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Abstract
Maintaining biodiversity is an essential task, but storing germ cells as genetic resources using liquid nitrogen is difficult, expensive, and easily disrupted during disasters. Our aim is to generate cloned mice from freeze-dried somatic cell nuclei, preserved at −30 °C for up to 9 months after freeze drying treatment. All somatic cells died after freeze drying, and nucleic DNA damage significantly increased. However, after nuclear transfer, we produced cloned blastocysts from freeze-dried somatic cells, and established nuclear transfer embryonic stem cell lines. Using these cells as nuclear donors for re-cloning, we obtained healthy cloned female and male mice with a success rate of 0.2–5.4%. Here, we show that freeze-dried somatic cells can produce healthy, fertile clones, suggesting that this technique may be important for the establishment of alternative, cheaper, and safer liquid nitrogen-free bio-banking solutions.
The development of safe preservation methods for genetic resources is important. Here, the authors successfully produce cloned mice from freeze-dried somatic cells, demonstrating the possibility of safe and low-cost preservation of genetic resources.
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1 University of Yamanashi, Faculty of Life and Environmental Science, Kofu, Japan (GRID:grid.267500.6) (ISNI:0000 0001 0291 3581); University of Yamanashi, Advanced Biotechnology Center, Kofu, Japan (GRID:grid.267500.6) (ISNI:0000 0001 0291 3581)
2 University of Yamanashi, Faculty of Life and Environmental Science, Kofu, Japan (GRID:grid.267500.6) (ISNI:0000 0001 0291 3581)