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Fertilisation of cryopreserved sperm and unfertilised quail ovum by intracytoplasmic sperm injection

Authors
Kang, Kyung SooPark, Tae SubRengaraj, DeivendranLee, Hyung ChulLee, Hong JoChoi, Hee JungMizushima, ShuseiOno, TamaoHan, Jae Yong
Issue Date
2016
Publisher
CSIRO PUBLISHING
Keywords
surrogate eggshell
Citation
REPRODUCTION FERTILITY AND DEVELOPMENT, v.28, no.12, pp 1974 - 1981
Pages
8
Journal Title
REPRODUCTION FERTILITY AND DEVELOPMENT
Volume
28
Number
12
Start Page
1974
End Page
1981
URI
https://scholarworks.bwise.kr/cau/handle/2019.sw.cau/64398
DOI
10.1071/RD15126
ISSN
1031-3613
1448-5990
Abstract
Intracytoplasmic sperm injection (ICSI) is an important technique in animal biotechnology for animal cloning and conservation of genetic resources, but has been a challenge for avian species. In the present study, we investigated the ability of cryopreserved quail spermatozoa to achieve fertilisation and embryo development. Female quail were killed 70-120min after previous oviposition to collect unfertilised oocytes from the oviduct. Fresh or cryopreserved-thawed spermatozoa were injected into the cytoplasm of unfertilised oocytes, and the manipulated oocytes were incubated in quail surrogate eggshells. Injection of fresh spermatozoa supplemented with inositol 1,4,5-trisphosphate (IP3) resulted in a significantly increased rate of embryo development compared with injection of fresh spermatozoa alone (90% vs 13%, respectively). Although >80% of embryos stopped cell division and development before Hamburger and Hamilton (HH) Stage 3, approximately 15% of embryos from the fresh sperm injection developed to past HH Stage 4, and one embryo survived up to HH Stage 39 (11 days of incubation). In the case of cryopreserved spermatozoa, the embryo development rate was 30% after ICSI, and this increased significantly to 74% with IP3 supplementation. In conclusion, cryopreserved spermatozoa combined with ICSI followed by surrogate eggshell culture can develop quail embryos.
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