Red blood cell-derived extracellular vesicles (RBC-EVs) are emerging as promising biomaterials for next-generation drug delivery, owing to their intrinsic biocompatibility, immune-evasion properties, and minimal oncogenic risk. However, their broader application is currently limited by unresolved challenges related to heterogeneity, reproducibility, and long-term storage stability. By combining discontinuous sucrose density gradient separation with high-resolution interferometric nanoparticle tracking analysis, we identified a sharp bimodal size distribution of vesicles in freshly prepared samples. We then tracked how long-term storage at −80 °C drove their conversion into a monomodal distribution. To reproduce these conditions in a shorter time frame, we developed an “accelerated-ageing” protocol based on freeze–thaw cycles that generates RBC-EV samples with homogeneous density, size distribution, and biological activity, effectively replicating the properties of preparations stored for six months at −80 °C. This new vesicle population remains stable and retains membrane integrity and cellular internalization capacity, as confirmed by surface-associated enzymatic activity assays and uptake tests in cancer cell lines. These results suggest that freezing-induced “accelerated ageing” represents an effective method for the optimization and standardization of RBC-EVs as building blocks for biomaterial and bioengineering applications.

Red blood cell-derived extracellular vesicles as biomaterials: the opportunity of freezing-induced accelerated aging

Paolini, Lucia;Romano, Miriam;Mangolini, Valentina;Tassoni, Selene;Mazzoldi, Elena Laura;Musicò, Angelo;Zendrini, Andrea;Giliani, Silvia Clara;Bergese, Paolo;Radeghieri, Annalisa
2026-01-01

Abstract

Red blood cell-derived extracellular vesicles (RBC-EVs) are emerging as promising biomaterials for next-generation drug delivery, owing to their intrinsic biocompatibility, immune-evasion properties, and minimal oncogenic risk. However, their broader application is currently limited by unresolved challenges related to heterogeneity, reproducibility, and long-term storage stability. By combining discontinuous sucrose density gradient separation with high-resolution interferometric nanoparticle tracking analysis, we identified a sharp bimodal size distribution of vesicles in freshly prepared samples. We then tracked how long-term storage at −80 °C drove their conversion into a monomodal distribution. To reproduce these conditions in a shorter time frame, we developed an “accelerated-ageing” protocol based on freeze–thaw cycles that generates RBC-EV samples with homogeneous density, size distribution, and biological activity, effectively replicating the properties of preparations stored for six months at −80 °C. This new vesicle population remains stable and retains membrane integrity and cellular internalization capacity, as confirmed by surface-associated enzymatic activity assays and uptake tests in cancer cell lines. These results suggest that freezing-induced “accelerated ageing” represents an effective method for the optimization and standardization of RBC-EVs as building blocks for biomaterial and bioengineering applications.
2026
Altre Amm. Pubb. Italiane
LS1_2 General biochemistry and metabolism
LS9_9 Biotechnology, bioreactors, applied microbiology
PE4_4 Surface science and nanostructures
Esperti anonimi
Inglese
Internazionale
ELETTRONICO
14
1
122
139
18
Utilizzata la piattaforma banca criogenica del dipartimento di MMT
https://pubs.rsc.org/en/content/articlehtml/2026/bm/d5bm01349f
Not applicable
14
info:eu-repo/semantics/article
262
Paolini, Lucia; Romano, Miriam; Mangolini, Valentina; Tassoni, Selene; Jiang, Shuhan; Mazzoldi, Elena Laura; Musicò, Angelo; Zendrini, Andrea; Kashkan...espandi
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Utilizza questo identificativo per citare o creare un link a questo documento: https://hdl.handle.net/11379/637005
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