Impact of Extraction Methods and Transportation Conditions on Lipid Profiles of Bovine Oocytes

Camila Bruna de Lima; Marcella Pecora Milazzotto; Alessandra Aparecida Vireque; Daniel Carlino Joaquim; Tiago Jose Paschoal Sobreira; Christina Ramires Ferreira

doi:10.1007/s43032-024-01524-9

Impact of Extraction Methods and Transportation Conditions on Lipid Profiles of Bovine Oocytes

Reprod Sci. 2024 Apr 1. doi: 10.1007/s43032-024-01524-9. Online ahead of print.

Authors

Camila Bruna de Lima^{1

2

3}, Marcella Pecora Milazzotto², Alessandra Aparecida Vireque⁴, Daniel Carlino Joaquim⁴, Tiago Jose Paschoal Sobreira⁵, Christina Ramires Ferreira^{5

6}

Affiliations

¹ Department of Animal Sciences, Université Laval, Québec, QC, Canada.
² Center of Natural and Human Sciences, Universidade Federal Do ABC, Santo André, São Paulo, Brazil.
³ , Ville de Québec, Canada.
⁴ Invitra, Assisted Reproductive Technologies Ltd., Supera Innovation and Technology Park, Ribeirão Preto, SP, 14056-680, Brazil.
⁵ Center for Analytical Instrumentation Development, Department of Chemistry, Purdue University, West Lafayette, IN, 47907, USA.
⁶ Bindley Bioscience Center, Purdue University, West Lafayette, IN, 47907, USA.

PMID: 38561471
DOI: 10.1007/s43032-024-01524-9

Abstract

Lipids play numerous pivotal physiological roles in mammalian reproduction, being indispensable for oocyte competence acquisition and post-fertilization embryonic development. Profiling lipids in minute samples, such as oocytes, presents challenges but has been accomplished through mass spectrometry technologies like Multiple Reaction Monitoring (MRM) profiling. With the dual objectives of simplifying workflow and examining the influence of preanalytical conditions, we assessed whether transportation at room temperature affects the lipid profile of bovine oocytes. To this end, samples were prepared using either monophasic (methanol only) or biphasic liquid extraction protocols (Bligh & Dyer method) and transported either on dry ice or at room temperature inside sealed-vacuum packages to prevent lipid oxidation. Subsequently, employing a comprehensive method, we screened a list of 316 MRMs from 10 different lipid subclasses in oocyte lipid extracts. Principal Component Analysis (PCA) revealed similar lipid profiles concerning temperature during transportation, whereas clear differentiation among samples was observed based on the lipid extraction method. Univariate analysis indicated that the one-phase methanol extraction resulted in higher relative abundances of phospholipids, except for phosphatidylserines. Conversely, the Bligh & Dyer extraction favored the detection of neutral intracellular lipids (triacylglycerols, free fatty acids, cholesteryl esters, and acyl-carnitines). Consequently, lipid recovery was directly correlated with the polarity of lipid class and the extraction method. Regarding transportation temperature, phosphatidylethanolamine, triacylglycerol, and free fatty acids exhibited lower abundances when samples were transported at room temperature. Based on multivariate and univariate analyses, we conclude that if samples undergo the same lipid extraction protocol and are transported in the same batch at room temperature inside vacuum-sealed bags, it is feasible to analyze lipid extracts of bovine oocytes and still obtain informative lipid profiling results.

Keywords: Bovine; Lipid extraction; Multiple Reaction Monitoring; Oocytes; Room temperature; Vacuum pressure.

Grants and funding

R21EB015722/EB/NIBIB NIH HHS/United States