Journal of Extracellular Vesicles (Aug 2024)

Comparison of EV characterization by commercial high‐sensitivity flow cytometers and a custom single‐molecule flow cytometer

  • James Kim,
  • Shihan Xu,
  • Seung‐Ryoung Jung,
  • Alya Nguyen,
  • Yuanhua Cheng,
  • Mengxia Zhao,
  • Bryant S. Fujimoto,
  • Wyatt Nelson,
  • Perry Schiro,
  • Jeffrey L. Franklin,
  • James N. Higginbotham,
  • Robert J. Coffey,
  • Min Shi,
  • Lucia N. Vojtech,
  • Florian Hladik,
  • Muneesh Tewari,
  • John Tigges,
  • Ionita Ghiran,
  • Tijana Jovanovic‐Talisman,
  • Louise C. Laurent,
  • Saumya Das,
  • Olesia Gololobova,
  • Kenneth W. Witwer,
  • Tuoye Xu,
  • Al Charest,
  • Kendall Van Keuren Jensen,
  • Robert L. Raffai,
  • Jennifer C. Jones,
  • Joshua A. Welsh,
  • John P. Nolan,
  • Daniel T. Chiu

DOI
https://doi.org/10.1002/jev2.12498
Journal volume & issue
Vol. 13, no. 8
pp. n/a – n/a

Abstract

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Abstract High‐sensitivity flow cytometers have been developed for multi‐parameter characterization of single extracellular vesicles (EVs), but performance varies among instruments and calibration methods. Here we compare the characterization of identical (split) EV samples derived from human colorectal cancer (DiFi) cells by three high‐sensitivity flow cytometers, two commercial instruments, CytoFLEX/CellStream, and a custom single‐molecule flow cytometer (SMFC). DiFi EVs were stained with the membrane dye di‐8‐ANEPPS and with PE‐conjugated anti‐EGFR or anti‐tetraspanin (CD9/CD63/CD81) antibodies for estimation of EV size and surface protein copy numbers. The limits of detection (LODs) for immunofluorescence and vesicle size based on calibration using cross‐calibrated, hard‐dyed beads were ∼10 PE/∼80 nm EV diameter for CytoFLEX and ∼10 PEs/∼67 nm for CellStream. For the SMFC, the LOD for immunofluorescence was 1 PE and ≤ 35 nm for size. The population of EVs detected by each system (di‐8‐ANEPPS+/PE+ particles) differed widely depending on the LOD of the system; for example, CellStream/CytoFLEX detected only 5.7% and 1.5% of the tetraspanin‐labelled EVs detected by SMFC, respectively, and median EV diameter and antibody copy numbers were much larger for CellStream/CytoFLEX than for SMFC as measured and validated using super‐resolution/single‐molecule TIRF microscopy. To obtain a dataset representing a common EV population analysed by all three platforms, we filtered out SMFC and CellStream measurements for EVs below the CytoFLEX LODs as determined by bead calibration (10 PE/80 nm). The inter‐platform agreement using this filtered dataset was significantly better than for the unfiltered dataset, but even better concordance between results was obtained by applying higher cutoffs (21 PE/120 nm) determined by threshold analysis using the SMFC data. The results demonstrate the impact of specifying LODs to define the EV population analysed on inter‐instrument reproducibility in EV flow cytometry studies, and the utility of threshold analysis of SMFC data for providing semi‐quantitative LOD values for other flow cytometers.

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