Surface Plasmon Resonance is an Analytically Sensitive Method for Antigen Profiling of Extracellular Vesicles

Author:

Gool Elmar L123,Stojanovic Ivan4,Schasfoort Richard B M4,Sturk Auguste23,van Leeuwen Ton G13,Nieuwland Rienk23,Terstappen Leon W M M34,Coumans Frank A W13

Affiliation:

1. Department of Biomedical Engineering and Physics

2. Department of Clinical Chemistry

3. Vesicle Observation Center, Amsterdam Medical Center, University of Amsterdam, Amsterdam, the Netherlands

4. Department of Medical Cell Biophysics, University of Twente, Enschede, the Netherlands

Abstract

Abstract BACKGROUND Identification, enumeration, and characterization of extracellular vesicles (EVs) are hampered by the small size of EVs, a low refractive index, and low numbers of antigens on their surface. METHODS We investigated the potential of a 48-multiplex surface plasmon resonance imaging (SPRi) system to perform EV phenotyping. Antigen surface density of 11 antigens was measured on the human breast cancer cell lines HS578T, MCF7, and SKBR3 and their EVs by use of both SPRi and the widely used flow cytometry (FCM). RESULTS For cells, the SPRi and FCM signals for antigen exposure correlated (RHS578T cells2 = 0.66, RMCF7 cells2 = 0.78, RSKBR3 cells2 = 0.60). With regard to EVs, SPRi detected 31 out of 33 tested antibody–EV pairs, whereas our flow cytometer detected 5 antibody–EV pairs because of high blank and isotype control signals. For HS578T-derived EVs, the SPRi and FCM signals correlated (R2HS578T EVs = 0.98). However, on MCF7- and SKBR3-derived EVs, insufficient antigens were detected by our flow cytometer. To confirm that the SPRi responses correlated with mean antigen density on EVs, the SPRi responses of EVs were correlated with antigen density on parental cells as measured by FCM (RHS578T2 = 0.77, RMCF72 = 0.49, RSKBR32 = 0.52). CONCLUSIONS SPRi responses correlate with mean antigen density. Moreover, SPRi detects lower antigen-exposure levels than FCM because SPRi measures an ensemble of EVs binding to the sensor surface, whereas FCM detects antigens of single EV.

Funder

Agentschap NL

Academia Mexicana de Ciencias

Europese Unie

SURFnet bv

Stichting voor de Technische Wetenschappen

Publisher

Oxford University Press (OUP)

Subject

Biochemistry (medical),Clinical Biochemistry

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