Abstract

A major goal of this proposal is to develop a novel experimental paradigm to engineer preventative HIV-1 vaccines. The V1/V2 domain of HIV-1 envelope is an important target for vaccine development for several reasons. V2 interaction with the ?4?7 integrin of mucosal T cells may play a key role in the efficient capture of HIV-1 virus at the site of initial exposure during sexual transmission. The V1/V2 domain is also a key player in regulating neutralization sensitivity of HIV-1, and consists of epitopes recognized by some of the most potent broadly neutralizing antibodies reported to date. Here, we hypothesize that induction of antibodies by vaccination with V1/V2 immunogens that interferes, specifically with the V2 ?4?7 interactions, confers protection against HIV-1 acquisition. Since the conformation of V2 is highly variable, the V2 domain will be constrained by transplanting it into the compactly folded 9 kDa small outer capsid protein (Soc) from bacteriophage T4. To select for the functionally important V2 conformations, libraries of V2 domain variants consisting of founder/acute virus sequences, different glycosylation patterns, and random mutations will be constructed and expressed in CHO cells as secretory proteins. High throughput assays will be developed, one to select ?4?7 binding conformations and another to select V2 conformational antibody binding variants. The biologically active Soc-V2 conformational variants will be arrayed on phage T4 nanoparticles by incubating the purified Soc-V2 proteins with Soc-minus Hoc-minus phage, up to 870 copies per particle. A Hoc- fused targeting ligand such as Dec205 mAb will also be assembled on the same capsid, up to 155 copies per capsid, to target the T4-V2 nanoparticles to the antigen-presenting dendritic cells. The immunogenicity of T4-V2 nanoparticles will be evaluated in mice by intramuscular route as well as transcutaneous (skin) route using heat labile enterotoxin as an adjuvant. The immune responses will be quantified for V2- ?4?7 interfering antibodies, virus neutralizing antibodies and transmission-blocking antibodies. The best V2 variants down-selected from these assays will then be tested in the rabbit model. A novel HIV-1 transmission assay will be developed, which will precisely quantify the number of virus genomes that cross the host membrane after a few minutes of exposure to CD4+, ?4?7+ and CCR5+ T cells. Based on real-time PCR, this assay would be extremely sensitive, rapid, and high throughput. Using this assay, V2 variants that can induce antibodies which block virus entry by interfering with the initial virus-host interactions will be selected. These might potentially serve as preventative HIV-1 vaccine candidates for further studies in nonhuman primates and clinical trials.

Public Health Relevance

The mechanism of HIV transmission at the site of exposure and how to develop vaccines that can prevent it remained as key goals in the development of preventative HIV vaccines. This proposal aims to analyze one of the HIV envelope components, the V1/V2 domain, which is involved in the initial interactions between the virus and the host. Using a combination of bacteriophage T4 display, molecular genetics, high throughput screening, and a new HIV transmission assay, V1/V2 nanoparticle immunogens that can induce transmission blocking antibodies will be selected as potential HIV preventative vaccines.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Allergy and Infectious Diseases (NIAID)
Type
Research Project (R01)
Project #
5R01AI102725-04
Application #
8868023
Study Section
Special Emphasis Panel (ZAI1)
Program Officer
Butler, Robert C
Project Start
2012-07-01
Project End
2017-06-30
Budget Start
2015-07-01
Budget End
2017-06-30
Support Year
4
Fiscal Year
2015
Total Cost
Indirect Cost

  Institution

Name
Catholic University of America
Department
Biology
Type
Schools of Arts and Sciences
DUNS #
041962788
City
Washington
State
DC
Country
United States
Zip Code
20064

  Publications

Kim, Jiae; Jobe, Ousman; Peachman, Kristina K et al. (2017) Quantitative analyses reveal distinct sensitivities of the capture of HIV-1 primary viruses and pseudoviruses to broadly neutralizing antibodies. Virology 508:188-198
Chand, Subhash; Messina, Emily L; AlSalmi, Wadad et al. (2017) Glycosylation and oligomeric state of envelope protein might influence HIV-1 virion capture by ?4?7 integrin. Virology 508:199-212
Jobe, Ousman; Trinh, Hung V; Kim, Jiae et al. (2016) Effect of cytokines on Siglec-1 and HIV-1 entry in monocyte-derived macrophages: the importance of HIV-1 envelope V1V2 region. J Leukoc Biol 99:1089-106
Jobe, Ousman; Kim, Jiae; Rao, Mangala (2016) The role of Siglec-1 in HIV-1/macrophage interaction. Macrophage (Houst) 3:
AlSalmi, Wadad; Mahalingam, Marthandan; Ananthaswamy, Neeti et al. (2015) A New Approach to Produce HIV-1 Envelope Trimers: BOTH CLEAVAGE AND PROPER GLYCOSYLATION ARE ESSENTIAL TO GENERATE AUTHENTIC TRIMERS. J Biol Chem 290:19780-95
Allam, Atef; Majji, Sai; Peachman, Kristina et al. (2015) TFH cells accumulate in mucosal tissues of humanized-DRAG mice and are highly permissive to HIV-1. Sci Rep 5:10443
Rao, Mangala; Peachman, Kristina K; Kim, Jiae et al. (2013) HIV-1 variable loop 2 and its importance in HIV-1 infection and vaccine development. Curr HIV Res 11:427-38
Gao, Guofen; Wieczorek, Lindsay; Peachman, Kristina K et al. (2013) Designing a soluble near full-length HIV-1 gp41 trimer. J Biol Chem 288:234-46
Tao, Pan; Mahalingam, Marthandan; Marasa, Bernard S et al. (2013) In vitro and in vivo delivery of genes and proteins using the bacteriophage T4 DNA packaging machine. Proc Natl Acad Sci U S A 110:5846-51
Peachman, Kristina K; Li, Qin; Matyas, Gary R et al. (2012) Anthrax vaccine antigen-adjuvant formulations completely protect New Zealand white rabbits against challenge with Bacillus anthracis Ames strain spores. Clin Vaccine Immunol 19:11-6

Showing the most recent 10 out of 13 publications