Abstract

The clinical course of HIV infection is unpredictable and highly variable. HIV infected persons may live without symptoms for years or may succumb to opportunistic infections or cancer within a short time. We propose to study the controlling factors in the immune response to the HIV at the level of idiotypic network. Since the immune response to HIV is like any other immune response under network control, analysis of the idiotype/anti- idiotype interactions in the patient reflects the immunological state in the disease and provides useful parameters for predicting the further course of the infection. Specifically, we will analyze the immune response to the gp120 envelope in HIV positive individuals, ARC and AIDS patients. Antibodies against gp120 from these groups will be immortalized by """"""""rescue"""""""" human-mouse fusion. Monoclonal mouse anti-idiotypic antibodies will be generated against these human anti-gp120 antibodies. These monoclonal anti-idiotypes will be used as probes for the idiotype regulatory network in HIV individuals and patients. Human sera from HIV positive individuals and patients will be screened for binding to monoclonal anti-idiotype probes by ELISA and Western blots after isoelectrofocusing. Inhibition of anti-idiotype binding in the presence of gp120 protein will indicate which of these idiotopes are regulatory (Ag-, Id+). By employing a panel of anti- idiotypes we will try to establish correlations between expression of idiotypes and the clinical stage. Such correlations will produce predictive parameters for the course of the HIV infection. The role of the genetic variability of the HIV envelope in the idiotype network control will be addressed by isolating a panel of HIV gp120 variants from patients under study and by using vector expression envelope proteins from the different prototype sequence variants (see Project 1). Variant gp120 will be used to """"""""rescue"""""""" human anti-gp120 antibodies and to generate anti- idiotypes. These studies will provide important information on the immunological state of the HIV infected patient and thus will produce predictive parameters for the future course of the disease. Although the analysis of the idiotypic regulation will be done initially on a small number of patients correlative trends in idiotypic patterns with disease stage are expected. The panel of anti-idiotypic and idiotypic probes will then be made available to other AIDS research centers for further testing. Predictive data will be useful in choosing appropriate anti-viral or other therapies.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Allergy and Infectious Diseases (NIAID)
Type
Research Project--Cooperative Agreements (U01)
Project #
5U01AI025721-03
Application #
3814673
Study Section
Project Start
Project End
Budget Start
Budget End
Support Year
3
Fiscal Year
1989
Total Cost
Indirect Cost

  Institution

Name
State University of New York at Buffalo
Department
Type
DUNS #
038633251
City
Buffalo
State
NY
Country
United States
Zip Code
14260

  Publications

Dundr, M; Meier, U T; Lewis, N et al. (1997) A class of nonribosomal nucleolar components is located in chromosome periphery and in nucleolus-derived foci during anaphase and telophase. Chromosoma 105:407-17
Dundr, M; Leno, G H; Lewis, N et al. (1996) Location of the HIV-1 Rev protein during mitosis: inactivation of the nuclear export signal alters the pathway for postmitotic reentry into nucleoli. J Cell Sci 109 ( Pt 9):2239-51
Berkowitz, R D; Hammarskjold, M L; Helga-Maria, C et al. (1995) 5' regions of HIV-1 RNAs are not sufficient for encapsidation: implications for the HIV-1 packaging signal. Virology 212:718-23
Srinivasakumar, N; Hammarskjold, M L; Rekosh, D (1995) Characterization of deletion mutations in the capsid region of human immunodeficiency virus type 1 that affect particle formation and Gag-Pol precursor incorporation. J Virol 69:6106-14
Dundr, M; Leno, G H; Hammarskjold, M L et al. (1995) The roles of nucleolar structure and function in the subcellular location of the HIV-1 Rev protein. J Cell Sci 108 ( Pt 8):2811-23
Mak, J; Jiang, M; Wainberg, M A et al. (1994) Role of Pr160gag-pol in mediating the selective incorporation of tRNA(Lys) into human immunodeficiency virus type 1 particles. J Virol 68:2065-72
Hammarskjold, M L; Li, H; Rekosh, D et al. (1994) Human immunodeficiency virus env expression becomes Rev-independent if the env region is not defined as an intron. J Virol 68:951-8
Bray, M; Prasad, S; Dubay, J W et al. (1994) A small element from the Mason-Pfizer monkey virus genome makes human immunodeficiency virus type 1 expression and replication Rev-independent. Proc Natl Acad Sci U S A 91:1256-60
Smith, A J; Srinivasakumar, N; Hammarskjold, M L et al. (1993) Requirements for incorporation of Pr160gag-pol from human immunodeficiency virus type 1 into virus-like particles. J Virol 67:2266-75
Keefer, M C; Bonnez, W; Roberts Jr, N J et al. (1991) Human immunodeficiency virus (HIV-1) gp160-specific lymphocyte proliferative responses of mononuclear leukocytes from HIV-1 recombinant gp160 vaccine recipients. J Infect Dis 163:448-53

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