Viruses (Feb 2019)

Induction of Tier 1 HIV Neutralizing Antibodies by Envelope Trimers Incorporated into a Replication Competent Vesicular Stomatitis Virus Vector

  • C. Anika Bresk,
  • Tamara Hofer,
  • Sarah Wilmschen,
  • Marina Krismer,
  • Anja Beierfuß,
  • Grégory Effantin,
  • Winfried Weissenhorn,
  • Michael J. Hogan,
  • Andrea P. O. Jordan,
  • Rebecca S. Gelman,
  • David C. Montefiori,
  • Hua-Xin Liao,
  • Joern E. Schmitz,
  • Barton F. Haynes,
  • Dorothee von Laer,
  • Janine Kimpel

DOI
https://doi.org/10.3390/v11020159
Journal volume & issue
Vol. 11, no. 2
p. 159

Abstract

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A chimeric vesicular stomatitis virus with the glycoprotein of the lymphocytic choriomeningitis virus, VSV-GP, is a potent viral vaccine vector that overcomes several of the limitations of wild-type VSV. Here, we evaluated the potential of VSV-GP as an HIV vaccine vector. We introduced genes for different variants of the HIV-1 envelope protein Env, i.e., secreted or membrane-anchored, intact or mutated furin cleavage site or different C-termini, into the genome of VSV-GP. We found that the addition of the Env antigen did not attenuate VSV-GP replication. All HIV-1 Env variants were expressed in VSV-GP infected cells and some were incorporated very efficiently into VSV-GP particles. Crucial epitopes for binding of broadly neutralizing antibodies against HIV-1 such as MPER (membrane-proximal external region), CD4 binding site, V1V2 and V3 loop were present on the surface of VSV-GP-Env particles. Binding of quaternary antibodies indicated a trimeric structure of VSV-GP incorporated Env. We detected high HIV-1 antibody titers in mice and showed that vectors expressing membrane-anchored Env elicited higher antibody titers than vectors that secreted Envs. In rabbits, Tier 1A HIV-1 neutralizing antibodies were detectable after prime immunization and titers further increased after boosting with a second immunization. Taken together, VSV-GP-Env is a promising vector vaccine against HIV-1 infection since this vector permits incorporation of native monomeric and/or trimeric HIV-1 Env into a viral membrane.

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