Complete meiosis in rat prepubertal testicular tissue under in vitro sequential culture conditions

Justine Saulnier; Mathilde Soirey; Nasreddine Kébir; Marion Delessard; Aurélie Rives-Feraille; Laura Moutard; Ludovic Dumont; Nathalie Rives; Christine Rondanino

doi:10.1111/andr.13325

Complete meiosis in rat prepubertal testicular tissue under in vitro sequential culture conditions

Andrology. 2023 Jan;11(1):167-176. doi: 10.1111/andr.13325. Epub 2022 Nov 22.

Authors

Justine Saulnier¹, Mathilde Soirey¹, Nasreddine Kébir², Marion Delessard¹, Aurélie Rives-Feraille¹, Laura Moutard¹, Ludovic Dumont¹, Nathalie Rives¹, Christine Rondanino¹

Affiliations

¹ INSERM, U1239, Adrenal and Gonadal Pathophysiology team, Laboratory of Neuroendocrine Endocrine and Germinal Differentiation and Communication, Rouen University Hospital, Rouen Normandy University, Rouen, France.
² Normandie Univ, INSA Rouen Normandie, Laboratoire PBS, Saint-Etienne-du-Rouvray, France.

Abstract

Background: Testicular tissue cryopreservation before gonadotoxic treatments allows fertility preservation in children suffering from cancer. Fertility restoration strategies, in particular in vitro maturation of prepubertal testicular tissue, are being developed mainly in animal models. The rat, widely used in biomedical research, including in reproductive biology, is a relevant model.

Objectives: To determine whether sequential two-step culture protocols can improve the efficiency of rat in vitro spermatogenesis.

Materials and methods: Rat prepubertal testicular tissues were cultured on agarose gels with either a one-step or two-step protocol with or without polydimethylsiloxane (PDMS) ceiling chips. The progression of spermatogenesis, germ/Sertoli cell ratio, cell proliferation, seminiferous tubule area, and intratubular cell density were assessed by histological and immunohistochemical analyses. Terminal deoxynucleotidyl transferase-mediated dUTP nick-end labeling (TUNEL) assays and Peanut Agglutinin (PNA) lectin labeling were performed to analyze the Deoxyribonucleic Acid (DNA) integrity and differentiation step of in vitro-produced spermatids.

Results: Sequential two-step protocols allowed the production of spermatids with a higher efficiency compared with the one-step culture protocol. However, the efficiency was low, as less than 1.5% of tubules contained spermatids. Most of the in vitro-produced spermatids contained unfragmented DNA and were at an early step of differentiation. Rare elongating spermatids could be detected in the cultured explants. Although complete in vitro spermatogenesis could not be obtained with PDMS ceiling chips, entry into meiosis was promoted in one-step organotypic cultures.

Discussion and conclusion: Complete in vitro meiosis and the beginning of the elongation phase of spermiogenesis were obtained in a rat model using sequential culture methods. Because of their low efficiency, further work will be necessary to identify the culture conditions allowing the completion of spermiogenesis. These optimizations could pave the way for future applications, including the development of an in vitro fertility restoration procedure for childhood cancer survivors, which is still far from being clinically available.

Keywords: in vitro organ culture; meiosis; sequential condition; spermatogenesis; testis.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Animals
DNA
Male
Meiosis
Rats
Seminiferous Tubules*
Spermatogenesis / genetics
Testis*

Substances

DNA