Abstract

The overall goal of our research effort is to define the genetic basis for infection and pathogenesis by particular feline leukemia virus (FeLV) variants. Experiments designed to address this question will be conducted using molecularly cloned FeLVs that we obtained directly from the tissues of cats with fatal immunodeficiency disease. These cloned variants have diverse pathogenicities in vitro and in vivo. The abilities of these variants to induce cytopathic effects (CPE) in a feline T cell line predicts their abilities to induce immunodeficiency disease in cats, thus providing an in vitro assay to study the pathogenic mechanisms of FeLV induced immunodeficiency disease. Several preliminary studies suggest that high levels of replication by immunodeficiency inducing FeLVs contributes to the cytopathic effects of these variants. Our results also suggest that the T cell cytopathic potential of FeLV variants may be determined at the level of transcription, splicing of viral RNA, and processing of the envelope polyprotein precursor. The proposed project will explore whether differences at the level of transcription and/or postranscriptional modification are determinants for the distinct pathogenicities of an immunodeficiency inducing FeLV(61C) and a closely related, but minimally pathogenic FeLV(61E). Viral sequences that determine differences in the cytopathic potential of these FeLVs will be identified. If the pathogenic potential of FeLV variants is determined at the level of transcription, the cellular and/or viral factors that enhance expression of immunodeficiency inducing FeLV variants in feline T cells and their viral responsive sequences will be identified and characterized. Experiments in progress suggest that a defect in the processing of the envelope polyprotein (gp85) may play a role in the delayed kinetics of cell killing by a FeLV variant (61B) that induces immunodeficiency in cats only after a prolonged asymtomatic period. We will pursue studies to precisely identify the viral genetic basis for the defect in processing of 61B and determine if alterations in the processing of the 61B envelope precursor are responsible for attenuation of this variant. The FeLV system offers a unique model in which to study the mechanisms of retroviral induced T cell cytopathicity and immunodeficiency disease using closely related molecularly cloned virus variants. The pathogenicity of these viruses have been characterized in their natural host, and several variants that induce feline immunodeficiency as well as FeLVs that do not induce immunodeficiency have been identified. In addition, an in vitro assay has been developed that predicts the ability of FeLV to induce immunodeficiency in cats. Understanding the mechanism of FeLV induced disease and the relationship of viral genetic variation to pathogenicity should facilitate the design of effective therapies against immunodeficiency inducing retroviruses that can ultimately be tested in this model system.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Cancer Institute (NCI)
Type
Research Project (R01)
Project #
5R01CA051080-02
Application #
3195722
Study Section
Special Emphasis Panel (ARR (V1))
Project Start
1990-03-12
Project End
1995-02-28
Budget Start
1991-03-01
Budget End
1992-02-29
Support Year
2
Fiscal Year
1991
Total Cost
Indirect Cost

  Institution

Name
University of Washington
Department
Type
Schools of Medicine
DUNS #
135646524
City
Seattle
State
WA
Country
United States
Zip Code
98195

  Publications

Mendoza, Ramon; Miller, A Dusty; Overbaugh, Julie (2013) Disruption of thiamine uptake and growth of cells by feline leukemia virus subgroup A. J Virol 87:2412-9
Cheng, Heather H; Anderson, Maria M; Overbaugh, Julie (2007) Feline leukemia virus T entry is dependent on both expression levels and specific interactions between cofactor and receptor. Virology 359:170-8
Cheng, Heather H; Anderson, Maria M; Hankenson, F Claire et al. (2006) Envelope determinants for dual-receptor specificity in feline leukemia virus subgroup A and T variants. J Virol 80:1619-28
Mendoza, Ramon; Anderson, Maria M; Overbaugh, Julie (2006) A putative thiamine transport protein is a receptor for feline leukemia virus subgroup A. J Virol 80:3378-85
Lauring, Adam S; Cheng, Heather H; Eiden, Maribeth V et al. (2002) Genetic and biochemical analyses of receptor and cofactor determinants for T-cell-tropic feline leukemia virus infection. J Virol 76:8069-78
Faix, Peggy Ho; Feldman, Steven A; Overbaugh, Julie et al. (2002) Host range and receptor binding properties of vectors bearing feline leukemia virus subgroup B envelopes can be modulated by envelope sequences outside of the receptor binding domain. J Virol 76:12369-75
Sugai, J; Eiden, M; Anderson, M M et al. (2001) Identification of envelope determinants of feline leukemia virus subgroup B that permit infection and gene transfer to cells expressing human Pit1 or Pit2. J Virol 75:6841-9
Lauring, A S; Anderson, M M; Overbaugh, J (2001) Specificity in receptor usage by T-cell-tropic feline leukemia viruses: implications for the in vivo tropism of immunodeficiency-inducing variants. J Virol 75:8888-98
Anderson, M M; Lauring, A S; Robertson, S et al. (2001) Feline Pit2 functions as a receptor for subgroup B feline leukemia viruses. J Virol 75:10563-72
Gwynn, S R; Hankenson, F C; Lauring, A S et al. (2000) Feline leukemia virus envelope sequences that affect T-cell tropism and syncytium formation are not part of known receptor-binding domains. J Virol 74:5754-61

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