Immunogenicity, Efficacy, and Safety of a Novel Synthetic Microparticle Pre-Erythrocytic Malaria Vaccine in Multiple Host Species

被引:0
作者
Powell, Thomas J. [1 ]
Tang, Jie [1 ]
Mitchell, Robert [2 ]
Derome, Mary E. [1 ,3 ]
Jacobs, Andrea [1 ]
Palath, Naveen [1 ,4 ]
Cardenas, Edwin [1 ]
Yorke, Michelle [1 ]
Boyd, James G. [1 ]
Kaba, Stephen A. [5 ,6 ]
Nardin, Elizabeth [2 ]
Tsuji, Moriya
机构
[1] Artificial Cell Technol Inc, 5 Sci Pk, Suite 13, New Haven, CT 06511 USA
[2] NYU, Sch Med, Dept Microbiol, New York, NY 10010 USA
[3] Multiple Myeloma Res Fdn, 383 Main Ave, 5th Floor, Norwalk, CT 06851 USA
[4] Pfizer Inc, Andover, MA 01810 USA
[5] Walter Reed Army Inst Res, Malaria Vaccine Branch, Silver Spring, MD 20910 USA
[6] GreenLight Biosci Inc, Lexington, MA 02421 USA
关键词
malaria vaccine; microparticle; non-human primate; peptide; sporozoite; T-CELL RESPONSES; PLASMODIUM-FALCIPARUM; CIRCUMSPOROZOITE PROTEIN; REPETITIVE EPITOPE; PHASE-3; TRIAL; LIVER STAGES; SPOROZOITES; PROTECTION; ANTIBODY; PARASITES;
D O I
10.3390/vaccines11121789
中图分类号
R392 [医学免疫学]; Q939.91 [免疫学];
学科分类号
100102 ;
摘要
We previously reported a protective antibody response in mice immunized with synthetic microparticle vaccines made using layer-by-layer fabrication (LbL-MP) and containing the conserved T1BT* epitopes from the P. falciparum circumsporozoite protein. To further optimize the vaccine candidate, a benchtop tangential flow filtration method (LbL-by-TFF) was developed and utilized to produce vaccine candidates that differed in the status of base layer crosslinking, inclusion of a TLR2 ligand in the antigenic peptide, and substitution of serine or alanine for an unpaired cysteine residue in the T* epitope. Studies in mice revealed consistent superiority of the Pam3Cys-modified candidates and a modest benefit of base layer crosslinking, as evidenced by higher and more persistent antibody titers (up to 18 months post-immunization), a qualitative improvement of T-cell responses toward a Th1 phenotype, and greater protection from live parasite challenges compared to the unmodified prototype candidate. Immunogenicity was also tested in a non-human primate model, the rhesus macaque. Base layer-crosslinked LbL-MP loaded with T1BT* peptide with or without covalently linked Pam3Cys elicited T1B-specific antibody responses and T1BT*-specific T-cell responses dominated by IFN gamma secretion with lower levels of IL-5 secretion. The Pam3Cys-modified construct was more potent, generating antibody responses that neutralized wild-type P. falciparum in an in vitro hepatocyte invasion assay. IgG purified from individual macaques immunized with Pam3Cys.T1BT* LbL-MP protected naive mice from challenges with transgenic P. berghei sporozoites that expressed the full-length PfCS protein, with 50-88% of passively immunized mice parasite-free for >= 15 days. Substitution of serine for an unpaired cysteine in the T* region of the T1BT* subunit did not adversely impact immune potency in the mouse while simplifying the manufacture of the antigenic peptide. In a Good Laboratory Practices compliant rabbit toxicology study, the base layer-crosslinked, Pam3Cys-modified, serine-substituted candidate was shown to be safe and immunogenic, eliciting parasite-neutralizing antibody responses and establishing the dose/route/regimen for a clinical evaluation of this novel synthetic microparticle pre-erythrocytic malaria vaccine candidate.
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