# PA-21-259, SBIR, Phase I, Self-Amplifying RNA Replicon-Based Platform for Generating Multivalent Influenza Vaccine

> **NIH ALLCDC R43** · CAROGEN CORPORATION · 2022 · $263,991

## Abstract

PROJECT ABSTRACT
Current vaccines are mainly strain-specific and have limited efficacy in preventing new, potentially pandemic
influenza strains. Interest in a universal influenza vaccine (UIV) to prevent future pandemics has been greatly
boosted by the success of mRNA-based coronavirus vaccines. However, developing a UIV has been particularly
challenging for two reasons: (1) the failure of immunization to induce broadly neutralizing antibodies against
conserved epitopes and (2) the lack of a safe and effective vaccine platform to induce broad and long-lasting
immunity. Virus-like vesicles (VLVs) are infectious, self-propagating alphavirus-vesiculovirus hybrid vaccine vectors
that can be engineered to express foreign antigens to elicit a protective immune response. These self-amplifying
RNA replicons are safe, highly immunogenic, and scalable to produce. The goal of this proposal is to rationally
design and engineer a VLV to express multiple flu antigens and thus induce broad and long-lasting immunity. As
shown in our published studies, the ectodomain of M2 (M2e) and domains of the immunodominant hemagglutinin
(HA) globular head can elicit robust antibody responses that mitigate disease and protect mice from lethal challenge.
We have also established that VLV carrying RNA encoding one or more of the major antigens of hepatitis B virus
(HBV) in a single open reading frame drives a broad multi-specific immune response that results in substantial
clearance of HBV in the mouse liver. Recent improvements in the development of this VLV immunotherapy vector
enhanced gene expression with a concomitant increase in both T-cell responses and antibodies. In preliminary
studies, we found that signal sequences promote efficient secretion of recombinant proteins that are highly
conserved among influenza strains, i.e., M2e, nucleoprotein, the long-alpha helix (LAH) of subunit 2 of HA, and
fusion peptide from VLV-infected cells. Our initial single-dose screening of individual flu antigen VLV vaccines
(sponsored by the Respiratory Diseases Branch of NIAID/NIH) showed promising mitigation of disease progression.
A reduction in lung virus titer was apparent in HA2 VLV vaccines. Albeit low, viral neutralizing titers (VNTs) were
present in all immunized groups (>1:16). In addition, our serological data show an increased induction of IgG1 and
IgG2a in most flu-based VLV-immunized groups. These virus-specific IgG isotypes correlate better with vaccine
efficacy than neutralization alone. We will carry out three specific aims: Aim 1. Characterize the immunogenicity of
VLV-Multi-Ag constructs in mice. Aim 2. Evaluate vaccine efficacy in a lethal influenza mouse model. Aim 3.
Evaluate prime-boost regimens to optimize flu-specific immune responses. The results of these studies will provide
initial data on the feasibility of developing a UIV. VLV-mediated delivery of multi-antigens targeting multiple epitopes
of conserved proteins may provide an effective strategy to prevent ...

## Key facts

- **NIH application ID:** 10611056
- **Project number:** 1R43IP001228-01
- **Recipient organization:** CAROGEN CORPORATION
- **Principal Investigator:** Valerian Nakaar
- **Activity code:** R43 (R01, R21, SBIR, etc.)
- **Funding institute:** ALLCDC
- **Fiscal year:** 2022
- **Award amount:** $263,991
- **Award type:** 1
- **Project period:** 2023-09-30 → 2024-09-29

## Primary source

NIH RePORTER: https://reporter.nih.gov/project-details/10611056

## Citation

> US National Institutes of Health, RePORTER application 10611056, PA-21-259, SBIR, Phase I, Self-Amplifying RNA Replicon-Based Platform for Generating Multivalent Influenza Vaccine (1R43IP001228-01). Retrieved via AI Analytics 2026-05-27 from https://api.ai-analytics.org/grant/nih/10611056. Licensed CC0.

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