Abstract

Kaposi's sarcoma-associated herpesvirus (KSHV) is the etiologic agent of the majority of AIDS- associated cancers. It is endemic in many areas of Africa and, due to the extraordinarily high HIV burden there, Kaposi's sarcoma is emerging as one of the most common cancers on that continent. During AIDS-induced immunosuppression, KSHV replication is no longer effectively controlled, and, together with a large latently infected population of cells, contributes to disease progression. Amplification of KSHV is dependent on its ability to exert strong control over the gene expression environment of the infected cell. A primary mechanism the virus uses to regulate gene expression is to induce widespread degradation of messenger RNA (mRNA) in the cytoplasm. This phenotype plays numerous roles in the viral lifecycle and immune evasion, and is driven by a virally encoded nuclease termed SOX. Although SOX cleaves an extremely large number of transcripts, it exhibits clear specificity for RNA Polymerase II (Pol II) transcribed RNAs and does not have significant RNA binding activity. How it recognizes and is brought to its targets remains a central unanswered question in the field and is the focus of the first Aim of this proposal. We will apply bimolecular complementation-based protein interaction screening, unbiased ribonucleoprotein complex purification, and directed functional studies to pinpoint how SOX is directed to its target mRNAs. Identification and characterization of factors that mediate SOX targeting is central to understanding how KSHV maintains control of gene expression, and may similarly provide new insight into cellular strategies to govern RNA fate. The depletion of cytosolic mRNA by SOX is presumably sensed by the cell, and thus offers a unique opportunity to reveal cellular responses to broad changes in the gene expression landscape, such as those induced by pathogens. In this regard, recent results in yeast indicate the existence of feedback mechanisms to detect and respond to altered activity of different stages of gene expression. Using gamma-herpesviruses as tools, we have now discovered an analogous pathway in mammalian cells that links mRNA degradation with transcription. Activation of this pathway, which we term `transcriptional priming', impacts the rate of nascent mRNA synthesis. Though it is likely that the normal role of this host pathway is to regulate cellular gene expression in response to stress, we hypothesize that during KSHV infection its activation by SOX instead serves to enhance Pol II transcription of viral genes. Defining how this pathway is controlled and how it impacts the viral life cycle are the goals of Aim 2. Results from these studies should provide new insight into how seemingly distant stages of gene expression are integrated, and how viral pathogens like KSHV take advantage of these cellular controls to enhance their replicative success.

Public Health Relevance

Kaposi's sarcoma-associated herpesvirus (KSHV) is an emerging Group 1 pathogen and the major cause of cancers in untreated AIDS patients. The success of KSHV replication hinges on its ability to control gene expression in the infected cell, which is most broadly achieved via widespread destruction of protein coding RNAs. This grant is focused on revealing how the viral protein responsible for this process recognizes its RNA targets, and how the cell responds to message depletion.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Cancer Institute (NCI)
Type
Research Project (R01)
Project #
5R01CA136367-09
Application #
9513444
Study Section
AIDS-associated Opportunistic Infections and Cancer Study Section (AOIC)
Program Officer
Read-Connole, Elizabeth Lee
Project Start
2015-09-25
Project End
2020-08-31
Budget Start
2018-09-01
Budget End
2019-08-31
Support Year
9
Fiscal Year
2018
Total Cost
Indirect Cost

  Institution

Name
University of California Berkeley
Department
Other Basic Sciences
Type
Earth Sciences/Resources
DUNS #
124726725
City
Berkeley
State
CA
Country
United States
Zip Code
94704

  Publications

Gilbertson, Sarah; Federspiel, Joel D; Hartenian, Ella et al. (2018) Changes in mRNA abundance drive shuttling of RNA binding proteins, linking cytoplasmic RNA degradation to transcription. Elife 7:
Karijolich, John; Zhao, Yang; Alla, Ravi et al. (2017) Genome-wide mapping of infection-induced SINE RNAs reveals a role in selective mRNA export. Nucleic Acids Res 45:6194-6208
Tucker, Jessica M; Glaunsinger, Britt A (2017) Host Noncoding Retrotransposons Induced by DNA Viruses: a SINE of Infection? J Virol 91:
Muller, Mandy; Glaunsinger, Britt A (2017) Nuclease escape elements protect messenger RNA against cleavage by multiple viral endonucleases. PLoS Pathog 13:e1006593
Glaunsinger, Britt A (2015) Modulation of the Translational Landscape During Herpesvirus Infection. Annu Rev Virol 2:311-33
Abernathy, Emma; Gilbertson, Sarah; Alla, Ravi et al. (2015) Viral Nucleases Induce an mRNA Degradation-Transcription Feedback Loop in Mammalian Cells. Cell Host Microbe 18:243-53
Abernathy, Emma; Glaunsinger, Britt (2015) Emerging roles for RNA degradation in viral replication and antiviral defense. Virology 479-480:600-8
Davis, Zoe H; Verschueren, Erik; Jang, Gwendolyn M et al. (2015) Global mapping of herpesvirus-host protein complexes reveals a transcription strategy for late genes. Mol Cell 57:349-60
Gaglia, Marta Maria; Rycroft, Chris H; Glaunsinger, Britt A (2015) Transcriptome-Wide Cleavage Site Mapping on Cellular mRNAs Reveals Features Underlying Sequence-Specific Cleavage by the Viral Ribonuclease SOX. PLoS Pathog 11:e1005305
Muller, Mandy; Hutin, Stephanie; Marigold, Oliver et al. (2015) A ribonucleoprotein complex protects the interleukin-6 mRNA from degradation by distinct herpesviral endonucleases. PLoS Pathog 11:e1004899

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