Flow Cytometry Analysis of Circulating Extracellular Vesicle Subtypes from Fresh Peripheral Blood Samples
0301 basic medicine
polychromatic flow cytometry
Liquid Biopsy
biomarkers
Reproducibility of Results
fresh peripheral blood
Flow Cytometry
Sensitivity and Specificity
Article
biomarkers; extracellular vesicles; fresh peripheral blood; polychromatic flow cytometry; proteomics.
Extracellular Vesicles
Plasma
03 medical and health sciences
proteomics
Biomarkers; Extracellular vesicles; Fresh peripheral blood; Polychromatic flow cytometry; Proteomics
Animals
Humans
Particle Size
extracellular vesicles
Biomarkers
DOI:
10.3390/ijms22010048
Publication Date:
2020-12-23T13:38:43Z
AUTHORS (17)
ABSTRACT
Extracellular vesicles (EVs) are released by shedding during different physiological processes and are increasingly thought to be new potential biomarkers. However, the impact of pre-analytical processing phases on the final measurement is not predictable and for this reason, the translation of basic research into clinical practice has been precluded. Here we have optimized a simple procedure in combination with polychromatic flow cytometry (PFC), to identify, classify, enumerate, and separate circulating EVs from different cell origins. This protocol takes advantage of a lipophilic cationic dye (LCD) able to probe EVs. Moreover, the application of the newly optimized PFC protocol here described allowed the obtainment of repeatable EVs counts. The translation of this PFC protocol to fluorescence-activated cell sorting allowed us to separate EVs from fresh peripheral blood samples. Sorted EVs preparations resulted particularly suitable for proteomic analyses, which we applied to study their protein cargo. Here we show that LCD staining allowed PFC detection and sorting of EVs from fresh body fluids, avoiding pre-analytical steps of enrichment that could impact final results. Therefore, LCD staining is an essential step towards the assessment of EVs clinical significance.
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