The human polyomavirus JC virus (JCV) causes the fatal demyelinating disease progressive multifocal leukoencephalopathy (PML) in immunocompromised individuals, especially patients with Acquired Immunodeficiency Syndrome (AIDS). JCV infects tissues of the kidney, and is persistently shed during the lifetime of the individual. Up to 39% of the population is seroreactive to JCV, and viral DNA can be detected in up to 50% of normal kidney tissue. While infection in immunocompetent individuals is generally thought to be asymptomatic, reactivation of JCV in immunocompromised individuals results in dissemination of JCV to the brain and lytic infection of oligodendrocytes, resulting in PML. PML is present in about 5% of AIDS patients and before the introduction of anti-retroviral therapy, the prognosis was usually fatal within 6 months. With the advent of effective antiretroviral therapy, mortality rates have fallen, but PML is still fatal in about 50% of patients. More recently, immunomodulatory treatments that manage multiple sclerosis have unexpectedly resulted in PML. Currently, few options exist for the treatment of PML as a result of a poor understanding of viral pathogenicity of JCV. This project proposes to increase our understanding of JCV pathogenesis, by studying exposure and delivery of the viral genome to the host cell nucleus. Since JCV must balance between protecting its viral genome and allowing the host replication machinery to access its encapsidated genome for viral replication, the factors that regulate viral genome release are critical for successful infection.
The first aim of this proposal will examine the cellular location of JCV uncoating by generating JCV virions whose capsid and genome are labeled with spectrally distinct fluorophores. Trafficking of these particles during infection will be performed in relation to fluorescently labeled cell markers by live cell confocal fluorescence microscopy.
The second aim will investigate the nuclear import of JCV through the nuclear pore complex (NPC), specifically characterizing how these particles, whose diameter is greater than the upper limit of the NPC, are able enter the nucleus.
The third aim proposes to reduce the diameter of a viral pore in the capsid and determine the effects on viral infectivity.
This aim may provide a mechanistic understanding of release of minor capsid proteins and genome are from JCV and may lead to the development of antiviral compound that prevent the egress of the minor capsid proteins or genome through this pore. Taken together, these aims will provide critical information on viral pathogenesis of JCV and will identify new targets for the development of novel anti- viral therapies.

Public Health Relevance

This proposed study will significantly increase our understanding of viral pathogenesis of the human polyomavirus JC virus. JC virus is the causative agent of the fatal disease progressive multifocal leukoencephalopathy, and is most commonly seen in patients with acquired immunodeficiency syndrome. Since there are limited treatment options for this disease, this research will provide critical information into the basic biology of these viruses, allowing for the identification of new targets for anti-viral therapy.

Agency
National Institute of Health (NIH)
Institute
National Institute of Neurological Disorders and Stroke (NINDS)
Type
Postdoctoral Individual National Research Service Award (F32)
Project #
1F32NS070687-01
Application #
7928519
Study Section
Special Emphasis Panel (ZRG1-AARR-H (22))
Program Officer
Wong, May
Project Start
2010-03-01
Project End
2013-02-28
Budget Start
2010-03-01
Budget End
2011-02-28
Support Year
1
Fiscal Year
2010
Total Cost
$47,606
Indirect Cost
Name
Brown University
Department
Biochemistry
Type
Schools of Medicine
DUNS #
001785542
City
Providence
State
RI
Country
United States
Zip Code
02912
Ströh, Luisa J; Maginnis, Melissa S; Blaum, Bärbel S et al. (2015) The Greater Affinity of JC Polyomavirus Capsid for ?2,6-Linked Lactoseries Tetrasaccharide c than for Other Sialylated Glycans Is a Major Determinant of Infectivity. J Virol 89:6364-75
Nelson, Christian D S; Ströh, Luisa J; Gee, Gretchen V et al. (2015) Modulation of a pore in the capsid of JC polyomavirus reduces infectivity and prevents exposure of the minor capsid proteins. J Virol 89:3910-21
Maginnis, Melissa S; Nelson, Christian D S; Atwood, Walter J (2015) JC polyomavirus attachment, entry, and trafficking: unlocking the keys to a fatal infection. J Neurovirol 21:601-13
Carney, Daniel W; Nelson, Christian D S; Ferris, Bennett D et al. (2014) Structural optimization of a retrograde trafficking inhibitor that protects cells from infections by human polyoma- and papillomaviruses. Bioorg Med Chem 22:4836-47
Zins, Stephen R; Nelson, Christian D S; Maginnis, Melissa S et al. (2014) The human alpha defensin HD5 neutralizes JC polyomavirus infection by reducing endoplasmic reticulum traffic and stabilizing the viral capsid. J Virol 88:948-60
Assetta, Benedetta; Maginnis, Melissa S; Gracia Ahufinger, Irene et al. (2013) 5-HT2 receptors facilitate JC polyomavirus entry. J Virol 87:13490-8
Lipovsky, Alex; Popa, Andreea; Pimienta, Genaro et al. (2013) Genome-wide siRNA screen identifies the retromer as a cellular entry factor for human papillomavirus. Proc Natl Acad Sci U S A 110:7452-7
Nelson, Christian D S; Carney, Dan W; Derdowski, Aaron et al. (2013) A retrograde trafficking inhibitor of ricin and Shiga-like toxins inhibits infection of cells by human and monkey polyomaviruses. MBio 4:e00729-13
Ferenczy, Michael W; Marshall, Leslie J; Nelson, Christian D S et al. (2012) Molecular biology, epidemiology, and pathogenesis of progressive multifocal leukoencephalopathy, the JC virus-induced demyelinating disease of the human brain. Clin Microbiol Rev 25:471-506
Nelson, Christian D S; Derdowski, Aaron; Maginnis, Melissa S et al. (2012) The VP1 subunit of JC polyomavirus recapitulates early events in viral trafficking and is a novel tool to study polyomavirus entry. Virology 428:30-40

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