Imaging of Isolated Exosomes by Correlative Microscopy

Author:

Demir Şeyda12ORCID,Erdal Esra34,Bagriyanik Hüsnü Alper124ORCID

Affiliation:

1. Department of Histology and Embryology, Faculty of Medicine

2. Department of Histology and Embryology, Health Science Institute

3. Department of Medical Biology and Genetics, Faculty of Medicine

4. Dokuz Eylul University, Izmir, Türkiye, and Izmir Biomedicine and Genome Center, 35340 Izmir, Türkiye

Abstract

Correlative microscopy is a sophisticated imaging technique that combines optical and electron microscopes, with the most common approach being the integration of light microscopy and electron microscopy, known as correlative light and electron microscopy (CLEM). While CLEM provides a comprehensive view of biological samples, it presents a significant challenge in sample preparation due to the distinct processes involved in each technique. Striking a balance between these methods is crucial. Despite numerous approaches, achieving seamless imaging with CLEM remains a complex task. Exosomes, nanovesicles ranging from 30 to 150 nm in size, are enclosed by a lipid bilayer and released by various cell types. Visualizing exosomes poses difficulties due to their small size and minimal electric charge. However, imaging exosomes at high resolution offers a direct method to understand their morphology and functions. In this study, we evaluated exosome imaging with CLEM using a combination of confocal, transmission electron microscope, and scanning electron microscope (SEM). In addition, we conducted a comparative analysis of these two techniques, evaluating their suitability and efficiency in imaging nanoscale structures. In this study, we found that confocal-SEM correlation is more applicable for imaging exosomes. Moreover, we observed that exosomes were found in clusters in confocal-SEM correlation.

Funder

Research fund of Dokuz Eylul University

Publisher

SAGE Publications

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