Ready‐made chromatography columns for extracellular vesicle isolation from plasma

Proteomic studies of circulating vesicles are hampered by difficulties in purifying vesicles from plasma and serum. Isolations are contaminated with high‐abundance blood proteins that may mask genuine vesicular‐associated proteins and/or simply provide misleading data. In this brief report, we explo...

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Bibliographic Details
Published inJournal of extracellular vesicles Vol. 4; no. 1; pp. 27269 - n/a
Main Authors Welton, Joanne Louise, Webber, Jason Paul, Botos, Laur‐Alexandru, Jones, Michael, Clayton, Aled
Format Journal Article
LanguageEnglish
Published United States Taylor & Francis 01.01.2015
John Wiley & Sons, Inc
Co-Action Publishing
Wiley
Subjects
Blood platelets
CD81 antigen
CD9 antigen
Cell culture
Cell size
Chromatography
exosome precipitation
exosomes
Immunology
Methods
nanoparticle tracking
Nanoparticles
Plasma
Prostate cancer
Protein purification
Proteins
Proteomics
Short Report
ultracentrifugation
Vesicles
United Kingdom > UK
plasma
exosomes
nanoparticle tracking
ultracentrifugation
exosome precipitation
chromatography
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Summary:Proteomic studies of circulating vesicles are hampered by difficulties in purifying vesicles from plasma and serum. Isolations are contaminated with high‐abundance blood proteins that may mask genuine vesicular‐associated proteins and/or simply provide misleading data. In this brief report, we explored the potential utility of a commercially available size exclusion chromatography column for rapid vesicle purification. We evaluated the performance of the column, with cancer cell line conditioned medium or healthy donor plasma, in terms of removing non‐vesicular protein and enriching for vesicles exhibiting exosome characteristics. Serial fractions revealed a peak for typical exosomal proteins (CD9, CD81 etc.) that preceded the peak for highly abundant proteins, including albumin, for either sample type, and harvesting only this peak would represent elimination of >95% of protein from the sample. The columns showed good reproducibility, and streamlining the workflow would allow the exosome‐relevant material to be collected in less than 10 minutes. Surprisingly, however, subsequent post‐column vesicle concentration steps whilst resulting in some protein loss also lead to low vesicle recoveries, with a net effect of reducing sample purity (assessed by the particle‐to‐protein ratio). The columns provide a convenient, reproducible and highly effective means of eliminating >95% of non‐vesicular protein from biological fluid samples such as plasma.
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Responsible Editor: Eva‐Maria Krämer‐Albers, Johannes Gutenberg University, Germany.
Supplementary files
Responsible Editor: Eva-Maria Krämer-Albers, Johannes Gutenberg University, Germany.
ISSN:2001-3078
2001-3078
DOI:10.3402/jev.v4.27269