Construction of LP-LNP with novel lipopeptides as adjuvants and its enhancing effects on mRNA vaccines

CAO Jingwen; CAO Jingwen; CHI Yu; LI Guocheng

doi:10.16016/j.2097-0927.202402048

陆军军医大学学报 (Sep 2024)

Construction of LP-LNP with novel lipopeptides as adjuvants and its enhancing effects on mRNA vaccines

CAO Jingwen,
CAO Jingwen,
CHI Yu,
LI Guocheng

Affiliations

CAO Jingwen: Clinical Medical School, Jiamusi University, Jiamusi, Heilongjiang Province, 154007
CAO Jingwen: Department of Microbiology and Biochemical Pharmacy, National Engineering Technology Research Center for Immune Biological Products, Faculty of Pharmacy and Laboratory Medicine, Army Medical University (Third Military Medical University), Chongqing, 400038
CHI Yu: Clinical Medical School, Jiamusi University, Jiamusi, Heilongjiang Province, 154007
LI Guocheng: Department of Microbiology and Biochemical Pharmacy, National Engineering Technology Research Center for Immune Biological Products, Faculty of Pharmacy and Laboratory Medicine, Army Medical University (Third Military Medical University), Chongqing, 400038

DOI: https://doi.org/10.16016/j.2097-0927.202402048
Journal volume & issue: Vol. 46, no. 17
pp. 1925 – 1933

Abstract

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Objective To construct lipid nanoparticles (lipopeptide-lipid nanoparticle, LP-LNP) with novel lipopeptides as adjuvants, and initially explore their synergistic effect on mRNA vaccines. Methods Two novel lipopeptides, SS-10 and SQ18, were designed and synthesized. Microfluidic technology was used to encapsulate lipopeptides in different proportions, as well as mRNAs encoding enhanced green fluorescent protein (eGFP), firefly luciferase (F-luc), and ovalbumin (OVA) into lipid nanoparticles to construct an mRNA delivery system with novel lipopeptides as adjuvants (LP-LNP). The particle size and polydispersity coefficient of LP-LNP were measured using dynamic light scattering. The activation effect on Toll-like receptors 2 (TLR2) was detected using HEK-BlueTM mTLR2 reporter cells to screen the optimal lipopeptide ratio. The preferred LP-LNP-eGFP-mRNA was transfected into HEK293T cells, and the expression of eGFP was observed under a fluorescence microscope. In vivo imaging was used to investigate the expression level of LP-LNP-F-luc-mRNA in mice. Flow cytometry was used to evaluate the ability of LP-LNP-OVA-mRNA to induce the maturation of dendritic cells (DCs) in draining lymph nodes and cross-presentation of antigens after immunization. Results Lipopeptides SQ18 and SS-10 were incorporated into LNP at 0.50% and 0.75% molar ratios, respectively, to obtain LP-LNP with uniform particle size, high encapsulation efficiency, and good in vitro safety. The ability of this formulation to activate TLR2 was significantly stronger than the positive control Pam2CSK4 (P < 0.01). The preferred LP-LNP obtained effective in vitro transfection, and LP-LNP prepared with SQ18 at 0.50% molar ratio had significantly better in vivo transfection efficiency than traditional LNP (P < 0.01), and significantly promoted the maturation of DCs in draining lymph nodes and cross-presentation of antigens (P < 0.05). Conclusion LP-LNP with novel lipopeptides as adjuvants can enhance the delivery capacity of mRNA and further improve the immune effect of mRNA vaccines.

Published in 陆军军医大学学报

ISSN: 2097-0927 (Print)
Publisher: Editorial Office of Journal of Army Medical University
Country of publisher: China
LCC subjects: Medicine: Medicine (General)
Website: http://aammt.tmmu.edu.cn/

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