Abstract

The long-term objectives of this research program remain directed at defining the mechanisms by which mRNA molecules are exported from the nucleus and determining under what circumstances and by what mechanisms nucleocytoplasmic transport is regulated. Our understanding of nucleocytoplasmic transport of proteins and small RNAs (e.g. tRNAs) has grown substantially through the identification of transport signals and karyopherin receptors that recognize them. We know much less about mRNA export, which is considerably more complex, in part because it is tightly coupled to mRNA biogenesis and checkpoints exist that permit only completely- and accurately-processed mRNAs to be exported. mRNAs are exported as RNA/protein complexes (mRNPs). Many factors required uniquely for mRNA export have been identified but how they work together is not known. A major focus is to understand the role in mRNA export of the DEADbox protein (DBP) Dbp5/Rat8. DBFs play essential roles in virtually all aspects of RNA metabolism. Dbp5 shuttles and interacts directly with components of the nuclear pore complex (NPC). To address two centrals questions about RNA export, the following specific aims are proposed:
Aim 1) To test the hypothesis that Dbp5 acts when bound to the cvtoplasmic filaments of NPCs to couple ATP hydrolysis with mRNP translocation through the pore and removal of mRNP proteins. The interactions between Dbp5, proteins of the cytoplasmic filaments of the NPC, and accessory proteins will be mapped. Genetic and physical approaches will be used to determine whether Dbp5 must bind to NPC filaments to mediate mRNA export. The dynamics of interaction between Dbp5 and NPCs will be analyzed using fluorescence recovery after photobleaching (FRAP) and with mating assays. Whether Dbp5 can disassemble model RNA/protein complexes in vitro will be determined.
Aim 2) To test the hypothesis that they key to export lies in the composition and organization of mRNP complexes. The studies will compare export-competent mRNPs from wild-type cells and mRNPs that accumulate in export mutant strains. Other studies will determine how exported heat shock mRNPs differ from mRNPs that accumulate in nuclei following heat shock.
Aim 3) To determine whether Dbp5 functions not only at NPCs but also in the nucleus and what it does in the nucleus.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
5R01GM033998-22
Application #
7097925
Study Section
Molecular Genetics B Study Section (MGB)
Program Officer
Shapiro, Bert I
Project Start
1984-08-01
Project End
2009-07-31
Budget Start
2006-08-01
Budget End
2007-07-31
Support Year
22
Fiscal Year
2006
Total Cost
$463,743
Indirect Cost

  Institution

Name
Dartmouth College
Department
Biochemistry
Type
Schools of Medicine
DUNS #
041027822
City
Hanover
State
NH
Country
United States
Zip Code
03755

  Publications

Estruch, Francisco; Hodge, Christine; Gomez-Navarro, Natalia et al. (2012) Insights into mRNP biogenesis provided by new genetic interactions among export and transcription factors. BMC Genet 13:80
Hodge, Christine A; Tran, Elizabeth J; Noble, Kristen N et al. (2011) The Dbp5 cycle at the nuclear pore complex during mRNA export I: dbp5 mutants with defects in RNA binding and ATP hydrolysis define key steps for Nup159 and Gle1. Genes Dev 25:1052-64
Noble, Kristen N; Tran, Elizabeth J; Alcázar-Román, Abel R et al. (2011) The Dbp5 cycle at the nuclear pore complex during mRNA export II: nucleotide cycling and mRNP remodeling by Dbp5 are controlled by Nup159 and Gle1. Genes Dev 25:1065-77
Folkmann, Andrew W; Noble, Kristen N; Cole, Charles N et al. (2011) Dbp5, Gle1-IP6 and Nup159: a working model for mRNP export. Nucleus 2:540-8
Hodge, Christine A; Choudhary, Vineet; Wolyniak, Michael J et al. (2010) Integral membrane proteins Brr6 and Apq12 link assembly of the nuclear pore complex to lipid homeostasis in the endoplasmic reticulum. J Cell Sci 123:141-51
Schneiter, Roger; Cole, Charles N (2010) Integrating complex functions: coordination of nuclear pore complex assembly and membrane expansion of the nuclear envelope requires a family of integral membrane proteins. Nucleus 1:387-92
Estruch, Francisco; Peiró-Chova, Lorena; Gómez-Navarro, Natalia et al. (2009) A genetic screen in Saccharomyces cerevisiae identifies new genes that interact with mex67-5, a temperature-sensitive allele of the gene encoding the mRNA export receptor. Mol Genet Genomics 281:125-34
Scarcelli, John J; Viggiano, Susan; Hodge, Christine A et al. (2008) Synthetic genetic array analysis in Saccharomyces cerevisiae provides evidence for an interaction between RAT8/DBP5 and genes encoding P-body components. Genetics 179:1945-55
Scarcelli, John J; Hodge, Christine A; Cole, Charles N (2007) The yeast integral membrane protein Apq12 potentially links membrane dynamics to assembly of nuclear pore complexes. J Cell Biol 178:799-812
Rollenhagen, Christiane; Hodge, Christine A; Cole, Charles N (2007) Following temperature stress, export of heat shock mRNA occurs efficiently in cells with mutations in genes normally important for mRNA export. Eukaryot Cell 6:505-13

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