Successful cross-breeding of cloned pigs expressing endo-β-galactosidase C and human decay accelerating factor

• Published in: Xenotransplantation (Københaven) Vol. 16; no. 6; pp. 511 - 521
• Main Authors: Yazaki, Satoko, Iwamoto, Masaki, Onishi, Akira, Miwa, Yuko, Suzuki, Shunichi, Fuchimoto, Dai-ichiro, Sembon, Shoichiro, Furusawa, Tadashi, Hashimoto, Michiko, Oishi, Takatsugu, Liu, DaGe, Nagasaka, Takaharu, Kuzuya, Takafumi, Maruyama, Shoichi, Ogawa, Haruko, Kadomatsu, Kenji, Uchida, Kazuharu, Nakao, Akimasa, Kobayashi, Takaaki
• Format: Journal Article
• Language: English
• Published: Oxford, UK Blackwell Publishing Ltd 01.11.2009
• Subjects: alpha-Galactosidase - genetics; alpha-Galactosidase - metabolism; Animals; Animals, Genetically Modified - genetics; Animals, Genetically Modified - metabolism; CD55 Antigens - genetics; CD55 Antigens - metabolism; Cells, Cultured; cloned pig; Cloning, Organism; crossbreeding; endo-β-galactosidase C; Endothelial Cells - cytology; Endothelial Cells - metabolism; Female; Fibroblasts - cytology; Fibroblasts - metabolism; Glycoside Hydrolases - genetics; Glycoside Hydrolases - metabolism; human DAF; Humans; Hybridization, Genetic; Male; Nuclear Transfer Techniques; Papio; Pedigree; Sus scrofa; Transgenes; Transplantation, Heterologous
• ISSN: 0908-665X; 1399-3089
• DOI: 10.1111/j.1399-3089.2009.00549.x

Yazaki S, Iwamoto M, Onishi A, Miwa Y, Suzuki S, Fuchimoto D, Sembon S, Furusawa T, Hashimoto M, Oishi T, Liu D, Nagasaka T, Kuzuya T, Maruyama S, Ogawa H, Kadomatsu K, Uchida K, 
Nakao A, Kobayashi T. Successful cross‐breeding of cloned pigs expressing endo‐β‐galactosidase C and human decay accelerating factor. Xenotransplantation 2009; 16: 511–521. © 2009 John Wiley & Sons A/S. : Background:  For successful organ xenotransplantation, genetically engineered pigs have been actively produced. Our attention has focused on (i) reduction of αGal expression by its digestion enzyme, endo‐β‐galactosidase C (EndoGalC), and (ii) inhibition of complement activation by human decay accelerating factor (hDAF). Cell sorting and nuclear transfer enabled the effective production of cloned pigs expressing transgene at high levels. We report the successful cross‐breeding of pigs expressing EndoGalC and hDAF. Methods:  After hDAF and EndoGalC genes were transfected into pig fibroblasts from the fetus of Landrace × Yorkshire and Meishan, respectively, transfected cells expressing transgenes effectively were collected using a cell sorter. Cloned pigs were produced using the technology of somatic cell nuclear transfer. After cross‐breeding of cloned pigs, kidneys expressing both EndoGalC and hDAF were transplanted into baboons to examine the efficacy of gene transduction. Results:  Well‐designed cloned pigs were produced by cross‐breeding. αGal expression levels in cloned pigs were reduced up to 2 to 14%, compared to that in wild‐type pigs. hDAF expression reached about 10‐ to 70‐fold, compared to that in human umbilical vein endothelial cells. No congenital deformity was observed. There was no problem of increased stillbirth rate or growth retardation. Hyperacute rejection could be avoided in such a cloned pig to baboon kidney transplantation without any treatment for anti‐pig antibody removal. However, grafts suffered from fibrin deposition as early as 1 h after transplantation, and were rejected after 1 week. Conclusions:  Using a cell sorting system for effective collection of transfected cells, two types of cloned pigs were produced with a very high level of hDAF expression and a low level of αGal expression. Such genetic modification was effective in preventing hyperacute rejection, but there was an immediate lapse into procoagulation after transplantation, resulting in acute vascular rejection. Effective suppression of antibody binding to the graft would be necessary, even if a high level of hDAF is expressed.