Development of germ cell transplants in mice

Development of spermatogonial transplants was studied by using 5- to 6-wk-old histocompatible mice as cell donors and sterile (W-locus) mice as recipients. Groups of animals transplanted with germ cell suspensions were killed at 10 min, 9 h, 24 h, 1 wk, 1 mo, 2 mo, and 3 mo along with age-matched â...

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Bibliographic Details
Published in:	Biology of reproduction Vol. 59; no. 6; pp. 1360 - 1370
Main Authors:	Parreira, G.G. (Southern Illinois University School of Medicine, Carbondale, IL.), Ogawa, T, Avarbock, M.R, Franca, L.R, Brinster, R.L, Russell, L.D
Format:	Journal Article
Language:	English
Published:	Madison, WI Society for the Study of Reproduction 01-12-1998
Subjects:	ANIMAL TRANSGENIQUE ANIMALES TRANSGENICOS Animals Biological and medical sciences Clone Cells EPIDIDYMIS Epididymis - cytology ESPERMATOGENESIS ESPERMATOZOO Fundamental and applied biological sciences. Psychology GAMETE GAMETES GAMETOS Male Mammalian male genital system MICE Morphology. Physiology Organ Size PESO Phagocytosis POIDS RATON Seminiferous Epithelium - cytology SEMINIFEROUS TUBULES Sertoli Cells - physiology SOURIS SPERMATIDS SPERMATOCYTES Spermatocytes - cytology SPERMATOGENESE SPERMATOGENESIS SPERMATOGONIA Spermatogonia - physiology Spermatogonia - transplantation SPERMATOZOA SPERMATOZOIDE TESTES TESTICULE TESTICULOS Testis - cytology TRANSGENIC ANIMALS TRANSPLANTATION TRASPLANTES Vertebrates: reproduction WEIGHT Spermatogenesis Rodentia Male genital duct Transplantation Germinal cell Testicle Male genital system Vertebrata Epididymis Mammalia Mouse Spermatogonia Development
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Summary:	Development of spermatogonial transplants was studied by using 5- to 6-wk-old histocompatible mice as cell donors and sterile (W-locus) mice as recipients. Groups of animals transplanted with germ cell suspensions were killed at 10 min, 9 h, 24 h, 1 wk, 1 mo, 2 mo, and 3 mo along with age-matched âstartâ and âendâ W-locus controls. Weight of testes increased significantly at 24 h through 3 mo after germ cell transplantation, suggesting that the infused cells quickly stimulated organ function. Small clones of young spermatocytes were evident at 1 mo and sperm at 2 mo. The percentage of tubular profiles containing active spermatogenesis originating from spermatogonia increased with time (0.8% at 1 mo, 8.9% at 2 mo, and 28.2% at 3 mo). Most transplanted germ cells were eliminated from the seminiferous epithelium through phagocytosis by Sertoli cells that occurred primarily before 1 wk, although some pachytene cells were able to proceed through meiosis by 1 wk. A variety of abnormal features are described that characterize developing spermatogenesis in the transplanted testis. Spermatogenesis improved quantitatively and qualitatively with time although released sperm were frequently engulfed by intratubular macrophages and Sertoli cells. A quantitative analysis of spermatogenesis from transplanted germ cells will serve as a basis for improving spermatogonial transplant efficiency.
Bibliography:	1997095116 L10 L53
ISSN:	0006-3363 1529-7268
DOI:	10.1095/biolreprod59.6.1360