Saponin adjuvant enhancement of antigen-specific immune responses to an experimental HIV-1 vaccine

Saponin adjuvant enhancement of antigen-specific immune responses to an experimental HIV-1 vaccine

The adjuvant activity of a single highly purified saponin from the soap bark tree Quillaja saponaria was evaluated by using it as a component in an experimental vaccine containing rHIV-1 envelope protein (HIV-1 160D) adsorbed to alum. BALB/c mice immunized with experimental vaccine formulations cont...

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Veröffentlicht in:The Journal of immunology (1950) 1992-03, Vol.148 (5), p.1519-1525
Hauptverfasser: Wu, JY, Gardner, BH, Murphy, CI, Seals, JR, Kensil, CR, Recchia, J, Beltz, GA, Newman, GW, Newman, MJ
Format: Artikel
Sprache:eng
Schlagworte:
Adjuvants, Immunologic - pharmacology
AIDS Vaccines - immunology
AIDS/HIV
Animals
Biological and medical sciences
Esterases - biosynthesis
Female
Fundamental and applied biological sciences. Psychology
Gene Products, env - immunology
HIV Antibodies - analysis
HIV Envelope Protein gp160
HIV-1 - immunology
human immunodeficiency virus 1
Lymphocyte Activation
Mice
Mice, Inbred BALB C
Microbiology
Protein Precursors - immunology
Saponins - pharmacology
Vaccines, antisera, therapeutical immunoglobulins and monoclonal antibodies
Vaccines, Synthetic - immunology
Virology
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Zusammenfassung:The adjuvant activity of a single highly purified saponin from the soap bark tree Quillaja saponaria was evaluated by using it as a component in an experimental vaccine containing rHIV-1 envelope protein (HIV-1 160D) adsorbed to alum. BALB/c mice immunized with experimental vaccine formulations containing the saponin adjuvant QS-21 produced significantly higher titers of antibodies than mice vaccinated with only the alum-adsorbed HIV-1 160D. Potent amnestic antibody responses to HIV-1 viral proteins were also induced. Ag-specific proliferative responses to recombinant proteins and to three variants of HIV-1 were significantly increased using QS-21 as an adjuvant. Alum-adsorbed HIV-1 160D failed to induce measurable proliferative responses to inactivated HIV-1 viruses, but group-specific proliferative responses were raised when the QS-21 adjuvant was used in the vaccine formulation. MHC class I restricted CTL specific for the immunodominant V-3 loop were induced but only when the QS-21 adjuvant was included in the vaccine formulation. The production of serine esterase by Ag-activated splenic mononuclear cells, indicating the maturation of precursor CTL, was used as a secondary measure of CTL activity, and this response was also increased. The specificity of antibody responses was not significantly broadened using QS-21; the adjuvant increased the immune recognition of epitopes throughout the HIV-1 glycoprotein 160. However, the specificity of the proliferation and serine esterase responses was broadened, suggesting that the QS-21 augmented cell-mediated immune responses specific for epitopes outside of the V-3 loop. Additionally, the QS-21 adjuvant appeared to induce recognition of weakly immunogenic epitopes that were not recognized using only alum-adsorbed HIV-1 160D. The ability of QS-21 to augment both antibody and cell-mediated immune responses suggests that this adjuvant could be a valuable component in subunit vaccines.
ISSN:0022-1767
1550-6606
DOI:10.4049/jimmunol.148.5.1519