Single-cell multiomics sequencing reveals the reprogramming defects in embryos generated by round spermatid injection

Wang, Jing; Cai, Zhou; Gao, Shuai; Song, Xiuling; Yang, Xinyan; Fan, Jiaqi; Ren, Shaofang; Ma, Linzi; Zhao, Jiexiang; Cui, Manman; Song, Ke; Wang, Mei; Li, Chaohui; Zheng, Yi; Luo, Fang; Kai, Masahiro; Bai, Xia; Hutchins, Andrew P.; Li, Lin; Chang, Gang; Zhao, Xiaoyang

doi:10.1126/sciadv.abm3976

Cited by 4 publications

(2 citation statements)

References 79 publications

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“…To analyze the stage-specific gene expression at distinct antral follicle in sheep oocytes, the cDNA of 10 oocytes was synthesized using a reverse transcription system and amplified using the Single Cell Sequence Specific Amplification Kit (Vazyme, Nanjing, China; Cat#P621-01) according to the manufacturer's instructions [85]. qPCR was conducted with the TB Green ® Premix Ex Taq™ II (Tli RNaseH Plus) (Cat#RR820L) on a StepOnePlus Real-Time PCR System (Thermo Fisher Scientific).…”

Section: Reverse Transcription and Qpcrmentioning

confidence: 99%

Single-Cell Transcriptome Analysis Reveals Development-Specific Networks at Distinct Synchronized Antral Follicle Sizes in Sheep Oocytes

Song,

Zhang,

Zhang

et al. 2024

IJMS

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The development of the ovarian antral follicle is a complex, highly regulated process. Oocytes orchestrate and coordinate the development of mammalian ovarian follicles, and the rate of follicular development is governed by a developmental program intrinsic to the oocyte. Characterizing oocyte signatures during this dynamic process is critical for understanding oocyte maturation and follicular development. Although the transcriptional signature of sheep oocytes matured in vitro and preovulatory oocytes have been previously described, the transcriptional changes of oocytes in antral follicles have not. Here, we used single-cell transcriptomics (SmartSeq2) to characterize sheep oocytes from small, medium, and large antral follicles. We characterized the transcriptomic landscape of sheep oocytes during antral follicle development, identifying unique features in the transcriptional atlas, stage-specific molecular signatures, oocyte-secreted factors, and transcription factor networks. Notably, we identified the specific expression of 222 genes in the LO, 8 and 6 genes that were stage-specific in the MO and SO, respectively. We also elucidated signaling pathways in each antral follicle size that may reflect oocyte quality and in vitro maturation competency. Additionally, we discovered key biological processes that drive the transition from small to large antral follicles, revealing hub genes involved in follicle recruitment and selection. Thus, our work provides a comprehensive characterization of the single-oocyte transcriptome, filling a gap in the mapping of the molecular landscape of sheep oogenesis. We also provide key insights into the transcriptional regulation of the critical sizes of antral follicular development, which is essential for understanding how the oocyte orchestrates follicular development.

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Section: Reverse Transcription and Qpcrmentioning

confidence: 99%

Single-Cell Transcriptome Analysis Reveals Development-Specific Networks at Distinct Synchronized Antral Follicle Sizes in Sheep Oocytes

Song,

Zhang,

Zhang

et al. 2024

IJMS

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“…Scriptaid treatment (250 mM, 10 h) of mouse ROSI embryos at the pronucleus stage more enhanced blastocyst formation and delivery rates restoring gene expression and abnormal DNA methylation. 21 Wang et al 100 recently found that a compound “A366” which were selected by screening of the epigenetic modification‐related small compound library was effective on normal development and delivery of mouse ROSI embryos improving epigenetic abnormalities (300 nM, 20 h). As Hosseini and Salehi, 99 confirmed, very brief exposure of round spermatids to these compounds may be equally effective and reduce predictable risks.…”

Section: Recovery Of Poor Rosi Embryo Developmentmentioning

confidence: 99%

How to improve the clinical outcome of round spermatid injection (ROSI) into the oocyte: Correction of epigenetic abnormalities

Tanaka

Watanabe

2023

Reprod Medicine & Biology

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Background First successful human round spermatid injection (ROSI) was conducted by Tesarik et al. in 1996 for the sole treatment of nonobstructive azoospermic men whose most advanced spermatogenic cells were elongating round spermatids. Nine offsprings from ROSI were reported between 1996 and 2000. No successful deliveries were reported for 15 years after that. Tanaka et al. reported 90 babies born after ROSI and their follow‐up studies in 2015 and 2018 showed no significant differences in comparison with those born after natural conception in terms of physical and cognitive abilities. However, clinical outcomes remain low. Method Clinical and laboratory data of successful cases in the precursor ROSI groups and those of Tanaka et al. were reviewed. Results Differences were found between the two groups in terms of identification of characteristics of round spermatid and oocyte activation. Additionally, epigenetic abnormalities were identified as underlying causes for poor ROSI results, besides correct identification of round spermatid and adequate oocyte activation. Correction of epigenetic errors could lead to optimal embryonic development. Conclusion Correction of epigenetic abnormalities has a probability to improve the clinical outcome of ROSI.

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Single-cell multi-omics sequencing of human spermatogenesis reveals a DNA demethylation event associated with male meiotic recombination

Huang,

Li,

et al. 2023

Nat Cell Biol

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Single-cell multiomics sequencing reveals the reprogramming defects in embryos generated by round spermatid injection

Cited by 4 publications

References 79 publications

Single-Cell Transcriptome Analysis Reveals Development-Specific Networks at Distinct Synchronized Antral Follicle Sizes in Sheep Oocytes

Single-Cell Transcriptome Analysis Reveals Development-Specific Networks at Distinct Synchronized Antral Follicle Sizes in Sheep Oocytes

How to improve the clinical outcome of round spermatid injection (ROSI) into the oocyte: Correction of epigenetic abnormalities

Single-cell multi-omics sequencing of human spermatogenesis reveals a DNA demethylation event associated with male meiotic recombination

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