Human T-cell leukemia virus type 1 (HTLV-1) is the causative agent of adult T-cell leukemia and an inflammatory neurological disease referred to as tropical spastic paraparesis or HTLV-1-associated myelopathy. Infectious transmission of retroviruses like HTLV-1 can be divided into two phases: 1) the assembly and release of virions from the infected cell and 2) virion entry and replication in the target cell. For HTLV-1, the molecular mechanisms underlying the individual steps in these processes are not well defined. Our current studies focus on these two interrelated project areas with the goal of better understanding HTLV-1 pathogenesis. Recent experimental evidence supports a model in which HTLV-1 is transmitted directly between T lymphocytes and where virus assembly, release, transmission, and replication would be coordinately regulated with formation of a cell-cell synapse. We are examining the components and pathways that control HTLV-1 virion morphogenesis, transmission, and replication in the conceptual framework of this model. We are using biochemical, functional, and electron microscopic methods to study HTLV-1 virion assembly and release. We recently showed that interaction between a peptide motif in the viral matrix protein and a cellular NEDD4-family ubiquitin ligase (WWP1) is required for virion morphogenesis. We are currently determining what other cellular proteins are recruited to the nascent virion. We have also observed that intracellular HTLV-1 particles colocalized with the cellular transmembrane 4 protein CD82 at the plasma membrane. This finding is important, because CD82 is known to organize cell surface adhesion proteins and segregates to the immunological synapse. The association of HTLV-1 with CD82 and other cell surface and cytoskeletal proteins may be necessary to coordinate virion transmission with formation of intercellular synapses. After entry into the target cell, the viral enzymes and structural proteins form a replication complex that converts the single-stranded viral genomic RNA into a double-stranded DNA, which is integrated into the host cell chromosome. We have developed the cell culture systems, infectious molecular clones, and viral vectors that make it possible to examine HTLV-1 replication and to study anti-HTLV-1 therapeutic agents. We showed that infection with HTLV-1 virions is orders of magnitude less efficient compared with other retroviruses and that his inefficiency is the result of a post-entry block in the replication process. We are determining whether this block is conferred by the properties of viral replication enzymes, results from the actions of cellular restriction factors, reflects the need for cell-cell contact, or is caused by a combination of these factors. We have begun to characterize HTLV-1 replication enzymes and analyze reverse transcription in infected cells. We are also studying the mechanisms that HTLV-1 has evolved to evade cellular defense mechanisms that restrict the replication of other retroviruses. We also examined the expression of HTLV-1 accessory proteins, Tax and p30, and studied their roles in regulating both viral and cellular gene expression. We are determining whether these viral accessory proteins participate in coordinating and modulating the infection process. Although the basic mechanisms for transmission and replication are conserved among retroviruses, variations on common themes are likely to reveal important insights into the strategies that different viruses use for propagation and persistence in vivo. In this respect, it is useful to compare HTLV-1 and HIV-1, because both are T-cell-tropic retroviruses whose very different biological properties may be traced back to divergent strategies for escaping host-mediated immune and cellular defense mechanisms.

Agency
National Institute of Health (NIH)
Institute
Division of Basic Sciences - NCI (NCI)
Type
Intramural Research (Z01)
Project #
1Z01BC010003-09
Application #
7048984
Study Section
(RRL)
Project Start
Project End
Budget Start
Budget End
Support Year
9
Fiscal Year
2004
Total Cost
Indirect Cost
Name
Basic Sciences
Department
Type
DUNS #
City
State
Country
United States
Zip Code
LaRue, Rebecca S; Andresdottir, Valgerdur; Blanchard, Yannick et al. (2009) Guidelines for naming nonprimate APOBEC3 genes and proteins. J Virol 83:494-7
Mazurov, Dmitriy; Heidecker, Gisela; Derse, David (2007) The inner loop of tetraspanins CD82 and CD81 mediates interactions with human T cell lymphotrophic virus type 1 Gag protein. J Biol Chem 282:3896-903
Mitchell, Michael S; Bodine, Ellen T; Hill, Shawn et al. (2007) Phenotypic and genotypic comparisons of human T-cell leukemia virus type 1 reverse transcriptases from infected T-cell lines and patient samples. J Virol 81:4422-8
Derse, David; Hill, Shawn A; Princler, Gerald et al. (2007) Resistance of human T cell leukemia virus type 1 to APOBEC3G restriction is mediated by elements in nucleocapsid. Proc Natl Acad Sci U S A 104:2915-20
Wencker, Melanie; Sausse, Celine; Derse, David et al. (2007) Human T-cell leukemia virus type 1 Tax protein down-regulates pre-T-cell receptor alpha gene transcription in human immature thymocytes. J Virol 81:301-8
Heidecker, Gisela; Lloyd, Patricia A; Soheilian, Ferri et al. (2007) The role of WWP1-Gag interaction and Gag ubiquitination in assembly and release of human T-cell leukemia virus type 1. J Virol 81:9769-77
Mitchell, Michael S; Tozser, Jozsef; Princler, Gerald et al. (2006) Synthesis, processing, and composition of the virion-associated HTLV-1 reverse transcriptase. J Biol Chem 281:3964-71
Liao, Huey-Jane; Baker, Carl C; Princler, Gerald L et al. (2004) cis-Acting and trans-acting modulation of equine infectious anemia virus alternative RNA splicing. Virology 323:131-40
Nicot, Christophe; Dundr, Miroslav; Johnson, Julie M et al. (2004) HTLV-1-encoded p30II is a post-transcriptional negative regulator of viral replication. Nat Med 10:197-201
Heidecker, Gisela; Lloyd, Patricia A; Fox, Kristi et al. (2004) Late assembly motifs of human T-cell leukemia virus type 1 and their relative roles in particle release. J Virol 78:6636-48

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