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Reproduction (2007) 134 767-779
DOI: 10.1530/REP-07-0240
Copyright © 2007 Society for Reproduction and Fertility
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RESEARCH

Decontamination of leukemic cells and enrichment of germ cells from testicular samples from rats with Roser’s T-cell leukemia by flow cytometric sorting

Mi Hou1, Margareta Andersson3, Chengyun Zheng2,4, Anne Sundblad3, Olle Söder1 and Kirsi Jahnukainen1,5

1 Department of Woman and Child Health, Astrid Lindgren Children’s Hospital, Pediatric Endocrinology Unit, Q2:08 and 2 Children’s Cancer Research Unit, Karolinska Insitutet and University Hospital, SE-171 76 Stockholm, Sweden, 3 Department of Medicine, Division of Hematology, Karolinska Institutet and University Hospital, Stockholm, Sweden, 4 Second Hospital of ShanDong University, Jinan, China and 5 Departments of Pediatrics and Physiology, University of Turku, Turku, Finland

Correspondence should be addressed to M Hou; Email: mi.hou{at}ki.se

Testicular germ cell transplantation is a novel strategy for preservation of fertility in prepubertal cancer patients, but the risk of reseeding tumor cells into cured patients presently limits clinical application of this approach. To date, no systematic evaluation of the limitations of surface marker-based decontamination of testicular samples with acute lymphoblastic leukemia has been performed. Here, surface markers for leukemic (CD4 and major histocompatibility complex class I) and germ cells (epithelia cell adhesion molecule) in testicular samples infiltrated with Roser’s T-cell leukemia were identified. These markers were then used to delete leukemic cells and/or select for germ cells by flow cytometry (FACS). The resulting cell populations were analyzed by FACS, immunocytochemistry, or evaluation of leukemia transmission in syngeneic piebald variegated rats. Simple positive selection of germ cells or deletion of leukemic cells using specific surface markers was unable to effectively decontaminate testicular samples. The poor specificity of spermatogonial surface markers and aggregation of germ and leukemic cells limited the positive selection of germ cells, while immunophenotypic variation among lymphoblastic leukemia cells prevented adequate deletion of leukemic cells. Enzymatic treatment to disperse the testicular cells and feature of the intratesticular environment contributed to this immunophenotypic variation. Only germ cell selection in combination with leukemic cell deletion prevented leukemia transmission in association with intratesticular injection of the sorted cells. However, with such combined sorting, only 0.23% of the original testicular cells were recovered. With presently available techniques, flow cytometric purification of germ cells from a leukemic donor is not sufficiently effective or safe for clinical use.




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J.-B. Stukenborg, S. Schlatt, M. Simoni, C.-H. Yeung, M. A. Elhija, C. M. Luetjens, M. Huleihel, and J. Wistuba
New horizons for in vitro spermatogenesis? An update on novel three-dimensional culture systems as tools for meiotic and post-meiotic differentiation of testicular germ cells
Mol. Hum. Reprod., September 1, 2009; 15(9): 521 - 529.
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