Abstract

Human respiratory syncytial virus (RSV) is the most important viral agent of pediatric respiratory tract disease worldwide and is responsible for a huge burden of morbidity and significant mortality. A licensed vaccine or effective antiviral therapy is unavailable. Obstacles to vaccine development include the poor growth of the virus in cell culture, the semi-permissive nature of infection in most animal models, the difficulty of achieving an appropriate balance between immunogenicity and attenuation, and the inefficiency of the immune response in the very young infant. We developed a method for producing infectious recombinant RSV by the intracellular coexpression of cDNAs encoding a complete RSV replicative intermediate RNA (antigenome) and the N, P, L and M2-1 proteins, which together constitute a nucleocapsid that is fully competent for RNA synthesis. This provides an important tool for basic molecular and pathogenesis studies as well as a method for fine-tuning the level of attenuation of candidate vaccine viruses. We showed that RSV encodes ten mRNAs and eleven unique proteins (the M2 mRNA contains two overlapping ORFs encoding the M2-1 and M2-2 proteins). Five RSV genes, namely NS1, NS2, SH, M2-2 and G, could be """"""""knocked out"""""""" (deleted) singly and in some cases in combination without ablating the ability of the virus to grow in cell culture. However, in most cases growth was less efficient. Deletion of the NS1 and NS2 genes singly or in combination was found to be highly attenuating in mice and chimpanzees. These deletions are candidates for inclusion in a live-attenuated vaccine. The M2-2 deletion virus exhibited a shift favoring transcription over replication. This implicates this protein as a regulatory factor in RNA synthesis. This mutation has the novel property of reducing growth while increasing, rather than decreasing, gene expression, and thus might make a vaccine that is """"""""better than nature"""""""". The G knockout virus demonstrated cell-specific differences in growth efficiency, implying that it is using an alternative receptor whose distribution is cell-specific. Thus, these findings have important implications for virus assembly and receptor usage. Fully-viable chimeric viruses were constructed between human RSVs representing the two antigenic subgroups, making it possible to use a single attenuated backbone to express the major antigenic determinants of each of the subgroups. Fully-viable chimeras also were constructed between human RSV and bovine RSV, a virus that has a host range restriction that renders it highly attenuated in primates and thus represents a new method of attenuating an RSV vaccine. As another approach to making an RSV vaccine """"""""better than nature"""""""", recombinant RSV was engineered to express various cytokines and chemokines in order to enhance immunogenicity and, in some cases, attenuate the virus.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Allergy and Infectious Diseases (NIAID)
Type
Intramural Research (Z01)
Project #
1Z01AI000372-18
Application #
6431557
Study Section
(LID)
Project Start
Project End
Budget Start
Budget End
Support Year
18
Fiscal Year
2000
Total Cost
Indirect Cost

  Institution

Name
Niaid Extramural Activities
Department
Type
DUNS #
City
State
Country
United States
Zip Code

  Publications

Buchholz, Ursula J; Ward, Jerrold M; Lamirande, Elaine W et al. (2009) Deletion of nonstructural proteins NS1 and NS2 from pneumonia virus of mice attenuates viral replication and reduces pulmonary cytokine expression and disease. J Virol 83:1969-80
Munir, Shirin; Le Nouen, Cyril; Luongo, Cindy et al. (2008) Nonstructural proteins 1 and 2 of respiratory syncytial virus suppress maturation of human dendritic cells. J Virol 82:8780-96
Collins, Peter L; Graham, Barney S (2008) Viral and host factors in human respiratory syncytial virus pathogenesis. J Virol 82:2040-55
Chapman, Joanna; Abbott, Elizabeth; Alber, Dagmar G et al. (2007) RSV604, a novel inhibitor of respiratory syncytial virus replication. Antimicrob Agents Chemother 51:3346-53
Krempl, Christine D; Wnekowicz, Anna; Lamirande, Elaine W et al. (2007) Identification of a novel virulence factor in recombinant pneumonia virus of mice. J Virol 81:9490-501
Vallbracht, Simone; Jessen, Birthe; Mrusek, Sonja et al. (2007) Influence of a single viral epitope on T cell response and disease after infection of mice with respiratory syncytial virus. J Immunol 179:8264-73
Harker, James; Bukreyev, Alexander; Collins, Peter L et al. (2007) Virally delivered cytokines alter the immune response to future lung infections. J Virol 81:13105-11
Chi, Bo; Dickensheets, Harold L; Spann, Kirsten M et al. (2006) Alpha and lambda interferon together mediate suppression of CD4 T cells induced by respiratory syncytial virus. J Virol 80:5032-40
Bukreyev, Alexander; Serra, Maria Elina; Laham, Federico R et al. (2006) The cysteine-rich region and secreted form of the attachment G glycoprotein of respiratory syncytial virus enhance the cytotoxic T-lymphocyte response despite lacking major histocompatibility complex class I-restricted epitopes. J Virol 80:5854-61
Kotelkin, Alexander; Belyakov, Igor M; Yang, Lijuan et al. (2006) The NS2 protein of human respiratory syncytial virus suppresses the cytotoxic T-cell response as a consequence of suppressing the type I interferon response. J Virol 80:5958-67

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