An Efficient Method for Producing α(1,3)-Galactosyltransferase Gene Knockout Pigs

We have reported relatively efficient methods for somatic cell nuclear transfer and for knocking out the α(1,3)-galactosyltransferase (α1,3-GT) gene in porcine fetal fibroblasts using a nonisogenic promoterless construct approach. Here we report the production of α1,3-GT gene knockout pigs using these procedures. Seven α1,3-GT gene knockout cell clones were identified by long-range PCR from 108 neomycin resistant (neoR) 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. α1,3-GT gene knockout pigs were identified by long-range PCR...