Enhancing toxin-based vaccines against botulism

Enhancing toxin-based vaccines against botulism

•In a mouse model of botulism, M-BoNT/A1 was not toxic at >106-fold greater amounts than native BoNT/A.•M-BoNT/A1(W1266A) (M-BoNT/A1W) was created to prevent neuronal cell binding.•M-BoNT/A1 vaccination protected against challenge by 106 LD50 of native BoNT/A1.•LCHCN elicited a higher neutralizin...

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Veröffentlicht in:Vaccine 2018-02, Vol.36 (6), p.827-832
Hauptverfasser: Przedpelski, Amanda, Tepp, William H., Zuverink, Madison, Johnson, Eric A., Pellet, Sabine, Barbieri, Joseph T.
Format: Artikel
Sprache:eng
Schlagworte:
Amino acids
Animals
Antibodies
Antibodies, Bacterial - immunology
Antibodies, Neutralizing - immunology
Antigens, Bacterial - immunology
Attachment
Bacterial Vaccines - immunology
Binding
Bioassays
Botulinum neurotoxin
Botulinum neurotoxin A1
Botulinum neurotoxin A2
Botulinum toxin
Botulinum Toxins - immunology
Botulism
Botulism - immunology
Botulism - prevention & control
Catalysis
Catalytic activity
Chains
Clostridium botulinum
Clostridium botulinum - immunology
Disease Models, Animal
E coli
ELISA
Enzyme-Linked Immunosorbent Assay
Epitopes - immunology
Escherichia coli
Experiments
Food contamination
Glycerol
Humans
Immune response
Immune system
Immunization
Immunoglobulins
Laboratories
Medical research
Mice
Mutation
Neurons - immunology
Neurons - metabolism
Neurotoxins
Neutralizing
Proteins
Recombinant Proteins
Toxicity
Toxins
Translocation
Vaccine
Vaccines
Waterborne diseases
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Zusammenfassung:•In a mouse model of botulism, M-BoNT/A1 was not toxic at >106-fold greater amounts than native BoNT/A.•M-BoNT/A1(W1266A) (M-BoNT/A1W) was created to prevent neuronal cell binding.•M-BoNT/A1 vaccination protected against challenge by 106 LD50 of native BoNT/A1.•LCHCN elicited a higher neutralizing antibody titer than HCC, showing neutralizing epitopes within LCHCN.•Engineered BoNT with defects in catalysis and receptor binding is a novel vaccine strategy against botulism. Botulinum neurotoxins (BoNT) are the most toxic proteins for humans. BoNTs are single chain proteins with an N-terminal light chain (LC) and a C-terminal heavy chain (HC). HC comprises a translocation domain (HCN) and a receptor binding domain (HCC). Currently, there are no approved vaccines against botulism. This study tests a recombinant, full-length BoNT/A1 versus LCHCN/A1 and HCC/A1 as vaccine candidates against botulism. Recombinant, full-length BoNT/A1 was detoxified by engineering 3-amino acid mutations (E224A/R363A/Y366F) (M-BoNT/A1) into the LC to eliminate catalytic activity, which reduced toxicity in a mouse model of botulism by >106-fold relative to native BoNT/A1. As a second step to improve vaccine safety, an additional mutation (W1266A) was engineered in the ganglioside binding pocket, resulting in reduced receptor binding, to produce M-BoNT/A1W. M-BoNT/A1W vaccination protected against challenge by 106 LD50 Units of native BoNT/A1, while M-BoNT/A1 or M-BoNT/A1W vaccination equally protected against challenge by native BoNT/A2, a BoNT subtype. Mice vaccinated with M-BoNT/A1W surviving BoNT challenge had dominant antibody responses to the LCHCN domain, but varied antibody responses to HCC. Sera from mice vaccinated with M-BoNT/A1W also neutralized BoNT/A1 action on cultured neuronal cells. The cell- and mouse-based assays measured different BoNT-neutralizing antibodies, where M-BoNT/A1W elicited a strong neutralizing response in both assays. Overall, M-BoNT/A1W, with defects in multiple toxin functions, elicits a potent immune response to BoNT/A challenge as a vaccine strategy against botulism and other toxin-mediated diseases.
ISSN:0264-410X
1873-2518
DOI:10.1016/j.vaccine.2017.12.064