Abstract

From the analysis of extensive nucleotide sequence data available for the env and gag genes of HIV-1, it has become clear that six subtypes of the virus can be identified. However, the immunologic relatedness of these various HIV-1 subtypes has not yet been examined. We propose to determine if serotypes of the virus exist, and if these serotypes parallel or diverge from the aforementioned sequence-based subtypes. Moreover, we will investigate whether intra-typic groups can be identified immunologically. To do this, we plan, first, to use several of the 60 anti-HIV human monoclonal antibodies (mAbs) which have been produced in our laboratory. These mAbs were induced by viral proteins during the course of natural human infection with HIV-1, Type B (the subtype which predominates in the United States). These mAbs were selected on the basis of their reactivity with Type B-HIV-1; they are specific for various regions of gp120, gp41, p24 and p17. Particular emphasis will be placed on studies of mAbs specific for the V3 loop and the CD4 binding domain of gp120, two epitopes in the extracellular domain of gp41, and various regions of p24. All of these mAbs will be tested for their ability to bind to viral lysates prepared from primary isolates of each of the six HIV-1 subtypes. Relevant anti-gp 120 nd gp41 mAbs will be tested as well for their ability to bind to the surface of infected cells and to neutralize and lyse viral specimens. In addition to determining whether these reagents can illuminate serotypes and intra-typic viral classes, we will determine if these mAbs can distinguish between various phenotypic groups of HIV-1 such as macrophage-tropic and T-cell tropic strains. Next, we propose to produce new human mAbs that will be selected on the other (non-Type B) HIV- 1 subtypes. These new mAbs will be characterized with respect to (a) their immunochemical reactivity, i.e., their epitopes, conformation-dependence, Kd, koo, etc.. (b) their biologic function, i.e., neutralizing and virolytic activity, and (c) their ability to distinguish and/or cross-react with diverse viral serotypes. The data generated using these various mAbs and viral subtypes will be analyzed by cluster analysis and other defined statistical techniques. This analysis will generate an immunologic classification scheme which will permit the various primary isolates from around the world to be divided into serotypes and intra-typic groups. This immunologic classification will be compared to tahe genotypic classification. Those mAbs which we identify as most useful for distinguishing serotypes and intra-typic groups will be selected for use in a serotyping panel which will be made available tot he scientific community for large-scale studies of global primary isolates. The immunologic classification scheme and the reagents that will be generated will be critical to the design of global strategies for the development of HIV vaccines and the selection of reagents for use in passive immunization to prevent the transmission of HIV-1.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Allergy and Infectious Diseases (NIAID)
Type
Research Project (R01)
Project #
5R01AI036085-04
Application #
2413679
Study Section
AIDS and Related Research Study Section 1 (ARRA)
Project Start
1994-08-01
Project End
1998-09-14
Budget Start
1997-05-01
Budget End
1998-09-14
Support Year
4
Fiscal Year
1997
Total Cost
Indirect Cost

  Institution

Name
New York University
Department
Pathology
Type
Schools of Medicine
DUNS #
City
New York
State
NY
Country
United States
Zip Code
10016

  Publications

Li, Liuzhe; Wang, Xiao-Hong; Williams, Constance et al. (2015) A broad range of mutations in HIV-1 neutralizing human monoclonal antibodies specific for V2, V3, and the CD4 binding site. Mol Immunol 66:364-74
Yu, Xuesong; Gilbert, Peter B; Hioe, Catarina E et al. (2012) Statistical approaches to analyzing HIV-1 neutralizing antibody assay data. Stat Biopharm Res 4:1-13
Agarwal, Alpna; Hioe, Catarina E; Swetnam, James et al. (2011) Quantitative assessment of masking of neutralization epitopes in HIV-1. Vaccine 29:6736-41
Changela, Anita; Wu, Xueling; Yang, Yongping et al. (2011) Crystal structure of human antibody 2909 reveals conserved features of quaternary structure-specific antibodies that potently neutralize HIV-1. J Virol 85:2524-35
Spurrier, Brett; Sampson, Jared M; Totrov, Maxim et al. (2011) Structural analysis of human and macaque mAbs 2909 and 2.5B: implications for the configuration of the quaternary neutralizing epitope of HIV-1 gp120. Structure 19:691-9
Ringe, Rajesh; Sharma, Deepak; Zolla-Pazner, Susan et al. (2011) A single amino acid substitution in the C4 region in gp120 confers enhanced neutralization of HIV-1 by modulating CD4 binding sites and V3 loop. Virology 418:123-32
Musich, Thomas; Peters, Paul J; Duenas-Decamp, Maria José et al. (2011) A conserved determinant in the V1 loop of HIV-1 modulates the V3 loop to prime low CD4 use and macrophage infection. J Virol 85:2397-405
Gorny, Miroslaw K; Sampson, Jared; Li, Huiguang et al. (2011) Human anti-V3 HIV-1 monoclonal antibodies encoded by the VH5-51/VL lambda genes define a conserved antigenic structure. PLoS One 6:e27780
Shmelkov, Evgeny; Nadas, Arthur; Swetnam, James et al. (2011) Indirect detection of an epitope-specific response to HIV-1 gp120 immunization in human subjects. PLoS One 6:e27279
Zolla-Pazner, Susan; Kong, X-P; Jiang, Xunqing et al. (2011) Cross-clade HIV-1 neutralizing antibodies induced with V3-scaffold protein immunogens following priming with gp120 DNA. J Virol 85:9887-98

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