Rikke Bæk ¹ Jenni Katrine Sloth ¹ Mohammad Mehedi Hasan ² Gtnet Midekessa ^3,4 Malene Møller Jørgensen ^1,5*

• ¹ Department of Clinical Immunology, Department of Clinical Immunology, Aalborg University Hospital, Aalborg, Denmark
• ² University College London, Elizabeth Garrett Anderson Institute for Women’s Health, Research Department of maternal and fetal medicine, London, United Kingdom
• ³ Department of Pathophysiology, Institute of Biomedicine and Translational Medicine, Faculty of Medicine, University of Tartu, Tartu, Tartu County, Estonia
• ⁴ Institute of Veterinary Medicine and Animal Sciences, Estonian University of Life Sciences, Tartu, Tartu County, Estonia
• ⁵ Department of Clinical Medicine, Aalborg University, Aalborg, Denmark

This protocol paper describes how to extract small extracellular vesicles (sEVs) from dried blood spots (DBS).The methodology is described in detail and offers further evidence that the extracted particles are sEVs using Western Blotting (anti-CD9, CD63 and CD81) and fluorescence nanoparticle tracking analysis (fNTA). In addition, we present evidence that approximately 40% of the sEVs were recovered from DBS compared with EVs analyzed from plasma directly.The protocol proves to be robust, reliable and displays very interesting performances even after several weeks (up to 3 weeks) of storage of the DBS when analyzing the sEVs using protein microarray for the presence of the markers CD9, CD63, CD81, EpCAM, Flotilin-1, CD62E/P, CD142 and CD235a.These findings have important implications for using sEVs as future potential diagnostic tools by supporting the validity of less-invasive methods that can be implemented within vulnerable populations or in the field.