can be made by optical methods, but some materials must also be subjected to subsequent analyses, sometimes including cultivation of the separated cells. In the absence of on-orbit analytical or fraction collecting procedures, some means is required to "capture" cells after separation. The use of solutions that form gels was therefore investigated as a means of maintaining cells and/or macromolecules in the separated state after two types of simple ground-based experiments. Microgravity electrophoresis experiments were simulated by separating model cell types (rat, chicken, human and rabbit erythrocytes) in a vertical density gradient containing low-conductivity buffer, 1.7%-6.5% Ficoll, 6.8-5.0% sucrose, and 1% SeaPrep low-melting temperature agarose and demonstrating that, upon cooling, a gel formed in the column, and cells could be captured in the positions to which they had migrated. Two-phase extraction experiments were simulated by choosing two-polymer solutions in which phase separation occurs in normal saline at temperatures compatible with cell viability and in which one or both phases form a gel upon cooling. Suitable polymers included commercial agaroses (1-2%), maltodextrin (5-7%) and gelatin (5-20%).
- Published
- 1989
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