Physical association of low density lipoprotein particles and extracellular vesicles unveiled by single particle analysis

Author:

Lozano‐Andrés Estefanía1ORCID,Enciso‐Martinez Agustin23ORCID,Gijsbers Abril4,Ridolfi Andrea5,Van Niel Guillaume6,Libregts Sten F. W. M.1,Pinheiro Cláudio78ORCID,van Herwijnen Martijn J. C.1,Hendrix An78,Brucale Marco9ORCID,Valle Francesco9,Peters Peter J.4,Otto Cees3,Arkesteijn Ger J. A.1,Wauben Marca H. M.1ORCID

Affiliation:

1. Department of Biomolecular Health Sciences, Faculty of Veterinary Medicine Utrecht University Utrecht The Netherlands

2. Department of Cell and Chemical Biology Leiden University Medical Center Leiden The Netherlands

3. Medical Cell Biophysics Group University of Twente Enschede The Netherlands

4. Maastricht Multimodal Molecular Imaging Institute, Division of Nanoscopy Maastricht University Maastricht The Netherlands

5. Department of Physics and Astronomy and LaserLaB Amsterdam Vrije Universiteit Amsterdam Amsterdam The Netherlands

6. Institute for Psychiatry and Neuroscience of Paris Hopital Saint‐Anne, Université Descartes Paris France

7. Laboratory of Experimental Cancer Research Department of Human Structure and Repair Ghent University Ghent Belgium

8. Cancer Research Institute Ghent Ghent Belgium

9. Institute for the Study of Nanostructured Materials (ISMN) Italian National Research Council (CNR) Bologna Italy

Abstract

AbstractExtracellular vesicles (EVs) in blood plasma are recognized as potential biomarkers for disease. Although blood plasma is easily obtainable, analysis of EVs at the single particle level is still challenging due to the biological complexity of this body fluid. Besides EVs, plasma contains different types of lipoproteins particles (LPPs), that outnumber EVs by orders of magnitude and which partially overlap in biophysical properties such as size, density and molecular makeup. Consequently, during EV isolation LPPs are often co‐isolated. Furthermore, physical EV‐LPP complexes have been observed in purified EV preparations. Since co‐isolation or association of LPPs can impact EV‐based analysis and biomarker profiling, we investigated the presence and formation of EV‐LPP complexes in biological samples by using label‐free atomic force microscopy, cryo‐electron tomography and synchronous Rayleigh and Raman scattering analysis of optically trapped particles and fluorescence‐based high sensitivity single particle flow cytometry. Furthermore, we evaluated the impact on flow cytometric analysis in the presence of LPPs using in vitro spike‐in experiments of purified tumour cell line‐derived EVs in different classes of purified human LPPs. Based on orthogonal single‐particle analysis techniques we demonstrate that EV‐LPP complexes can form under physiological conditions. Furthermore, we show that in fluorescence‐based flow cytometric EV analysis staining of LPPs, as well as EV‐LPP associations, can influence quantitative and qualitative EV analysis. Lastly, we demonstrate that the colloidal matrix of the biofluid in which EVs reside impacts their buoyant density, size and/or refractive index (RI), which may have consequences for down‐stream EV analysis and EV biomarker profiling.

Funder

Fondation pour la Recherche Médicale

Publisher

Wiley

Subject

Cell Biology,Histology

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