Purification and biodistribution of extracellular vesicles
Extracellular vesicles (EVs) are nano-sized vesicles that contain bioactive lipids, RNAs and proteins, which can be transferred to recipient cells. EVs are important for physiological as well as pathological processes, such as coagulation and immune homeostasis, aiding cancer metastasis and spread of infectious diseases. Owing to their relatively small size the purification of EVs is a challenge, hence we have established and optimised workflows consisting of ultrafiltration with subsequent size exclusion liquid chromatography (UFLC)( Paper I) and bind-elute combined with size exclusion (BE-SEC) columns (Paper III) for EV purification.
UF-LC allowed for purification of biophysically intact EVs with better yield and purity compared to ultracentrifugation (UC), which is the gold standard purification method in the field. The biodistribution of UF-LC EVs was different compared to vesicles isolated using UC, despite having highly similar protein composition according to proteomics analysis. We found that UF-LC vesicles accumulated less in lung, possibly owing to their higher integrity. Indeed, fluorescence correlation spectroscopy and transmission electron microscopy indicated that the high gravitational forces in UC lead to aggregation and disruption of the vesicles. The BE-SEC method is a similar method to UF-LC, however protein impurities less than 700 kDa in size are bound in the interior of the beads, thus improving simple size-based exclusion. The BE-SEC method is scalable, produces samples with better purity than UC, displaying yields exceeding 70% and demonstrates a good reproducibility between samples. Moreover, vesicles purified by BE-SEC display the same EV surface markers as UC purified EVs, and CD63-eGFP positive vesicles are taken up in recipient cells to the same extent. In summary, the BE-SEC method is a reproducible and fast alternative to UF-LC for large media volumes.
Reliable purification methods are important for the implementation of therapeutically active EVs, however knowledge regarding their eventual organotropism and biodistribution is equally important. Thus, in article II we evaluated the biodistribution of EVs specifically labeled with a near-infrared dye. The main sites of accumulation of exogenously injected EVs were liver, spleen and lungs. Biodistribution profile of EVs depended strongly on injection route, and to certain extent, on EV cell type source, as dendritic cell derived EVs exhibited a more pronounced uptake in spleen compared to the other cell sources tested. We further showed that small alterations of EV surface proteins could significantly affect biodistribution as well, since EVs equipped with a brain targeting peptide on their surface increased the uptake of targeted EVs in brain. This study highlights that the biodistribution of EVs follows other nano-sized particles with uptake mainly in liver. Administration route, cell source and a targeting peptide influence the distribution, however the overall distribution is unaltered with the highest signal originating from liver.
To summarise, this thesis has resulted in improvements of the EV field by systematically enhancing EV isolation workflows to achieve greater sample purity and at the same time preserving EV biophysical characteristics. Furthermore, it has laid groundwork for studying in vivo effects of exogenous vesicles. Both these aspects are particularly important for understanding EV biology more clearly and with increased detail.
List of scientific papers
I. Ultrafiltration with size-exclusion liquid chromatography for high yield isolation of extracellular vesicles preserving intact biophysical and functional properties. Joel Z. Nordin, Yi Lee, Pieter Vader, Imre Mäger, Henrik J. Johansson, Wolf Heusermann, Oscar P.B. Wiklander, Mattias Hällbrink, Yiqi Seow, Jarred J. Bultema, Jonathan Gilthorpe, Tim Davies, Paul J. Fairchild, Susanne Gabrielsson, Nicole C. Meisner-Kober, Janne Lehtiö, C.I. Edvard Smith, Matthew J.A. Wood, M.D., Samir EL Andaloussi. Nanomedicine: Nanotechnology, Biology, and Medicine. 2015, 11, 879–883.
https://doi.org/10.1016/j.nano.2015.01.003
II. Extracellular vesicle in vivo biodistribution is determined by cell source, route of administration and targeting. Oscar P. B. Wiklander, Joel Z. Nordin, Aisling O’Loughlin, Ylva Gustafsson, Giulia Corso, Imre Ma ̈ger, Pieter Vader, Yi Lee, Helena Sork, Yiqi Seow, Nina Heldring, Lydia Alvarez-Erviti, CI Edvard Smith, Katarina Le Blanc, Paolo Macchiarini, Philipp Jungebluth, Matthew J. A. Wood and Samir EL Andaloussi. Journal of Extracellular Vesicles. 2015, 4, 26316.
https://doi.org/10.3402/jev.v4.26316
III. Fast and reproducible purification of extracellular vesicles using combined size exclusion and ion exchange chromatography. Giulia Corso, Joel Z. Nordin, Imre Mäger, Yi Lee, André Görgens, Jarred Bultema, Bernd Giebel, Matthew J.A. Wood and Samir EL Andaloussi. [Manuscript]
History
Defence date
2017-03-03Department
- Department of Laboratory Medicine
Publisher/Institution
Karolinska InstitutetMain supervisor
El-Andaloussi, SamirPublication year
2017Thesis type
- Doctoral thesis
ISBN
978-91-7676-572-2Number of supporting papers
3Language
- eng