Abstract

RNA splicing, the biochemical process leading to the removal of introns from precursor RNA, is an essential step in the expression of genetic information. Unlike auto-catalyzed self-splicing reactions, splicing of nuclear pre-mRNA requires ATP and occurs in a complex, dynamic structure called the spliceosome composed of small nuclear ribonucleoproteins. A spliceosome containing unspliced pre-mRNA has been isolated from the yeast prp2 mutant. This functional spliceosome can be isolated and activated to splice upon the addition of ATP and extrinsic splicing factors (ESFs). One of the ESFs is an RNA-dependent ATPase encoded by the yeast PRP2 gene, which binds to the spliceosome and triggers splicing in the presence of ATP. Therefore, PRP2 may either be a key component of the catalytic center or function in a proofreading step. The long-term objectives of this research project are to understand the mechanism of nuclear pre-mRNA splicing through biochemical and genetic analysis of the spliceosomal components and the ESFs. Specifically, the components which constitute the catalytic center in the spliceosome will be investigated. Current studies focus on the identification of the spliceosomal components bound by PRP2 and the RNA activating the ATPase activity of PRP2. Radioactive PRP2 protein will be synthesized in vitro or isolated from yeast cells; splicing extracts will be prepared from prp2 mutants with or without radioactive labeling. The interacting proteins or RNAs can be identified by using UV cross-linking, immunological, and gel electrophoresis techniques. A genetic approach has also been taken to isolate an extragenic suppressor, SRP2; it suppresses the temperature-sensitive phenotype of prp2 and has a cold- sensitive phenotype by itself. The SRP2 gene will be isolated; its role in splicing and its relation with PRP2 will be investigated by molecular genetic techniques. The involvement of specific, important sequences of snRNAs in the catalytic steps of splicing will be analyzed by cleaving these sequences prior to the isolation of the functional spliceosome. The characterization of the heat stable ESF-bn and the search for prp2 proofreading mutants will be given a lower priority. Studies of the important constituents of the spliceosome and the ESFs in yeast may reveal the catalytic center of pre-mRNA splicing and lead to a better understanding of alternative and regulated splicing in higher organisms.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
3R01GM040639-07S1
Application #
2466470
Study Section
Molecular Biology Study Section (MBY)
Project Start
1988-08-01
Project End
1998-06-30
Budget Start
1995-12-01
Budget End
1998-06-30
Support Year
7
Fiscal Year
1997
Total Cost
Indirect Cost

  Institution

Name
City of Hope/Beckman Research Institute
Department
Type
DUNS #
City
Duarte
State
CA
Country
United States
Zip Code
91010

  Publications

Chandra, Manasa; Zang, Shengbing; Li, Haiqing et al. (2012) Nuclear translocation of type I transforming growth factor ýý receptor confers a novel function in RNA processing. Mol Cell Biol 32:2183-95
Gencheva, Marieta; Lin, Ting-Yu; Wu, Xiwei et al. (2010) Nuclear retention of unspliced pre-mRNAs by mutant DHX16/hPRP2, a spliceosomal DEAH-box protein. J Biol Chem 285:35624-32
Gencheva, Marieta; Kato, Mitsuo; Newo, Alain N S et al. (2010) Contribution of DEAH-box protein DHX16 in human pre-mRNA splicing. Biochem J 429:25-32
Dery, Kenneth J; Yean, Shyue-Lee; Lin, Ren-Jang (2008) Assembly and glycerol gradient isolation of yeast spliceosomes containing transcribed or synthetic U6 snRNA. Methods Mol Biol 488:41-63
Huang, Ching-Jung; Tang, Zhaohua; Lin, Ren-Jang et al. (2007) Phosphorylation by SR kinases regulates the binding of PTB-associated splicing factor (PSF) to the pre-mRNA polypyrimidine tract. FEBS Lett 581:223-32
Li, Chunxia; Kato, Mitsuo; Shiue, Lily et al. (2006) Cell type and culture condition-dependent alternative splicing in human breast cancer cells revealed by splicing-sensitive microarrays. Cancer Res 66:1990-9
Silverman, Edward J; Maeda, Ayaka; Wei, Janet et al. (2004) Interaction between a G-patch protein and a spliceosomal DEXD/H-box ATPase that is critical for splicing. Mol Cell Biol 24:10101-10
Edwalds-Gilbert, Gretchen; Kim, Dong-Ho; Silverman, Edward et al. (2004) Definition of a spliceosome interaction domain in yeast Prp2 ATPase. RNA 10:210-20
Silverman, Edward; Edwalds-Gilbert, Gretchen; Lin, Ren-Jang (2003) DExD/H-box proteins and their partners: helping RNA helicases unwind. Gene 312:1-16
Edwalds-Gilbert, G; Kim, D H; Kim, S H et al. (2000) Dominant negative mutants of the yeast splicing factor Prp2 map to a putative cleft region in the helicase domain of DExD/H-box proteins. RNA 6:1106-19

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