Antibody titrations are critical for microflow cytometric analysis of extracellular vesicles

Author:

Pink Desmond1,Basu Arghya1,Wong Michael12,Pham Diana1,Valencia Juliana1,Triana Vivian1,Beatty Perrin H.1,Rieger Aja M.2,Lewis John D.13

Affiliation:

1. Nanostics, Inc. Edmonton Alberta Canada

2. Faculty of Medicine and Dentistry University of Alberta Edmonton Alberta Canada

3. Department of Oncology University of Alberta Edmonton Alberta Canada

Abstract

AbstractOptimization of flow cytometry assays for extracellular vesicles (EVs) often fail to include appropriate reagent titrations – the most critically antibody titration is either not performed or is incomplete. Using nonoptimal antibody concentration is one of the main sources of error leading to a lack of reproducible data. Antibody titration for the analysis of antigens on the surface of EVs is challenging for a variety of technical reasons. Using platelets as surrogates for cells and platelet‐derived particles as surrogates for EV populations, we demonstrate our process for antibody titration, highlighting some of the key analysis parameters that may confound and surprise new researchers moving into the field of EV research. Additional care must be exercised to ensure instrument and reagent controls are utilized appropriately. Complete graphical analysis of positive and negative signal intensities, concentration, and separation or stain index data is highly beneficial when paired with visual analysis of the cytometry data. Using analytical flow cytometry procedures optimized for cells for EV analysis can lead to misleading and nonreproducible results.

Funder

Alberta Cancer Foundation

Prostate Cancer Canada

Prostate Cancer Fight Foundation

Publisher

Wiley

Subject

Cell Biology,Histology,Pathology and Forensic Medicine

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