Abstract

In mammalian cells, transcription of mRNA is catalyzed by RNA polymerase II (PolII), a DNA- dependent RNA polymerase. PolII also has RNA-dependent RNA polymerase (RdRP) activity; it can use RNA as a template to synthesize new RNA of de?ned sequence. The breadth of functions for the Pol II RdRP activity in mammalian cells is unknown, yet could have broad biological signi?cance. Pol II RdRP activity is medically relevant; it is required for replication of hepatitis delta virus, which causes liver disease. Seminal experiments are proposed to characterize the RdRP activity of Pol II in human and mouse cells and to determine its role in controlling RNA metabolism and retrotransposition. In addition, the RdRPome ? the RNAs made by RdRP activity ? will be identi?ed in human and mouse cells. This will be the ?rst concerted effort to determine the extent to which RdRP activity affects the RNA population in mammalian cells, paving the way for future studies of the biological impacts and functions of RdRP-generated or modi?ed RNAs.
Aim 1. Understand how the Pol II RdRP activity couples with Drosha and Dicer to control SINE RNA metabolism and SINE retrotransposition. Pol II RdRP activity can extend the 3' ends of B2 and Alu RNAs, which are transcribed from short interspersed elements (SINEs). Preliminary data suggest that this extension allows the RNAs to be cleaved by Drosha and perhaps Dicer. The roles of the Pol II RdRP, Drosha and Dicer in regulating the degradation of SINE RNAs will be determined using biochemical and cell-based experiments. In addition, studies will be performed to understand the roles of these three activities in controlling SINE retrotransposition, which requires an RNA intermediate and can cause disease.
Aim 2. Identify the human and mouse RdRPomes and determine the effect of the Pol II RdRP on the metabolism of select RNAs. The extent to which Pol II or other cellular polymerases function as RdRPs remains an open question, and no systematic method to identify mammalian RdRP-derived sequences has been devised. A technique will be developed that selectively labels RNA sequences made by RdRP activity in cells, puri?es these RNAs, and identi?es them via deep sequencing. The RdRP-generated RNAs made by Pol II will be de?ned, and functional studies will probe whether the Pol II RdRP activity regulates the stability of select RNAs in cells. The studies will test roles for Pol II that go beyond its function in the traditional central dogma. RdRPs have been shown to play important roles in non-mammalian systems; the proposed studies could reveal critical yet uncharacterized mechanisms of cellular regulation involving mammalian RdRP activity. The relative absence of studies aimed at understanding the prevalence and importance of RdRP activities in mammalian cells ampli?es the timeliness and signi?cance of the proposed research.

Public Health Relevance

Little is understood about the biological and medically relevant functions of the RNA-dependent RNA polymerase (RdRP) activity of mammalian RNA polymerase II, which we have found can modify the 3' end of a RNA to decrease its stability in cells. The proposed studies are aimed at de?ning the breadth of Pol II RdRP activity in human and mouse cells. In addition, we will learn how Pol II RdRP activity controls the metabolism of RNAs encoded from short interspersed elements (SINEs) that litter mammalian genomes, and how it limits SINE retrotransposition, which can be deleterious to somatic cells.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
2R01GM068414-13
Application #
9026086
Study Section
Molecular Genetics B Study Section (MGB)
Program Officer
Bender, Michael T
Project Start
2003-09-19
Project End
2019-08-31
Budget Start
2015-09-18
Budget End
2016-08-31
Support Year
13
Fiscal Year
2015
Total Cost
$332,822
Indirect Cost
$112,822

  Institution

Name
University of Colorado at Boulder
Department
Chemistry
Type
Schools of Arts and Sciences
DUNS #
007431505
City
Boulder
State
CO
Country
United States
Zip Code
80303

  Publications

Cardiello, Joseph F; Goodrich, James A; Kugel, Jennifer F (2018) Heat Shock Causes a Reversible Increase in RNA Polymerase II Occupancy Downstream of mRNA Genes, Consistent with a Global Loss in Transcriptional Termination. Mol Cell Biol 38:
Goodrich, James; Taatjes, Dylan (2018) Transcription regulation enters a new phase. Nature 558:197-198
Kugel, Jennifer F; Goodrich, James A (2017) Finding the start site: redefining the human initiator element. Genes Dev 31:1-2
Eidem, Tess M; Kugel, Jennifer F; Goodrich, James A (2016) Noncoding RNAs: Regulators of the Mammalian Transcription Machinery. J Mol Biol 428:2652-2659
Goodrich, James A; Kugel, Jennifer F (2015) Studying the affinity, kinetic stability, and specificity of RNA/protein interactions: SINE ncRNA/Pol II complexes as a model system. Methods Mol Biol 1206:165-78
Abrisch, Robert G; Eidem, Tess M; Yakovchuk, Petro et al. (2015) Infection by Herpes Simplex Virus 1 Causes Near-Complete Loss of RNA Polymerase II Occupancy on the Host Cell Genome. J Virol 90:2503-13
Ponicsan, Steven L; Kugel, Jennifer F; Goodrich, James A (2015) Repression of RNA Polymerase II Transcription by B2 RNA Depends on a Specific Pattern of Structural Regions in the RNA. Noncoding RNA 1:4-16
Kugel, Jennifer F; Goodrich, James A (2013) The regulation of mammalian mRNA transcription by lncRNAs: recent discoveries and current concepts. Epigenomics 5:95-102
Ponicsan, Steven L; Houel, Stephane; Old, William M et al. (2013) The non-coding B2 RNA binds to the DNA cleft and active-site region of RNA polymerase II. J Mol Biol 425:3625-38
Wagner, Stacey D; Yakovchuk, Petro; Gilman, Benjamin et al. (2013) RNA polymerase II acts as an RNA-dependent RNA polymerase to extend and destabilize a non-coding RNA. EMBO J 32:781-90

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