| Literature DB >> 22496889 |
Takehito Kaneko1, Tadao Serikawa.
Abstract
BACKGROUND: Freeze-drying sperm has been developed as a new preservation method where liquid nitrogen is no longer necessary. An advantage of freeze-drying sperm is that it can be stored at 4 °C and transported at room temperature. Although the successful freeze-drying of sperm has been reported in a number of animals, the possibility of long-term preservation using this method has not yet been studied. METHODOLOGY/PRINCIPALEntities:
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Year: 2012 PMID: 22496889 PMCID: PMC3322169 DOI: 10.1371/journal.pone.0035043
Source DB: PubMed Journal: PLoS One ISSN: 1932-6203 Impact factor: 3.240
Development of oocytes fertilized with rat epididymal or testicular sperm after freeze-drying.a
| Sperm collected from | Diamide treatment | No. of oocytes transferred | No. (%) of oocytes implanted | No. (%) of offspring |
| Epididymis | − | 54 | 15 (28) | 6 (11) |
| Testis | − | 36 | 0 (0) | 0 (0) |
| Testis | + | 50 | 4 (8) | 4 (8) |
Freeze-dried ampoules were stored for less than 1 month.
Percentages calculated from the number of oocytes transferred.
Within columns, percentages with different letters were significantly different (P<0.05) by analysis of χ2 tests with Yates correction for continuity.
Development of oocytes fertilized with freeze-dried rat sperm stored at 4°C for 5 years.
| No. of oocytes transferred | No. (%) of oocytes implanted | No. (%) of offspring |
| 92 | 18 (20) | 10 (11) |
Percentages calculated from the number of oocytes transferred.
Fertility of individuals derived from oocytes fertilized with freeze-dried sperm stored at 4°C for 5 years.
| Pairs | No. of offspring | No. of males | No. of females |
| A | 16 | 11 | 5 |
| B | 13 | 7 | 6 |
Figure 1DNA fragmentation analyses of sperm. (a) Sperm with normal DNA (left) or fragmented DNA (right).
Freeze-dried epididymal sperm stored at 4°C for 1 week (b) and 5 years (c). Testicular sperm freeze-dried (d) and freeze-dried after treatment with diamide (e) (original magnification 200×).