Imaging the subcellular viscoelastic properties of mouse oocytes

Author:

Flé Guillaume1,Van Houten Elijah2ORCID,Rémillard-Labrosse Gaudeline3,FitzHarris Greg34,Cloutier Guy15ORCID

Affiliation:

1. Laboratory of Biorheology and Medical Ultrasonics, University of Montreal Hospital Research Center, Montreal, QC H2X 0A9, Canada

2. Mechanical Engineering Department, University of Sherbrooke, Sherbrooke, QC J1K 2R1, Canada

3. Oocyte and Embryo Research Laboratory, University of Montreal Hospital Research Center, Montreal, QC H2X 0A9, Canada

4. Department of Obstetrics and Gynecology, University of Montreal, Montreal, QC H3T 1J4, Canada

5. Department of Radiology, Radio-Oncology and Nuclear Medicine, and Institute of Biomedical Engineering, University of Montreal, Montreal, QC H3T 1J4, Canada

Abstract

In recent years, cellular biomechanical properties have been investigated as an alternative to morphological assessments for oocyte selection in reproductive science. Despite the high relevance of cell viscoelasticity characterization, the reconstruction of spatially distributed viscoelastic parameter images in such materials remains a major challenge. Here, a framework for mapping viscoelasticity at the subcellular scale is proposed and applied to live mouse oocytes. The strategy relies on the principles of optical microelastography for imaging in combination with the overlapping subzone nonlinear inversion technique for complex-valued shear modulus reconstruction. The three-dimensional nature of the viscoelasticity equations was accommodated by applying an oocyte geometry-based 3D mechanical motion model to the measured wave field. Five domains—nucleolus, nucleus, cytoplasm, perivitelline space, and zona pellucida—could be visually differentiated in both oocyte storage and loss modulus maps, and statistically significant differences were observed between most of these domains in either property reconstruction. The method proposed herein presents excellent potential for biomechanical-based monitoring of oocyte health and complex transformations across lifespan. It also shows appreciable latitude for generalization to cells of arbitrary shape using conventional microscopy equipment.

Funder

Gouvernement du Canada | Natural Sciences and Engineering Research Council of Canada

Fonds de Recherche Quebec

Publisher

Proceedings of the National Academy of Sciences

Subject

Multidisciplinary

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