Purification and in vitro functional validation of exosomes from 293T cells with over-expressed membrane-localized IL-3

GAO Lu, CAI Menghua, XU Yi, HE Wei, CHEN Hui, ZHANG Jianmin

doi:10.16352/j.issn.1001-6325.2024.07.0947

Jichu yixue yu linchuang (Jul 2024)

Purification and in vitro functional validation of exosomes from 293T cells with over-expressed membrane-localized IL-3

GAO Lu, CAI Menghua, XU Yi, HE Wei, CHEN Hui, ZHANG Jianmin

Affiliations

GAO Lu, CAI Menghua, XU Yi, HE Wei, CHEN Hui, ZHANG Jianmin: 1. Department of Immunology, Key Laboratory for T Cell and Immunotherapy CAMS, State Key Laboratory of Common Mechanism Research for Major Disease, Institute of Basic Medical Sciences CAMS, School of Basic Medicine PUMC,Beijing 100005;;2. Changzhou Xitaihu Institute for Frontier Technology of Cell Therapy, Changzhou 213000, China

DOI: https://doi.org/10.16352/j.issn.1001-6325.2024.07.0947
Journal volume & issue: Vol. 44, no. 7
pp. 947 – 953

Abstract

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Objective To verify the function of exosomes from 293T cells over-expressing membrane-localized IL-3 in vitro, so as to lay a foundation for in vivo function verification in animal models of Alzheimer′s disease. Methods Using the patented structure of the group, a recombinant IL-3 lentiviral vector was constructed and virus-infected 293T cells were packaged. Stable cell strain over-expressing IL-3 was screened. The membrane localization of IL-3 was verified by flow cytometry and immuno-fluorescence. Il-3-exosomes were purified by ultra filtration centrifugation, the exosmic morphology was observed by transmission electron microscope, the size distribution and concentration of exosomes were detected by nano-flow analysis, and the expression of IL-3 and exosome related marker proteins were detected by Western blot. The effect of BV-2 on the phagocytosis of Aβ amyloid was detected by immuno-fluorescence. Results Through vector construction, virus infection, screening and verification of puromycin, 293T cell strain with stable over-expression membrane-anchored IL-3 was obtained. The purified exosomes were collected and the structures of double-layer membrane vesicles with a diameter of 50-100 nm were observed under transmission electron microscope. Western blot results proved the presence of CD63, ALIX, TSG101 and other exosome marker proteins and these molecules were rich in IL-3 as compared with the control, that suggested the successful purification of IL-3-exosomes. The results of immuno-fluorescence assay showed that IL-3-exosomes promoted the phagocytosis of Aβ amyloid by BV-2 cells in vitro. Conclusions The gene modified 293T cell exosomes membrane-anchored expression of IL-3 can play a role of both IL-3 and exosomes in vitro, which promote the phagocytosis of microglia, there for provides a new idea for the clinical treatment of Alzheimer′s disease.

interleukin-3(il-3)|exosome|mouse brain microglial cell line(bv-2)|alzheimer′s disease

Published in Jichu yixue yu linchuang

ISSN: 1001-6325 (Print)
Publisher: Institute of Basic Medical Sciences and Peking Union Medical College Hospital, Chinese Academy of Medical Sciences / Peking Union Medical College.
Country of publisher: China
LCC subjects: Medicine
Website: http://journal11.magtechjournal.com/Jwk_jcyxylc/EN/1001-6325/home.shtml

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