Throughout in vitro first spermatogenic wave: Next-generation sequencing gene expression patterns of fresh and cryopreserved prepubertal mice testicular tissue explants

Ludovic Dumont; Ludovic Dumont; Hélène Lopez Maestre; Hélène Lopez Maestre; Frédéric Chalmel; Louise Huber; Louise Huber; Aurélie Rives-Feraille; Aurélie Rives-Feraille; Laura Moutard; Laura Moutard; Frédérique Bateux; Frédérique Bateux; Christine Rondanino; Christine Rondanino; Nathalie Rives; Nathalie Rives; Nathalie Rives

doi:10.3389/fendo.2023.1112834

Frontiers in Endocrinology (Mar 2023)

Throughout in vitro first spermatogenic wave: Next-generation sequencing gene expression patterns of fresh and cryopreserved prepubertal mice testicular tissue explants

Ludovic Dumont,
Ludovic Dumont,
Hélène Lopez Maestre,
Hélène Lopez Maestre,
Frédéric Chalmel,
Louise Huber,
Louise Huber,
Aurélie Rives-Feraille,
Aurélie Rives-Feraille,
Laura Moutard,
Laura Moutard,
Frédérique Bateux,
Frédérique Bateux,
Christine Rondanino,
Christine Rondanino,
Nathalie Rives,
Nathalie Rives,
Nathalie Rives

Affiliations

Ludovic Dumont: Univ Rouen Normandie, INSERM, NORDIC UMR 1239 – Team Adrenal and Gonadal Pathophysiology (AGoPath), Rouen, France
Ludovic Dumont: Normandie, Institute for Research and Innovation in Biomedicine (IRIB), Rouen, France
Hélène Lopez Maestre: Univ Rouen Normandie, INSERM, PANTHER UMR 1234, Rouen, France
Hélène Lopez Maestre: Institut Pasteur, Hub de Bioinformatique et Biostatistique – Département Biologie Computationnelle, USR 3756, CNRS, Paris, France
Frédéric Chalmel: University of Rennes 1, Inserm U1085-IRSET, Rennes, France
Louise Huber: Univ Rouen Normandie, INSERM, NORDIC UMR 1239 – Team Adrenal and Gonadal Pathophysiology (AGoPath), Rouen, France
Louise Huber: Normandie, Institute for Research and Innovation in Biomedicine (IRIB), Rouen, France
Aurélie Rives-Feraille: Univ Rouen Normandie, INSERM, NORDIC UMR 1239 – Team Adrenal and Gonadal Pathophysiology (AGoPath), Rouen, France
Aurélie Rives-Feraille: Normandie, Institute for Research and Innovation in Biomedicine (IRIB), Rouen, France
Laura Moutard: Univ Rouen Normandie, INSERM, NORDIC UMR 1239 – Team Adrenal and Gonadal Pathophysiology (AGoPath), Rouen, France
Laura Moutard: Normandie, Institute for Research and Innovation in Biomedicine (IRIB), Rouen, France
Frédérique Bateux: Univ Rouen Normandie, INSERM, NORDIC UMR 1239 – Team Adrenal and Gonadal Pathophysiology (AGoPath), Rouen, France
Frédérique Bateux: Normandie, Institute for Research and Innovation in Biomedicine (IRIB), Rouen, France
Christine Rondanino: Univ Rouen Normandie, INSERM, NORDIC UMR 1239 – Team Adrenal and Gonadal Pathophysiology (AGoPath), Rouen, France
Christine Rondanino: Normandie, Institute for Research and Innovation in Biomedicine (IRIB), Rouen, France
Nathalie Rives: Univ Rouen Normandie, INSERM, NORDIC UMR 1239 – Team Adrenal and Gonadal Pathophysiology (AGoPath), Rouen, France
Nathalie Rives: Normandie, Institute for Research and Innovation in Biomedicine (IRIB), Rouen, France
Nathalie Rives: Rouen University Hospital, Biology of Reproduction-CECOS laboratory, Rouen, France

DOI: https://doi.org/10.3389/fendo.2023.1112834
Journal volume & issue: Vol. 14

Abstract

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IntroductionSuitable cryopreservation procedures of pre-pubertal testicular tissue associated with efficient culture conditions are crucial in the fields of fertility preservation and restoration. In vitro spermatogenesis remains a challenging technical procedure to undergo a complete spermatogenesis.The number of haploid cells and more specifically the spermatic yield produced in vitro in mice is still extremely low compared to age-matched in vivo controls and this procedure has never yet been successfully transferred to humans.MethodsTo evaluate the impact of in vitro culture and freezing procedure, pre-pubertal testicular mice testes were directly cultured until day 4 (D4), D16 and D30 or cryopreserved by controlled slow freezing then cultured until D30. Testes composed of a panel of 6.5 dpp (days postpartum), 10.5 dpp, 22.5 dpp, and 36.5 dpp mice were used as in vivo controls. Testicular tissues were assessed by histological (HES) and immunofluorescence (stimulated by retinoic acid gene 8, STRA8) analyses. Moreover, a detailed transcriptome evaluation study has been carried out to study the gene expression patterns throughout the first in vitro spermatogenic wave.ResultsTranscriptomic analyses reveal that cultured tissues expression profiles are almost comparable between D16 and D30; highlighting an abnormal kinetic throughout the second half of the first spermatogenesis during in vitro cultures. In addition, testicular explants have shown dysregulation of their transcriptomic profile compared to controls with genes related to inflammation response, insulin-like growth factor and genes involved in steroidogenesis.DiscussionThe present work first shows that cryopreservation had very little impact on gene expression in testicular tissue, either directly after thawing or after 30 days in culture. Transcriptomic analysis of testis tissue samples is highly informative due to the large number of expressed genes and identified isoforms. This study provides a very valuable basis for future studies concerning in vitro spermatogenesis in mice.

Published in Frontiers in Endocrinology

ISSN: 1664-2392 (Online)
Publisher: Frontiers Media S.A.
Country of publisher: Switzerland
LCC subjects: Medicine: Internal medicine: Specialties of internal medicine: Diseases of the endocrine glands. Clinical endocrinology
Website: https://www.frontiersin.org/journals/endocrinology

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