Abstract

The single most important cause of corneal blindness is herpes simplex virus (HSV) type 1 with as many as 500,000 cases per year in the US. This is a result of HSV's ability to establish latent infections that can reactivate to cause recurrent herpetic kerititis. The rate of recurrence in the eye has a major impact on the degree of corneal damage and the eventual outcome for the patient. Because the number of neurons in which latency is established directly correlates with the frequency of HSV reactivation, the factors that influence the establishment of latency also dictate the outcome of ocular infections. Although a general descriptive understanding of HSV establishment of latency is well established, most of the molecular details await discovery. A central question is how expression of the lytic viral gene cascade is repressed in a very large pool of neurons at the site of latency. The latently associated transcript locus (LAT) is the only viral gene known to specifically regulate the establishment of latency without exerting any impact on viral replication. The expression of LAT prevents the death of thousands of sensory neurons, and increases the number of neurons in which latency is established by 400%. How LAT accomplishes these tasks is controversial and presently not known. Defining how LAT preserves neurons and promotes the establishment of latency will provide insights into the viral/host cell interface critical to regulating this process, and point to antiviral targets potentially useful in preventing and/or controlling viral reactivation. Preventing reactivation would reduce the spread of infection through the population and also reduce the reactivation-mediated repetitive tissue insult responsible for corneal blindness. Our long-term goal is to delineate the molecular mechanisms of HSV pathogenesis in vivo, in order that effective therapeutic strategies can be developed to treat and/or prevent infection. Our objective will be to determine the molecular mechanism(s) by which LAT prevents the death of neurons and promotes the establishment of latency. Our central hypothesis is that LAT functions as a selective """"""""Off Switch"""""""" in neurons, inhibiting lytic gene expression during the establishment, maintenance, and reactivation stages of infection. Specifically we will (1) Determine how the LAT gene prevents neuronal death and promotes the establishment of latent infections; (2) Determine the role of the LAT gene in the establishment of latency and/or reactivation from latency in the rabbit ocular model; (3) Determine the biochemical mechanisms whereby the LAT gene exerts its biologically important effects.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Eye Institute (NEI)
Type
Research Project (R01)
Project #
5R01EY013168-07
Application #
7110935
Study Section
Special Emphasis Panel (ZRG1-VISA (01))
Program Officer
Shen, Grace L
Project Start
2000-09-30
Project End
2008-04-30
Budget Start
2006-09-20
Budget End
2008-04-30
Support Year
7
Fiscal Year
2006
Total Cost
$419,323
Indirect Cost

  Institution

Name
University of Cincinnati
Department
Genetics
Type
Schools of Medicine
DUNS #
041064767
City
Cincinnati
State
OH
Country
United States
Zip Code
45221

  Publications

Thompson, Richard L; Sawtell, Nancy M (2011) The herpes simplex virus type 1 latency associated transcript locus is required for the maintenance of reactivation competent latent infections. J Neurovirol 17:552-8
Sawtell, Nancy M; Triezenberg, Steven J; Thompson, Richard L (2011) VP16 serine 375 is a critical determinant of herpes simplex virus exit from latency in vivo. J Neurovirol 17:546-51
Thompson, Richard L; Sawtell, Nancy M (2010) Therapeutic implications of new insights into the critical role of VP16 in initiating the earliest stages of HSV reactivation from latency. Future Med Chem 2:1099-105
Thompson, Richard L; Preston, Chris M; Sawtell, Nancy M (2009) De novo synthesis of VP16 coordinates the exit from HSV latency in vivo. PLoS Pathog 5:e1000352
Thompson, R L; Sawtell, N M (2006) Evidence that the herpes simplex virus type 1 ICP0 protein does not initiate reactivation from latency in vivo. J Virol 80:10919-30
Sawtell, N M; Thompson, R L; Haas, R L (2006) Herpes simplex virus DNA synthesis is not a decisive regulatory event in the initiation of lytic viral protein expression in neurons in vivo during primary infection or reactivation from latency. J Virol 80:38-50
Sawtell, N M; Thompson, R L (2004) Comparison of herpes simplex virus reactivation in ganglia in vivo and in explants demonstrates quantitative and qualitative differences. J Virol 78:7784-94
Foster, William J; Fuller, Christine E; Perry, Arie et al. (2003) Status of the NF1 tumor suppressor locus in uveal melanoma. Arch Ophthalmol 121:1311-5
Thompson, R L; Shieh, May T; Sawtell, N M (2003) Analysis of herpes simplex virus ICP0 promoter function in sensory neurons during acute infection, establishment of latency, and reactivation in vivo. J Virol 77:12319-30
Sawtell, N M (2003) Quantitative analysis of herpes simplex virus reactivation in vivo demonstrates that reactivation in the nervous system is not inhibited at early times postinoculation. J Virol 77:4127-38

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