Method for cloning buffalo somatic cell
A technology of somatic cell cloning and donor cells, applied in the fields of botanical equipment and methods, biochemical equipment and methods, applications, etc., can solve the problems of unsuccessful egg development and low developmental potential
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Embodiment 1
[0014] On December 5, 2003, we used the method of the present invention to culture the subcultured (3 passages) female buffalo fetal fibroblasts with 0.1 μg / ml Aphidicolin for 24 hours, and then use the culture medium containing 0.5% FCS for starvation culture. 5d. These cultured cells were transplanted into enucleated native buffalo oocytes on December 11, 2003 to construct recombinant embryos. The recombinant embryos were cultured for 6 days to form blastocysts, which were transplanted into the recipient buffalo uterus on December 17, 2003. After 343 days of gestation, a female cloned buffalo was obtained by caesarean section on November 19, 2004. The cloned buffalo weighed 29kg and had the same gender as the donor cells. The cloned buffalo was completely identical to the donor cells through microsatellite DNA identification.
Embodiment 2
[0016] On March 31, 2004, we treated subcultured (5 passages) adult buffalo ovarian granulosa cells with 0.1 μg / ml Aphidicolin for 24 hours, and then starved them with 0.5% FCS-containing medium for 3 days. On April 4, 2004, these cultured buffalo ovary granulosa cells were used as donor cells to recombine with enucleated native buffalo oocytes to form reconstructed embryos, which were cultured in vitro for 6 days to form cloned blastocysts. On April 10, 2004, the cloned blastocysts were non-surgically transplanted into the recipient buffalo uterus. After 348 days of gestation, a female cloned buffalo was born on March 17, 2005. The cloned buffalo weighed 23kg, had a body length of 86cm, and a body height of 62.5cm. The gender was the same as that of the donor cells. The microsatellite DNA identification confirmed that the cloned buffalo was indeed from the donor cell.
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