Single-cell profiling reveals transcriptome dynamics during bovine oocyte growth

Lais Barbosa Latorraca; António Galvão; Maria Belen Rabaglino; Julieta Maria D'Augero; Gavin Kelsey; Trudee Fair

doi:10.1186/s12864-024-10234-0

Single-cell profiling reveals transcriptome dynamics during bovine oocyte growth

BMC Genomics. 2024 Apr 6;25(1):335. doi: 10.1186/s12864-024-10234-0.

Authors

Lais Barbosa Latorraca¹, António Galvão^{2

3}, Maria Belen Rabaglino⁴, Julieta Maria D'Augero¹, Gavin Kelsey^{2

5

6}, Trudee Fair⁷

Affiliations

¹ School of Agriculture and Food Science, University College Dublin, Dublin, Ireland.
² Epigenetics Programme, The Babraham Institute, Cambridge, UK.
³ Department of Comparative Biomedical Sciences, Royal Veterinary College, London, UK.
⁴ Department of Population Health Sciences, Faculty of Veterinary Medicine, Utrecht University, Yalelaan 7, 3584 CL, Utrecht, The Netherlands.
⁵ Centre for Trophoblast Research, University of Cambridge, Cambridge, UK.
⁶ Wellcome-MRC Institute of Metabolic Science-Metabolic Research Laboratories, Cambridge, UK.
⁷ School of Agriculture and Food Science, University College Dublin, Dublin, Ireland. trudee.fair@ucd.ie.

Abstract

Background: Mammalian follicle development is characterized by extensive changes in morphology, endocrine responsiveness, and function, providing the optimum environment for oocyte growth, development, and resumption of meiosis. In cattle, the first signs of transcription activation in the oocyte are observed in the secondary follicle, later than during mouse and human oogenesis. While many studies have generated extensive datasets characterizing gene expression in bovine oocytes, they are mostly limited to the analysis of fully grown and matured oocytes. The aim of the present study was to apply single-cell RNA sequencing to interrogate the transcriptome of the growing bovine oocyte from the secondary follicle stage through to the mid-antral follicle stage.

Results: Single-cell RNA-seq libraries were generated from oocytes of known diameters (< 60 to > 120 μm), and datasets were binned into non-overlapping size groups for downstream analysis. Combining the results of weighted gene co-expression network and Trendy analyses, and differently expressed genes (DEGs) between size groups, we identified a decrease in oxidative phosphorylation and an increase in maternal -genes and transcription regulators across the bovine oocyte growth phase. In addition, around 5,000 genes did not change in expression, revealing a cohort of stable genes. An interesting switch in gene expression profile was noted in oocytes greater than 100 μm in diameter, when the expression of genes related to cytoplasmic activities was replaced by genes related to nuclear activities (e.g., chromosome segregation). The highest number of DEGs were detected in the comparison of oocytes 100-109 versus 110-119 μm in diameter, revealing a profound change in the molecular profile of oocytes at the end of their growth phase.

Conclusions: The current study provides a unique dataset of the key genes and pathways characteristic of each stage of oocyte development, contributing an important resource for a greater understanding of bovine oogenesis.

Keywords: Cattle; Gene Expression; Oogenesis; RNA sequencing.

MeSH terms

Animals
Cattle
Cell Proliferation
Female
Humans
Mammals / genetics
Mice
Oocytes / metabolism
Oogenesis* / genetics
Ovarian Follicle / metabolism
Transcriptome*

Abstract

MeSH terms

Grants and funding