Abstract

Synthesis of mRNA in eukaryotes, and its utilization in the cytoplasm, requires modification at the RNA's 3'end by addition of a poly(A) tail. This process also serves as a point at which the cell can regulate the type and amount of mRNA derived from a particular gene. Even though mRNA 3'end formation occurs in an unexpectedly large complex, most, if not all, of the subunits of this machinery have been identified in the yeast S. cerevisiae. However, little is known about how these 21 proteins cooperate with each other to insure processing that is accurate as well as coupled in a timely fashion to other events in mRNA synthesis and packaging. With the 3'-end processing components in hand, and activities for several of these factors newly defined, a unique opportunity now exists to rigorously address the mechanism by which this essential and universal step in gene expression occurs and is regulated. The central hypothesis of this proposal is that definable rearrangements of protein partners occur within the complex as it evaluates the authenticity of the processing site, commits to cleavage at the poly(A) site, reorganizes to position the poly(A) polymerase for tail synthesis, and releases the final RNA product. The objective is to understand how such reorganizations drive the cycle of mRNA 3'end processing. The research focuses on four events that are likely to be critical transition points in this cycle yet whose underlying mechanisms are not understood. These include the initiation of cleavage and the role of the Ssuy2 protein in this step, the transition from cleavage to poly(A) addition and its regulation by phosphorylation of the Ptai scaffold protein, the control of poly(A) polymerase activity by interactions at its amino-terminus, and the release of processing factors following tail synthesis. The studies will use yeast as the model organism because of the ease of introducing tags and mutations into the genome, the availability of numerous 3'end processing mutants, the ease of purifying processing factors for biochemical studies, and the high degree of conservation of the 3'end processing machinery across eukaryotes. Relevance: Without poly(A) tails, mRNA is targeted for degradation in the nucleus, it does not get out of the nucleus very well, and it is not translated efficiently or turned over at the appropriate rate in the cytoplasm. Maturation of mRNA 3'ends is functionally linked to other essential processes such as transcription, mRNA export, chromosome segregation, DNA repair, and tissue-specific protein expression. Mistakes in polyadenylation can impact on all of these processes. The proposed research should significantly advance our insight into the dynamics of this essential step in mRNA synthesis and identify points at which the constitutive process is likely to be regulated.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
3R01GM041752-20S1
Application #
7988814
Study Section
Molecular Genetics A Study Section (MGA)
Program Officer
Bender, Michael T
Project Start
2009-12-17
Project End
2011-05-31
Budget Start
2009-12-17
Budget End
2011-05-31
Support Year
20
Fiscal Year
2010
Total Cost
$121,435
Indirect Cost

  Institution

Name
Tufts University
Department
Biochemistry
Type
Schools of Medicine
DUNS #
039318308
City
Boston
State
MA
Country
United States
Zip Code
02111

  Publications

Graber, Joel H; Nazeer, Fathima I; Yeh, Pei-chun et al. (2013) DNA damage induces targeted, genome-wide variation of poly(A) sites in budding yeast. Genome Res 23:1690-703
Ezeokonkwo, Chukwudi; Ghazy, Mohamed A; Zhelkovsky, Alexander et al. (2012) Novel interactions at the essential N-terminus of poly(A) polymerase that could regulate poly(A) addition in Saccharomyces cerevisiae. FEBS Lett 586:1173-8
Schmid, Manfred; Poulsen, Mathias Bach; Olszewski, Pawel et al. (2012) Rrp6p controls mRNA poly(A) tail length and its decoration with poly(A) binding proteins. Mol Cell 47:267-80
Gordon, James M B; Shikov, Sergei; Kuehner, Jason N et al. (2011) Reconstitution of CF IA from overexpressed subunits reveals stoichiometry and provides insights into molecular topology. Biochemistry 50:10203-14
Kuehner, Jason N; Pearson, Erika L; Moore, Claire (2011) Unravelling the means to an end: RNA polymerase II transcription termination. Nat Rev Mol Cell Biol 12:283-94
Ezeokonkwo, Chukwudi; Zhelkovsky, Alexander; Lee, Rosanna et al. (2011) A flexible linker region in Fip1 is needed for efficient mRNA polyadenylation. RNA 17:652-64
Zhao, J; Kessler, M; Helmling, S et al. (1999) Pta1, a component of yeast CF II, is required for both cleavage and poly(A) addition of mRNA precursor. Mol Cell Biol 19:7733-40
Aranda, A; Perez-Ortin, J E; Moore, C et al. (1998) Transcription termination downstream of the Saccharomyces cerevisiae FBP1 [changed from FPB1] poly(A) site does not depend on efficient 3'end processing. RNA 4:303-18
Zhao, J; Kessler, M M; Moore, C L (1997) Cleavage factor II of Saccharomyces cerevisiae contains homologues to subunits of the mammalian Cleavage/ polyadenylation specificity factor and exhibits sequence-specific, ATP-dependent interaction with precursor RNA. J Biol Chem 272:10831-8
Kessler, M M; Henry, M F; Shen, E et al. (1997) Hrp1, a sequence-specific RNA-binding protein that shuttles between the nucleus and the cytoplasm, is required for mRNA 3'-end formation in yeast. Genes Dev 11:2545-56

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