Vitrification with Dimethyl Sulfoxide Induces Transcriptomic Alteration of Gene and Transposable Element Expression in Immature Human Oocytes

Ashley Wiltshire; Renata Schaal; Fang Wang; Tiffany Tsou; Wilson McKerrow; David Keefe

doi:10.3390/genes14061232

Vitrification with Dimethyl Sulfoxide Induces Transcriptomic Alteration of Gene and Transposable Element Expression in Immature Human Oocytes

Genes (Basel). 2023 Jun 8;14(6):1232. doi: 10.3390/genes14061232.

Authors

Ashley Wiltshire¹, Renata Schaal¹, Fang Wang¹, Tiffany Tsou², Wilson McKerrow², David Keefe¹

Affiliations

¹ Department of Obstetrics and Gynecology, Division of Reproductive Endocrinology and Infertility, New York University Langone Fertility Center, 660 1st Avenue, New York, NY 10016, USA.
² Institute for Systems Genetics, New York University Langone Medical Center, 550 1st Avenue, New York, NY 10016, USA.

Abstract

Despite substantial advancements in the field of cryobiology, oocyte and embryo cryopreservation still compromise developmental competence. Furthermore, dimethyl sulfoxide (DMSO), one of the most commonly used cryoprotectants, has been found to exert potent effects on the epigenetic landscape of cultured human cells, as well as mouse oocytes and embryos. Little is known about its impact on human oocytes. Additionally, few studies investigate the effects of DMSO on transposable elements (TE), the control of which is essential for the maintenance of genomic instability. The objective of this study was to investigate the impact of vitrification with DMSO-containing cryoprotectant on the transcriptome, including on TEs, of human oocytes. Twenty-four oocytes at the GV stage were donated by four healthy women undergoing elective oocyte cryopreservation. Oocytes were paired such that half from each patient were vitrified with DMSO-containing cryoprotectant (Vitrified Cohort), while the other half were snap frozen in phosphate buffer, unexposed to DMSO (Non-Vitrified Cohort). All oocytes underwent RNA sequencing via a method with high fidelity for single cell analysis, and which allows for the analysis of TE expression through Switching Mechanism at the 5'-end of the RNA Transcript sequencing 2 (SMARTseq2), followed by functional enrichment analysis. Of the 27,837 genes identified by SMARTseq2, 7331 (26.3%) were differentially expressed (p < 0.05). There was a significant dysregulation of genes involved in chromatin and histone modification. Mitochondrial function, as well as the Wnt, insulin, mTOR, HIPPO, and MAPK signaling pathways were also altered. The expression of TEs was positively correlated with the expression of PIWIL2, DNMT3A, and DNMT3B, and negatively correlated with age. These findings suggest that the current standard process of oocyte vitrification, involving DMSO-containing cryoprotectant, induces significant transcriptome changes, including those involving TEs.

Keywords: DMSO; dimethyl sulfoxide; epigenetics; gene expression; germinal vesicle; oocytes; vitrification.

Publication types

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

MeSH terms

Animals
Argonaute Proteins
Cryopreservation / methods
Cryoprotective Agents / pharmacology
DNA Transposable Elements / genetics
Dimethyl Sulfoxide* / pharmacology
Female
Humans
Mice
Oocytes
Transcriptome
Vitrification*

Substances

Dimethyl Sulfoxide
DNA Transposable Elements
Cryoprotective Agents
PIWIL2 protein, human
Argonaute Proteins

Grants and funding

This study was funded by the Stanley H. Kaplan fund.