In Vitro Generation of Haploid Germ Cells from Human XY and XXY Immature Testes in a 3D Organoid System

Author:

Galdon Guillermo12ORCID,Zarandi Nima Pourhabibi13ORCID,Deebel Nicholas A.14ORCID,Zhang Sue15,Cornett Olivia1,Lyalin Dmitry67,Pettenati Mark J.6,Lue YanHe8ORCID,Wang Christina8,Swerdloff Ronald8,Shupe Thomas D.1,Bishop Colin1,Stogner Kimberly16,Kogan Stanley J.1,Howards Stuart14,Atala Anthony14ORCID,Sadri-Ardekani Hooman146ORCID

Affiliation:

1. Wake Forest Institute for Regenerative Medicine (WFIRM), Wake Forest School of Medicine, Winston-Salem, NC 27101, USA

2. Facultad de Medicina, Universidad de Barcelona, 08036 Barcelona, Spain

3. Department of Internal Medicine, University of Pittsburgh Medical Center, Harrisburg, PA 17101, USA

4. Department of Urology, Wake Forest School of Medicine, Winston-Salem, NC 27157, USA

5. Department of Biomedical Engineering, Boston University, Boston, MA 02215, USA

6. Department of Pathology, Wake Forest School of Medicine, Winston-Salem, NC 27157, USA

7. Department of Pathology, Molecular Diagnostics Division, Virginia Commonwealth University, Richmond, VA 23284, USA

8. Division of Endocrinology, Department of Medicine, The Lundquist Institute, Harbor-University of California Los Angeles (UCLA) Medical Center, Los Angeles, CA 90502, USA

Abstract

Increasing survival rates of children following cancer treatment have resulted in a significant population of adult survivors with the common side effect of infertility. Additionally, the availability of genetic testing has identified Klinefelter syndrome (classic 47,XXY) as the cause of future male infertility for a significant number of prepubertal patients. This study explores new spermatogonia stem cell (SSC)-based fertility therapies to meet the needs of these patients. Testicular cells were isolated from cryopreserved human testes tissue stored from XY and XXY prepubertal patients and propagated in a two-dimensional culture. Cells were then incorporated into a 3D human testicular organoid (HTO) system. During a 3-week culture period, HTOs maintained their structure, viability, and metabolic activity. Cell-specific PCR and flow cytometry markers identified undifferentiated spermatogonia, Sertoli, Leydig, and peritubular cells within the HTOs. Testosterone was produced by the HTOs both with and without hCG stimulation. Upregulation of postmeiotic germ cell markers was detected after 23 days in culture. Fluorescence in situ hybridization (FISH) of chromosomes X, Y, and 18 identified haploid cells in the in vitro differentiated HTOs. Thus, 3D HTOs were successfully generated from isolated immature human testicular cells from both euploid (XY) and Klinefelter (XXY) patients, supporting androgen production and germ cell differentiation in vitro.

Funder

Urology Care Foundation Research Scholar Award Program

American Urological Association Southeastern Section

Publisher

MDPI AG

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