Frontiers in Immunology (Feb 2021)

Modified Adenovirus Prime-Protein Boost Clade C HIV Vaccine Strategy Results in Reduced Viral DNA in Blood and Tissues Following Tier 2 SHIV Challenge

  • Delphine C. Malherbe,
  • Lo Vang,
  • Jason Mendy,
  • Philip T. Barnette,
  • David A. Spencer,
  • Jason Reed,
  • Bettie W. Kareko,
  • D. Noah Sather,
  • D. Noah Sather,
  • Shilpi Pandey,
  • Constantinos K. Wibmer,
  • Constantinos K. Wibmer,
  • Harlan Robins,
  • Deborah H. Fuller,
  • Byung Park,
  • Samir K. Lakhashe,
  • Samir K. Lakhashe,
  • James M. Wilson,
  • Michael K. Axthelm,
  • Ruth M. Ruprecht,
  • Ruth M. Ruprecht,
  • Penny L. Moore,
  • Penny L. Moore,
  • Penny L. Moore,
  • Penny L. Moore,
  • Jonah B. Sacha,
  • Jonah B. Sacha,
  • Jonah B. Sacha,
  • Ann J. Hessell,
  • Jeff Alexander,
  • Nancy L. Haigwood,
  • Nancy L. Haigwood

DOI
https://doi.org/10.3389/fimmu.2020.626464
Journal volume & issue
Vol. 11

Abstract

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Designing immunogens and improving delivery methods eliciting protective immunity is a paramount goal of HIV vaccine development. A comparative vaccine challenge study was performed in rhesus macaques using clade C HIV Envelope (Env) and SIV Gag antigens. One group was vaccinated using co-immunization with DNA Gag and Env expression plasmids cloned from a single timepoint and trimeric Env gp140 glycoprotein from one of these clones (DNA+Protein). The other group was a prime-boost regimen composed of two replicating simian (SAd7) adenovirus-vectored vaccines expressing Gag and one Env clone from the same timepoint as the DNA+Protein group paired with the same Env gp140 trimer (SAd7+Protein). The env genes were isolated from a single pre-peak neutralization timepoint approximately 1 year post infection in CAP257, an individual with a high degree of neutralization breadth. Both DNA+Protein and SAd7+Protein vaccine strategies elicited significant Env-specific T cell responses, lesser Gag-specific responses, and moderate frequencies of Env-specific TFH cells. Both vaccine modalities readily elicited systemic and mucosal Env-specific IgG but not IgA. There was a higher frequency and magnitude of ADCC activity in the SAd7+Protein than the DNA+Protein arm. All macaques developed moderate Tier 1 heterologous neutralizing antibodies, while neutralization of Tier 1B or Tier 2 viruses was sporadic and found primarily in macaques in the SAd7+Protein group. Neither vaccine approach provided significant protection from viral acquisition against repeated titered mucosal challenges with a heterologous Tier 2 clade C SHIV. However, lymphoid and gut tissues collected at necropsy showed that animals in both vaccine groups each had significantly lower copies of viral DNA in individual tissues compared to levels in controls. In the SAd7+Protein-vaccinated macaques, total and peak PBMC viral DNA were significantly lower compared with controls. Taken together, this heterologous Tier 2 SHIV challenge study shows that combination vaccination with SAd7+Protein was superior to combination DNA+Protein in reducing viral seeding in tissues in the absence of protection from infection, thus emphasizing the priming role of replication-competent SAd7 vector. Despite the absence of correlates of protection, because antibody responses were significantly higher in this vaccine group, we hypothesize that vaccine-elicited antibodies contribute to limiting tissue viral seeding.

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