Artificial Extracellular Vesicles Generated from T Cells Using Different Induction Techniques

Author:

Zmievskaya Ekaterina A.1,Mukhametshin Sabir A.1ORCID,Ganeeva Irina A.1,Gilyazova Elvina M.1,Siraeva Elvira T.1,Kutyreva Marianna P.2ORCID,Khannanov Artur A.2ORCID,Yuan Youyong3,Bulatov Emil R.14ORCID

Affiliation:

1. Institute of Fundamental Medicine and Biology, Kazan Federal University, 420008 Kazan, Russia

2. A.M. Butlerov Institute of Chemistry, Kazan Federal University, 420008 Kazan, Russia

3. School of Biomedical Sciences and Engineering, South China University of Technology, Guangzhou International Campus, Guangzhou 511442, China

4. Shemyakin-Ovchinnikov Institute of Bioorganic Chemistry, Russian Academy of Sciences, 117997 Moscow, Russia

Abstract

Cell therapy is at the forefront of biomedicine in oncology and regenerative medicine. However, there are still significant challenges to their wider clinical application such as limited efficacy, side effects, and logistical difficulties. One of the potential approaches that could overcome these problems is based on extracellular vesicles (EVs) as a cell-free therapy modality. One of the major obstacles in the translation of EVs into practice is their low yield of production, which is insufficient to achieve therapeutic amounts. Here, we evaluated two primary approaches of artificial vesicle induction in primary T cells and the SupT1 cell line—cytochalasin B as a chemical inducer and ultrasonication as a physical inducer. We found that both methods are capable of producing artificial vesicles, but cytochalasin B induction leads to vesicle yield compared to natural secretion, while ultrasonication leads to a three-fold increase in particle yield. Cytochalasin B induces the formation of vesicles full of cytoplasmic compartments without nuclear fraction, while ultrasonication induces the formation of particles rich in membranes and membrane-related components such as CD3 or HLAII proteins. The most effective approach for T-cell induction in terms of the number of vesicles seems to be the combination of anti-CD3/CD28 antibody activation with ultrasonication, which leads to a seven-fold yield increase in particles with a high content of functionally important proteins (CD3, granzyme B, and HLA II).

Funder

Russian Science Foundation

Publisher

MDPI AG

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