Eliminating malignant contamination from therapeutic human spermatogonial stem cells
Serena L. Dovey, … , Joseph S. Sanfilippo, Kyle E. Orwig
Serena L. Dovey, … , Joseph S. Sanfilippo, Kyle E. Orwig
Published March 15, 2013
Citation Information: J Clin Invest. 2013;123(4):1833-1843. https://doi.org/10.1172/JCI65822.
View: Text | PDF
Technical Advance

Eliminating malignant contamination from therapeutic human spermatogonial stem cells

Abstract

Spermatogonial stem cell (SSC) transplantation has been shown to restore fertility in several species and may have application for treating some cases of male infertility (e.g., secondary to gonadotoxic therapy for cancer). To ensure safety of this fertility preservation strategy, methods are needed to isolate and enrich SSCs from human testis cell suspensions and also remove malignant contamination. We used flow cytometry to characterize cell surface antigen expression on human testicular cells and leukemic cells (MOLT-4 and TF-1a). We demonstrated via FACS that EpCAM is expressed by human spermatogonia but not MOLT-4 cells. In contrast, HLA-ABC and CD49e marked >95% of MOLT-4 cells but were not expressed on human spermatogonia. A multiparameter sort of MOLT-4–contaminated human testicular cell suspensions was performed to isolate EpCAM+/HLA-ABC/CD49e (putative spermatogonia) and EpCAM/HLA-ABC+/CD49e+ (putative MOLT-4) cell fractions. The EpCAM+/HLA-ABC/CD49e fraction was enriched for spermatogonial colonizing activity and did not form tumors following human-to–nude mouse xenotransplantation. The EpCAM/HLA-ABC+/CD49e+ fraction produced tumors following xenotransplantation. This approach could be generalized with slight modification to also remove contaminating TF-1a leukemia cells. Thus, FACS provides a method to isolate and enrich human spermatogonia and remove malignant contamination by exploiting differences in cell surface antigen expression.

Authors

Serena L. Dovey, Hanna Valli, Brian P. Hermann, Meena Sukhwani, Julia Donohue, Carlos A. Castro, Tianjiao Chu, Joseph S. Sanfilippo, Kyle E. Orwig

×

Figure 3

Human-to–nude mouse xenotransplant colonizing activity is enriched in the EpCAMlo fraction of human testis cells.

Options: View larger image (or click on image) Download as PowerPoint
Human-to–nude mouse xenotransplant colonizing activity is enriched in th...
Unsorted and EpCAM-sorted human testis cell fractions (see Figure 2) were transplanted into the testes of immune-deficient nude mice. Two months after transplant, colonies of human spermatogonia were identified in mouse recipient testes using the rabbit anti-primate testis antibody and Alexa Fluor 488–conjugated secondary antibody (green) (scale bar: 50 μm) (inset). Mouse seminiferous tubules are demarcated by dashed white lines. Colonies in each recipient testis were counted and normalized to 105 viable cells transplanted per testis. *P < 0.001, compared with unsorted cells. Bars indicate the mean number of colonies per 106 viable cells in each fraction. Error bars represent SEM from 3 replicate sorting experiments.