MicroRNA Analysis of In Vitro Differentiation of Spermatogonial Stem Cells Using a 3D Human Testis Organoid System-Reference-Cited by-同舟云学术

MicroRNA Analysis of In Vitro Differentiation of Spermatogonial Stem Cells Using a 3D Human Testis Organoid System

Published:2024-08-06 Issue:8 Volume:12 Page:1774
ISSN:2227-9059
Container-title:Biomedicines
language:en
Short-container-title:Biomedicines

Author:

Cohen Adam B.¹²^ORCID,Nikmehr Banafsheh¹³^ORCID,Abdelaal Omar A.¹⁴,Escott Megan¹²,Walker Stephen J.¹^ORCID,Atala Anthony¹²^ORCID,Sadri-Ardekani Hooman¹²³^ORCID

Affiliation:

1. Wake Forest Institute of Regenerative Medicine, Winston-Salem, NC 27101, USA

2. Department of Urology, Atrium Health Wake Forest Baptist, Winston-Salem, NC 27157, USA

3. Carolinas Fertility Institute, Winston-Salem, NC 27103, USA

4. Department of Urology, Faculty of Medicine, Zagazig University, Zagazig 7120001, Egypt

Abstract

Spermatogenesis produces male gametes from spermatogonial stem cells (SSC), beginning at puberty. Modern-day laboratory techniques allow for the long-term culture of SSC and in vitro spermatogenesis. The specific biochemical processes that occur during spermatogenesis remain poorly understood. One particular element of spermatogenesis that has yet to be characterized is the role of microRNAs (miRNA), short, non-transcribed RNAs that act as post-translational regulators of gene activity. In this study, we seek to describe the presence of miRNA in a two-dimensional (2D) SSC culture and a 3D human testis organoid (HTO) system. Testicular cells were isolated from the frozen tissue of three brain-dead subjects, propagated in cultures for four to five weeks, and used to form 3D HTOs. Following organoid formation, differentiation of testicular cells was induced. RNA was isolated from the whole testis tissue (WT) showing in vivo conditions, HTO Day Zero (2D SSC culture), Day 2 HTOs, and Day 23 differentiated HTOs, then analyzed for changes in miRNA expression using the Nanostring nCounter miRNA panel. One hundred ninety-five miRNAs met the criteria for expression in WT, 186 in 2D culture, 190 in Day 2 HTOs, and 187 in differentiated HTOs. One hundred thirty-three miRNAs were common across all conditions, and 41, 17, 6, and 11 miRNAs were unique for WT, 2D culture, Day 2 HTOs, and differentiated HTOs, respectively. Twenty-two miRNAs were similar between WT and differentiated HTOS. We evaluated the miRNA expression profiles of progressively complex stages of testicular cell culture, culminating in a 3D organoid model capable of meiotic differentiation, and compared these to WT. We identified a great variance between the native tissue and the culture system; however, some miRNAs are preserved. These data may provide avenues for deeper understanding of spermatogenesis and the ability to improve this process in the laboratory. Research on miRNA continues to be an essential avenue for understanding human spermatogenesis.

Funder

Wake Forest Institute of Regenerative Medicine

NIH

Publisher

MDPI AG

Link

https://www.mdpi.com/2227-9059/12/8/1774/pdf

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