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Development of a Marburgvirus subunit vaccineadjuvanted with a novel TLR7/TLR8 agonist

  • Funded by National Institutes of Health (NIH)
  • Total publications:0 publications

Grant number: 1R43AI181292-01

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Key facts

  • Disease

    Marburg virus disease

  • Start & end year

    2024
    2026

  • Known Financial Commitments (USD)

    $299,528

  • Funder

    National Institutes of Health (NIH)

  • Principal Investigator

    DIRECTOR Shweta Kailasan

  • Research Location

    United States of America

  • Lead Research Institution

    ABVACC, INC.

  • Research Priority Alignment

    N/A

  • Research Category

    Vaccines research, development and implementation

  • Research Subcategory

    Pre-clinical studies

  • Special Interest Tags

    N/A

  • Study Type

    Non-Clinical

  • Clinical Trial Details

    N/A

  • Broad Policy Alignment

    Pending

  • Age Group

    Not Applicable

  • Vulnerable Population

    Not applicable

  • Occupations of Interest

    Not applicable

Abstract

There is an outbreak of Marburg virus disease (MVD), relative of Ebola virus, currently ongoing in Equatorial Guinea and Tanzania. There have been multiple, deadly outbreaks of MVD in the past with ~88% lethality. There are currently no approved vaccines or therapeutics for MVD and very few in clinical development. In this proposal, we have rationally designed an immunogen based on MARV glycoprotein (GP) by excluding domains known to trigger non-neutralizing antibodies allowing exposure of key neutralizing epitopes capable of generating a strong immune response. Combined with a novel TLR7/8 agonist adjuvant, Alhydroxyquim- II (AhQ-II), that has shown excellent safety and adjuvant activity in millions of people during COVID-19 pandemic, our rationally designed MARV vaccine induces broadly neutralizing antibodies against isolates Angola, CI67, and Musoke strains of MARV as well as the phylogenetically more distant RAVV. Mice immunized with this MARV vaccine with two or three doses compared to unadjuvanted antigen showed robust antigen-specific binding and neutralizing titers against all four MARV strains demonstrated by ELISA and pseudovirus neutralization assays. In the guinea pig model of MARV infection which shows all hallmarks of filovirus disease the vaccine provided 100% protection against lethal challenge with no detectable viremia, suggesting that the vaccine is likely inducing sterilizing immunity. In summary, this subunit vaccine represents a novel, highly efficacious, and safe candidate for protection against MVD. Here, we propose three specific aims to further develop this rationally designed immunogen: Aim1: To produce and generate a pooled stable cell line for the MARV subunit antigen with a cGMP-compliant tag and demonstrate biochemical and immunogenic properties comparable to the Streptavidin-tagged MARV material used in preliminary studies; Aim 2: to determine optimal effective dose and regimen for maximum protection in BSL-4 guinea pig MARV model; Aim 3: to demonstrate immunogenicity in the filovirus Gold Standard non-human primate model. Upon successful completion of this Phase I project we anticipate a Phase II focused on NHP efficacy studies and advanced development activities.