Abstract

The membrane proximal external region (MPER) of HIV gp41 comprises a highly conserved region involved in HIV viral fusion. It is an important target of antibody (Ab)-mediated neutralization as it contains epitopes for two broadly (b) neutralizing (Nt) monoclonal (M) Abs (2F5 and 4E10) and two MAbs that neutralize a significant, but not truly broad, range of HIV isolates (Z13 and m66.6), making the MPER an obvious target for an AIDS vaccine. However, all attempts to produce an MPER-targeting vaccine have failed. Most of these vaccines have been of three types: (i) synthetic peptides;(ii) MPER sequence grafted onto protein scaffolds;or (iii) onto proteins displayed on virus-like particles. In explaiing these failures, we hypothesize that previous vaccines have not faithfully mimicked the neutralization competent structure (NCS) of the MPER. Our preliminary work has shown that the gp41 transmembrane domain (TMD) is required for the full exposure of the MPER, since its replacement with the TMD from another membrane protein, decreases binding by MAb 4E10. Drs. Scott and Lu previously collaborated on producing a DNA vaccine that expresses a gp41 fragment comprising the MPER and TMD, so as to present the MPER in the context of the cell membrane. However, repeated immunization of rabbits with this DNA vaccine elicited low titer Abs that cross-reacted weakly with MPER peptides and did not neutralize virus;boosting immunizations with a virus-like particle vaccine did not improve anti-MPER titers, probably because of low MPER copy number. We propose to design more effective protein-boost immunogens that will mimic the NCS.
In specific aim 1 we plan to design liposome and nanoparticle immunogens that present the gp41 MPER+TMD in high copy number in lipid bilayers, so as to better mimic the NCS of the MPER without added proteins that might """"""""distract"""""""" the Ab response. We will produce DNA, liposome and nanoparticle candidates that have optimized the: (i) MPER, (ii) TMD, and (iii) composition of the lipid environment, based on relative binding affinity by bNt MAbs, the absence of binding by non-Nt mutants of the bNt MAbs, their behavior in a novel membrane leakage assay, and structural stabilization.
In specific aim 2 optimized DNA, liposome and nanoparticle candidates will be produced and tested for their ability to elicit MPER-binding activities and Nt Abs. The optimized liposome and nanoparticle vaccines will then be tested as protein boosts (i.e., following DNA priming) with the goal of maximizing MPER-specific Ab titers and Nt potency and breadth. In addition, antigenicity, immunogenicity and structural data will be used to develop a molecular model of the MPER NCS, which should support future vaccine design.

Public Health Relevance

The membrane proximal external region of the envelope protein gp41 (MPER) is a highly conserved region on the trimeric spike of infectious HIV-1, and a target of antibodies that neutralize a broad range of HIV-1 isolates. When used as a passive vaccine in monkeys, these antibodies protect against infection by HIV-like viruses;however so far there is no vaccine that can elicit such antibodies. Our goal is to produce a vaccine that will mimic the structure of the MPER on the infectious spike, and in so doing, will elicit antibodies that prevent infection by a broad spectrum of HIV-1 isolates;providing the important first steps in achieving a successful AIDS vaccine.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Allergy and Infectious Diseases (NIAID)
Type
Research Project (R01)
Project #
4R01AI097051-02
Application #
8431276
Study Section
HIV/AIDS Vaccines Study Section (VACC)
Program Officer
Schultz, Alan M
Project Start
2012-03-01
Project End
2016-02-29
Budget Start
2013-03-01
Budget End
2014-02-28
Support Year
2
Fiscal Year
2013
Total Cost
$648,324
Indirect Cost
$48,024

  Institution

Name
Simon Fraser University
Department
Type
DUNS #
208032946
City
Burnaby
State
BC
Country
Canada
Zip Code
V5 1-S6

  Publications

Rujas, Edurne; Caaveiro, José M M; Insausti, Sara et al. (2017) Peripheral Membrane Interactions Boost the Engagement by an Anti-HIV-1 Broadly Neutralizing Antibody. J Biol Chem 292:5571-5583
Chojnacki, Jakub; Waithe, Dominic; Carravilla, Pablo et al. (2017) Envelope glycoprotein mobility on HIV-1 particles depends on the virus maturation state. Nat Commun 8:545
Rujas, Edurne; Insausti, Sara; García-Porras, Miguel et al. (2017) Functional Contacts between MPER and the Anti-HIV-1 Broadly Neutralizing Antibody 4E10 Extend into the Core of the Membrane. J Mol Biol 429:1213-1226
Carravilla, Pablo; Cruz, Antonio; Martin-Ugarte, Itziar et al. (2017) Effects of HIV-1 gp41-Derived Virucidal Peptides on Virus-like Lipid Membranes. Biophys J 113:1301-1310
Rujas, Edurne; Gulzar, Naveed; Morante, Koldo et al. (2016) Reply to ""The Broadly Neutralizing, Anti-HIV Antibody 4E10: an Open and Shut Case?"". J Virol 90:3276-7
Rujas, Edurne; Caaveiro, Jose M M; Partida-Hanon, Angélica et al. (2016) Structural basis for broad neutralization of HIV-1 through the molecular recognition of 10E8 helical epitope at the membrane interface. Sci Rep 6:38177
Huarte, Nerea; Carravilla, Pablo; Cruz, Antonio et al. (2016) Functional organization of the HIV lipid envelope. Sci Rep 6:34190
Apellániz, Beatriz; Rujas, Edurne; Serrano, Soraya et al. (2015) The Atomic Structure of the HIV-1 gp41 Transmembrane Domain and Its Connection to the Immunogenic Membrane-proximal External Region. J Biol Chem 290:12999-3015
Walsh, Joseph D; Chu, Shidong; Zhang, Shao-Qing et al. (2015) Design and characterization of swapped-domain constructs of HIV-1 glycoprotein-41 as receptors for drug discovery. Protein Eng Des Sel 28:107-16
Apellániz, Beatriz; Nieva, José L (2015) Fusion-competent state induced by a C-terminal HIV-1 fusion peptide in cholesterol-rich membranes. Biochim Biophys Acta 1848:1014-22

Showing the most recent 10 out of 16 publications