Particle profiling of EV‐lipoprotein mixtures by AFM nanomechanical imaging

Author:

Ridolfi Andrea1,Conti Laura1,Brucale Marco12,Frigerio Roberto34,Cardellini Jacopo5,Musicò Angelo234,Romano Miriam24,Zendrini Andrea24,Polito Laura3,Bergamaschi Greta3,Gori Alessandro3,Montis Costanza25,Panella Stefano6,Barile Lucio6,Berti Debora25,Radeghieri Annalisa24,Bergese Paolo247,Cretich Marina3,Valle Francesco12

Affiliation:

1. Consiglio Nazionale delle Ricerche Istituto per lo Studio dei Materiali Nanostrutturati Bologna Italy

2. Consorzio Interuniversitario per lo Sviluppo dei Sistemi a Grande Interfase Firenze Italy

3. Consiglio Nazionale delle Ricerche Istituto di Scienze e Tecnologie Chimiche “Giulio Natta” Milan Italy

4. Dipartimento di Medicina Molecolare e Traslazionale Università degli Studi di Brescia Brescia Italy

5. Dipartimento di Chimica “Ugo Schiff” Università degli Studi di Firenze Firenze Italy

6. Istituto Cardiocentro Ticino Ente Ospedaliero Cantonale Lugano Switzerland

7. Consiglio Nazionale delle Ricerche, Istituto per la Ricerca e l'innovazione Biomedica Palermo Italy

Abstract

AbstractThe widely overlapping physicochemical properties of lipoproteins (LPs) and extracellular vesicles (EVs) represents one of the main obstacles for the isolation and characterization of these pervasive biogenic lipid nanoparticles. We herein present the application of an atomic force microscopy (AFM)‐based quantitative morphometry assay to the rapid nanomechanical screening of mixed LPs and EVs samples. The method can determine the diameter and the mechanical stiffness of hundreds of individual nanometric objects within few hours. The obtained diameters are in quantitative accord with those measured via cryo‐electron microscopy (cryo‐EM); the assignment of specific nanomechanical readout to each object enables the simultaneous discrimination of co‐isolated EVs and LPs even if they have overlapping size distributions. EVs and all classes of LPs are shown to be characterised by specific combinations of diameter and stiffness, thus making it possible to estimate their relative abundance in EV/LP mixed samples in terms of stoichiometric ratio, surface area and volume. As a side finding, we show how the mechanical behaviour of specific LP classes is correlated to distinctive structural features revealed by cryo‐EM. The described approach is label‐free, single‐step and relatively quick to perform. Importantly, it can be used to analyse samples which prove very challenging to assess with several established techniques due to ensemble‐averaging, low sensibility to small particles, or both, thus providing a very useful tool for quickly assessing the purity of EV/LP isolates including plasma‐ and serum‐derived preparations.

Publisher

Wiley

Subject

Cell Biology,Histology

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