Revealing stage-specific expression patterns of long noncoding RNAs along mouse spermatogenesis

Trovero, María F.; Rodríguez-Casuriaga, Rosana; Romeo, Carlos; Santiñaque, Federico F.; François, Mateo; Folle, Gustavo A.; Benavente, Ricardo; Sotelo‐Silveira, José; Geisinger, Adriana

doi:10.1080/15476286.2019.1700332

Cited by 31 publications

(32 citation statements)

References 86 publications

(196 reference statements)

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“…In our laboratory, we have developed a protocol for the purification of testicular cell populations by FACS using Vybrant DyeCycle Green, a non-cytotoxic vital dye with the advantage over Hoechst 33342 that it is excited with a blue laser thus avoiding the need of a UV laser, which in turn minimizes potential damage to nucleic acids caused by UV light exposure ( Rodríguez-Casuriaga et al, 2014 ; Geisinger and Rodríguez-Casuriaga, 2017 ). This protocol allowed the profiling of coding transcripts and lncRNAs along spermatogenesis through RNAseq, using highly pure (>95%) stage-specific cell populations ( da Cruz et al, 2016 ; Trovero et al, 2020 ). These studies included the L/Z cell population, thus enabling for the first time to compare the transcriptomic profiles, as obtained through NGS, between early and medium/late meiotic prophase, and providing information on gene expression fluctuations along meiotic prophase ( da Cruz et al, 2016 ).…”

Section: Strategies For the Obtainment Of Meiotic Cells For Rnaseqmentioning

confidence: 99%

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Transcriptomics of Meiosis in the Male Mouse

Geisinger

Rodríguez-Casuriaga

Benavente

2021

Front. Cell Dev. Biol.

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Molecular studies of meiosis in mammals have been long relegated due to some intrinsic obstacles, namely the impossibility to reproduce the process in vitro, and the difficulty to obtain highly pure isolated cells of the different meiotic stages. In the recent years, some technical advances, from the improvement of flow cytometry sorting protocols to single-cell RNAseq, are enabling to profile the transcriptome and its fluctuations along the meiotic process. In this mini-review we will outline the diverse methodological approaches that have been employed, and some of the main findings that have started to arise from these studies. As for practical reasons most studies have been carried out in males, and mostly using mouse as a model, our focus will be on murine male meiosis, although also including specific comments about humans. Particularly, we will center on the controversy about gene expression during early meiotic prophase; the widespread existing gap between transcription and translation in meiotic cells; the expression patterns and potential roles of meiotic long non-coding RNAs; and the visualization of meiotic sex chromosome inactivation from the RNAseq perspective.

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Section: Strategies For the Obtainment Of Meiotic Cells For Rnaseqmentioning

confidence: 99%

“…GC, gonocytes; SPG, spermatogonia; PL, preleptotene; L, leptotene; Z, zygotene; PS, pachytene; D, diplotene; M, meiotic divisions; 1–16 represent the different spermatid stages. Adapted from Trovero et al (2020) , under the Creative Commons Attribution License.…”

Section: The Lag Between Transcription and Translationmentioning

confidence: 99%

Transcriptomics of Meiosis in the Male Mouse

Geisinger

Rodríguez-Casuriaga

Benavente

2021

Front. Cell Dev. Biol.

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“… 6 Recently, numerous lncRNAs have been identified in humans and other organisms that play diverse roles in regulating various phenomenon, such as cell proliferation and apoptosis, 7 , 8 cell development, 9 cell differentiation, 10 and development of certain diseases. 11 , 12 Specifically, lncRNAs are involved in regulating spermatogenesis, 13 , 14 steroidogenesis, 15 embryo implantation 16 and development, 17 follicular development, 18 oocyte maturation, 19 GC apoptosis and proliferation, 20 , 21 and reproductive diseases, 22 , 23 suggesting their importance in reproduction. 24 However, only a few lncRNAs have been identified in domestic animals.…”

