Abstract

Human cytomegalovirus (CMV) is a major opportunistic pathogen affecting AIDS patients. This virus has been suggested to be one of several possible contributors to progression in this disease. Viral pathogenesis and determinants of replication, persistence and latency are key to reactivation and dissemination of CMV in AIDS patients but mechanisms remain poorly defined because of a lack of appropriate model systems for this species specific virus. Bone marrow derived hematopoietic cells have been thought to be an important natural reservoir of latent virus. This application will identify bone marrow cell types capable of harboring the viral genome, focussing on the granulocyte-macrophage (GM) lineage, and will investigate the extent of viral gene expression and the form that the viral genome takes in these cells. First, we will investigate the quiescent infection of the GM lineage cells in culture as a model of viral latency, studying the expression of the ie1 gene that has been detected in these cells, identifying other viral transcripts and analyzing the form of the viral genome. This information will be used to guide investigations in experimentally infected SCID-hu (bone/bone marrow) mice and naturally infected bone marrow cells from seropositive individuals. Second, we will investigate the signal(s) and mechanism(s) of viral reactivation when infected GM precursors are subjected to long-term coculture with permissive human fibroblast cells. Factors that stimulate differentiation and growth of GM precursors will be evaluated as a means to increase efficiency of reactivation. Parameters for reactivation that efficiently reactivate virus in the cultured GM cell model and in SCID-hu mice will be applied to peripheral blood or bone marrow cells of naturally infected individuals. The long term aim is to establish in biological assay for a process that has never yielded to experimental manipulation; virus has only been shown to reactivate when an individual is severely immunosuppressed, or when latently infected blood or tissues are transfused or transplanted into another human being. Third, we will investigate the viral genetic basis for latency (establishment and reactivation) using the GM cell culture and SCID-hu mouse models. Individual regulatory genes (ie1, ie2) and newly identified latent infection associated genes will be deleted from the viral genome and the resultant mutant viruses will be evaluated for their biological phenotype in establishment of latency and ability to reactivate. Taken together, the proposed research will define the biological spectrum of infection in bone marrow and will establish the contribution of viral functions that control latency and reactivation. This information will provide information on viral latency that should directly impact on the approaches to control reactivation following immunosuppression and transplantation.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Allergy and Infectious Diseases (NIAID)
Type
Research Project (R01)
Project #
5R01AI033852-05
Application #
2672200
Study Section
AIDS and Related Research Study Section 3 (ARRC)
Project Start
1994-08-01
Project End
1999-06-30
Budget Start
1998-05-01
Budget End
1999-06-30
Support Year
5
Fiscal Year
1998
Total Cost
Indirect Cost

  Institution

Name
Stanford University
Department
Microbiology/Immun/Virology
Type
Schools of Medicine
DUNS #
800771545
City
Stanford
State
CA
Country
United States
Zip Code
94305

  Publications

Vana, Marcy L; Formankova, Danuse; Cha, Steven et al. (2008) Comparison of polymerase chain reaction of polymorphonuclear leukocytes and plasma identifies patients who control cytomegalovirus infection after hematopoietic cell transplantation. Clin Infect Dis 47:535-9
Noda, Satoshi; Aguirre, Shirley A; Bitmansour, Andrew et al. (2006) Cytomegalovirus MCK-2 controls mobilization and recruitment of myeloid progenitor cells to facilitate dissemination. Blood 107:30-8
Slobedman, Barry; Stern, J Lewis; Cunningham, Anthony L et al. (2004) Impact of human cytomegalovirus latent infection on myeloid progenitor cell gene expression. J Virol 78:4054-62
Abate, Davide A; Watanabe, Shinya; Mocarski, Edward S (2004) Major human cytomegalovirus structural protein pp65 (ppUL83) prevents interferon response factor 3 activation in the interferon response. J Virol 78:10995-1006
Hertel, Laura; Mocarski, Edward S (2004) Global analysis of host cell gene expression late during cytomegalovirus infection reveals extensive dysregulation of cell cycle gene expression and induction of Pseudomitosis independent of US28 function. J Virol 78:11988-2011
Hertel, Laura; Lacaille, Vashti G; Strobl, Herbert et al. (2003) Susceptibility of immature and mature Langerhans cell-type dendritic cells to infection and immunomodulation by human cytomegalovirus. J Virol 77:7563-74
Slobedman, Barry; Mocarski, Edward S; Arvin, Ann M et al. (2002) Latent cytomegalovirus down-regulates major histocompatibility complex class II expression on myeloid progenitors. Blood 100:2867-73
Saederup, N; Aguirre, S A; Sparer, T E et al. (2001) Murine cytomegalovirus CC chemokine homolog MCK-2 (m131-129) is a determinant of dissemination that increases inflammation at initial sites of infection. J Virol 75:9966-76
White, K L; Slobedman, B; Mocarski, E S (2000) Human cytomegalovirus latency-associated protein pORF94 is dispensable for productive and latent infection. J Virol 74:9333-7
Slobedman, B; Mocarski, E S (1999) Quantitative analysis of latent human cytomegalovirus. J Virol 73:4806-12

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