An efficient method for producing α(1,3)-galactosyltransferase gene knockout pigs

被引:42
作者
Harrison, S
Boquest, A
Grupen, C
Faast, R
Guildolin, A
Giannakis, C
Crocker, L
McIlfatrick, S
Ashman, R
Wengle, J
Lyons, I
Tolstoshev, P
Cowan, P
Robins, A
O'Connell, P
D'Apice, AJF
Nottle, M
机构
[1] BresaGen Ltd, Adelaide, SA, Australia
[2] Univ Melbourne, St Vincents Hosp, Immunol Res Ctr, Melbourne, Vic, Australia
[3] Univ Sydney, Westmead Hosp, Natl Pancreas Transplant Unit, Sydney, NSW 2006, Australia
关键词
D O I
10.1089/clo.2004.6.327
中图分类号
Q813 [细胞工程];
学科分类号
摘要
We have reported relatively efficient methods for somatic cell nuclear transfer and for knocking out the alpha(1,3)-galactosyltransferase (alpha1,3-GT) gene in porcine fetal fibroblasts using a nonisogenic promoterless construct approach. Here we report the production of alpha1,3-GT gene knockout pigs using these procedures. Seven alpha1,3-GT gene knockout cell clones were identified by long-range PCR from 108 neomycin resistant (neo(R)) colonies, giving a 6.5% targeting efficiency. Three cell clones were used for nuclear transfer. Nuclear transfer was performed using a fusion before activation protocol using in vitro-matured adult oocytes. Between 51 and 110 fused couplets were transferred to 10 recipients synchronized 1 day behind the embryos. Parturition was induced on day 115, and piglets were delivered by caesarean section. Four recipients gave birth to a total of 18 live piglets. All pigs were female, and all three clones resulted in the birth of live pigs. alpha1,3-GT gene knockout pigs were identified by long-range PCR and confirmed by Southern blot analysis. The efficiency (embryos transferred/piglets born) of our cloning protocol was 1.9% for all transfers and 4.6% for animals that gave birth.
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收藏
页码:327 / 331
页数:5
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