Section: Introductionmentioning

confidence: 99%

lncRNA FDNCR promotes apoptosis of granulosa cells by targeting the miR-543-3p/DCN/TGF-β signaling pathway in Hu sheep

Yao

Gao

Bao

et al. 2021

Molecular Therapy - Nucleic Acids

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Long non-coding RNAs (lncRNAs) regulate the development of follicles and reproductive diseases, but the mechanisms by which lncRNAs regulate ovarian functions and fertility remain elusive. We profiled the expression of lncRNAs in ovarian tissues of Hu sheep with different prolificacy and identified 21,327 lncRNAs. Many of the lncRNAs were differentially expressed in different groups. We further characterized an lncRNA that was predominantly expressed in the ovaries of the low prolificacy Fec B+ (LPB+) group and mainly present in granulosa cells (GCs), and the expression of this lncRNA decreased during follicular development, which we named follicular development-associated lncRNA ( FDNCR ). Next, we found that FDNCR directly binds miR-543-3p, and decorin ( DCN ) was identified as a target of miR-543-3p. FDNCR overexpression promoted GC apoptosis through increased expression of DCN , which could be attenuated by miR-543-3p. Furthermore, miR-543-3p increased and FDNCR reduced the expression of transforming growth factor-β (TGF-β) pathway-related genes, including TGF-β1 and inhibin beta A ( INHBA ), which were upregulated upon DCN silencing. Our results demonstrated that FDNCR sponges miR-543-3p in GCs and prevents miR-543-3p from binding to the DCN 3′ UTR, resulting in DCN transactivation and TGF-β pathway inhibition and promotion of GC apoptosis in Hu sheep. These findings provide insights into the mechanisms underlying prolificacy in sheep.

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“…More recently, we applied our VDG-based sorting protocol [ 49 , 50 ] for RNA seq of four testicular cell populations, including two meiotic prophase I populations (L/Z and P/D) (see Figure 2 B). The high purity of the sorted fractions (>95%), combined with RNAseq technology, enabled accurately establishment of the transcriptome fluctuations along spermatogenesis, both for coding and for long non-coding transcripts (lncRNAs) [ 94 , 95 ]. Moreover, the purification of the L/Z population allowed for the first time the comparison of the RNAseq-derived transcriptomes of early meiotic prophase I (in which essential events such as homologous chromosome alignment and pairing occur) and medium/late meiotic prophase cells (in which crossing over takes place) [ 94 ].…”

Section: Fcm As a Preparative Tool In Spermatogenic Studiesmentioning

confidence: 99%

Contributions of Flow Cytometry to the Molecular Study of Spermatogenesis in Mammals

Rodríguez-Casuriaga

Geisinger

2021

IJMS

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Mammalian testes are very heterogeneous organs, with a high number of different cell types. Testicular heterogeneity, together with the lack of reliable in vitro culture systems of spermatogenic cells, have been an obstacle for the characterization of the molecular bases of the unique events that take place along the different spermatogenic stages. In this context, flow cytometry has become an invaluable tool for the analysis of testicular heterogeneity, and for the purification of stage-specific spermatogenic cell populations, both for basic research and for clinical applications. In this review, we highlight the importance of flow cytometry for the advances on the knowledge of the molecular groundwork of spermatogenesis in mammals. Moreover, we provide examples of different approaches to the study of spermatogenesis that have benefited from flow cytometry, including the characterization of mutant phenotypes, transcriptomics, epigenetic and genome-wide chromatin studies, and the attempts to establish cell culture systems for research and/or clinical aims such as infertility treatment.

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Revealing stage-specific expression patterns of long noncoding RNAs along mouse spermatogenesis

Cited by 31 publications

References 86 publications

Transcriptomics of Meiosis in the Male Mouse

Transcriptomics of Meiosis in the Male Mouse

lncRNA FDNCR promotes apoptosis of granulosa cells by targeting the miR-543-3p/DCN/TGF-β signaling pathway in Hu sheep

Contributions of Flow Cytometry to the Molecular Study of Spermatogenesis in Mammals

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