Transcriptomic Analysis of Vitrified–Warmed vs. Fresh Mouse Blastocysts: Cryo-Induced Physiological Mechanisms and Implantation Impact

Chi-Ying Lee; Han-Ni Tsai; En-Hui Cheng; Tsung-Hsien Lee; Pin-Yao Lin; Maw-Sheng Lee; Chun-I Lee

doi:10.3390/ijms25168658

International Journal of Molecular Sciences (Aug 2024)

Transcriptomic Analysis of Vitrified–Warmed vs. Fresh Mouse Blastocysts: Cryo-Induced Physiological Mechanisms and Implantation Impact

Chi-Ying Lee,
Han-Ni Tsai,
En-Hui Cheng,
Tsung-Hsien Lee,
Pin-Yao Lin,
Maw-Sheng Lee,
Chun-I Lee

Affiliations

Chi-Ying Lee: Genetic Diagnosis Laboratory, Lee Women’s Hospital, Taichung 40652, Taiwan
Han-Ni Tsai: Genetic Diagnosis Laboratory, Lee Women’s Hospital, Taichung 40652, Taiwan
En-Hui Cheng: Genetic Diagnosis Laboratory, Lee Women’s Hospital, Taichung 40652, Taiwan
Tsung-Hsien Lee: Division of Infertility, Lee Women’s Hospital, Taichung 40402, Taiwan
Pin-Yao Lin: Post Baccalaureate Medicine, National Chung Hsing University, Taichung 40227, Taiwan
Maw-Sheng Lee: Division of Infertility, Lee Women’s Hospital, Taichung 40402, Taiwan
Chun-I Lee: Division of Infertility, Lee Women’s Hospital, Taichung 40402, Taiwan

DOI: https://doi.org/10.3390/ijms25168658
Journal volume & issue: Vol. 25, no. 16
p. 8658

Abstract

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Blastocyst vitrification has significantly improved embryo transfer methods, leading to higher implantation success rates and better pregnancy outcomes in subsequent frozen embryo transfer cycles. This study aimed to simulate the transcriptional changes caused by vitrifying human blastocysts using mouse blastocysts as a model and to further investigate these changes’ effects. Utilizing a human vitrification protocol, we implanted both vitrified and fresh embryos into mice. We observed the implantation success rates and performed transcriptomic analysis on the blastocysts. To validate the results from messenger RNA sequencing, we conducted reverse transcriptase-quantitative polymerase chain reaction (RT-qPCR) to measure the expression levels of specific genes. Based on mRNA profiling, we predicted the microRNAs responsible for the regulation and used qPCR basic microRNA assays for validation. Our observations revealed a higher implantation success rate for vitrified embryos than fresh embryos. Transcriptomic analysis showed that vitrified–warmed blastocysts exhibited differentially expressed genes (DEGs) primarily associated with thermogenesis, chemical carcinogenesis-reactive oxygen species, oxidative phosphorylation, immune response, and MAPK-related signaling pathways. RT-qPCR confirmed increased expression of genes such as Cdk6 and Nfat2, and decreased expression of genes such as Dkk3 and Mapk10. Additionally, gene-microRNA interaction predictions and microRNA expression analysis identified twelve microRNAs with expression patterns consistent with the predicted results, suggesting potential roles in uterine epithelial cell adhesion, trophectoderm development, invasive capacity, and immune responses. Our findings suggest that vitrification induces transcriptomic changes in mouse blastocysts, and even small changes in gene expression can enhance implantation success. These results highlight the importance of understanding the molecular mechanisms underlying vitrification to optimize embryo transfer techniques and improve pregnancy outcomes.

Published in International Journal of Molecular Sciences

ISSN: 1661-6596 (Print); 1422-0067 (Online)
Publisher: MDPI AG
Country of publisher: Switzerland
LCC subjects: Science: Biology (General); Science: Chemistry
Website: http://www.mdpi.com/journal/ijms

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