4.7 Article

Tetraspanins distinguish separate extracellular vesicle subpopulations in human serum and plasma - Contributions of platelet extracellular vesicles in plasma samples

Journal

JOURNAL OF EXTRACELLULAR VESICLES
Volume 11, Issue 5, Pages -

Publisher

WILEY
DOI: 10.1002/jev2.12213

Keywords

biomarkers; exosomes; extracellular vesicles; microvesicles; plasma; serum; subpopulations

Categories

Funding

  1. Swedish Research Council [2016-02854]
  2. Swedish Heart and Lung Foundation [2018-0569]
  3. Swedish Cancer Foundation [CAN2017/739]
  4. VBG Group Herman Krefting Foundation for Asthma and Allergy Research
  5. Swedish Research Council [2016-02854] Funding Source: Swedish Research Council

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This study reveals the presence of multiple subpopulations of extracellular vesicles (EVs) carrying different tetraspanins in both plasma and serum. The sampling methods and centrifugation protocols used for blood can impact EV analysis results.
Background: The ability to isolate extracellular vesicles (EVs) from blood is vital in the development of EVs as disease biomarkers. Both serum and plasma can be used, but few studies have compared these sources in terms of the type of EVs that are obtained. The aim of this study was to determine the presence of different subpopulations of EVs in plasma and serum. Method: Blood was collected from healthy subjects, and plasma and serum were isolated in parallel. ACD or EDTA tubes were used for the collection of plasma, while serum was obtained in clot activator tubes. EVs were isolated utilising a combination of density cushion and SEC, a combination of density cushion and gradient or by a bead antibody capturing system (anti-CD63, anti-CD9 and anti-CD81 beads). The subpopulations of EVs were analysed by NTA, Western blot, SP-IRIS, conventional and nano flow cytometry, magnetic bead E LISA and mass spectrometry. Additionally, different isolation protocols for plasma were compared to determine the contribution of residual platelets in the analysis. Results: This study shows that a higher number of CD9(+) EVs were present in EDTA-plasma compared to ACD-plasma and to serum, and the presence of CD41a on these EVs suggests that they were released from platelets. Furthermore, only a very small number of EVs in blood were double-positive for CD63 and CD81. The CD63(+) EVs were enriched in serum, while CD81(+) vesicles were the rarest subpopulation in both plasma and serum. Additionally, EDTA-plasma contained more residual platelets than ACD-plasma and serum, and two centrifugation steps were crucial to reduce the number of platelets in plasma prior to EV isolation. Conclusion: These results show that human blood contains multiple subpopulations of EVs that carry different tetraspanins. Blood sampling methods, including the use of anti-coagulants and choice of centrifugation protocols, can affect EV analyses and should always be reported in detail.

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