Abstract

The long-term objective of the proposed work is to achieve a detailed understanding of the mechanisms of pre-mRNA splicing. Splicing plays a essential role in the maturation of most pre-mRNAs in higher eukaryotes, and alternative splicing is involved in regulating the expression of a number of genes. Most pre-mRNAs are highly complex, containing multiple introns that range in size from 65 to 100,000 nucleotides. Thus, elucidating the mechanisms by which each intron is accurately excised, without deleting essential protein coding information is of fundamental biological importance. The main focus of the proposed research is the assembly, structure and function of the spliceosome. Although a great deal of prior work has focused on the identification of the snRNAs involved in splicing, relatively little is known about the protein components of he spliceosome. In the proposed studies, intermediate splicing complexes assembled during the in vitro splicing reaction will be purified and characterized. A two-step method recently established for the large-scale purification of the spliceosome will be employed to isolate each splicing complex, and the RNA and protein components of the complexes will be identified. Complexes assembled on pre-mRNAs containing mutations that block splicing at a specific step of the reaction, as well as intermediate splicing complexes generated during the course of the in vitro splicing reaction ,will be examined. These studies should lead to the identification of splicing factors that interact stably with the pre-mRNA and are involved in different steps of he splicing reaction. In addition ,analysis of intermediate complexes generated very early in the splicing reaction should lead to the identification of factors that play an important role in establishing the pattern of splice-site selection. In subsequent studies, antibodies will be raised against specific proteins that appear to play a central role in splicing. The antibodies will then be used to clone the genes encoding these factors and further defined their function in the splicing reaction. Finally, structural analysis of the spliceosome will be carried out using electron microscopy. These studies analysis of the spliceosome will be carried out using electron microscopy. These studies should provide unique information on the spatial arrangement of pre-mRNA and splicing components within the spliceosome.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
5R01GM043375-03
Application #
3302455
Study Section
Molecular Biology Study Section (MBY)
Project Start
1990-07-01
Project End
1995-06-30
Budget Start
1992-07-01
Budget End
1993-06-30
Support Year
3
Fiscal Year
1992
Total Cost
Indirect Cost

  Institution

Name
Harvard University
Department
Type
Schools of Medicine
DUNS #
082359691
City
Boston
State
MA
Country
United States
Zip Code
02115

  Publications

Chi, Binkai; O'Connell, Jeremy D; Yamazaki, Tomohiro et al. (2018) Interactome analyses revealed that the U1 snRNP machinery overlaps extensively with the RNAP II machinery and contains multiple ALS/SMA-causative proteins. Sci Rep 8:8755
Paolella, Brenton R; Gibson, William J; Urbanski, Laura M et al. (2017) Copy-number and gene dependency analysis reveals partial copy loss of wild-type SF3B1 as a novel cancer vulnerability. Elife 6:
Yin, Shanye; Lopez-Gonzalez, Rodrigo; Kunz, Ryan C et al. (2017) Evidence that C9ORF72 Dipeptide Repeat Proteins Associate with U2 snRNP to Cause Mis-splicing in ALS/FTD Patients. Cell Rep 19:2244-2256
Wang, Lili; Brooks, Angela N; Fan, Jean et al. (2016) Transcriptomic Characterization of SF3B1 Mutation Reveals Its Pleiotropic Effects in Chronic Lymphocytic Leukemia. Cancer Cell 30:750-763
Kumar, Raman; Corbett, Mark A; van Bon, Bregje W M et al. (2015) THOC2 Mutations Implicate mRNA-Export Pathway in X-Linked Intellectual Disability. Am J Hum Genet 97:302-10
Yin, Shanye; Yu, Yong; Reed, Robin (2015) Primary microRNA processing is functionally coupled to RNAP II transcription in vitro. Sci Rep 5:11992
Shi, Min; Zhang, Heng; Wang, Lantian et al. (2015) Premature Termination Codons Are Recognized in the Nucleus in A Reading-Frame Dependent Manner. Cell Discov 1:
Yu, Yong; Chi, Binkai; Xia, Wei et al. (2015) U1 snRNP is mislocalized in ALS patient fibroblasts bearing NLS mutations in FUS and is required for motor neuron outgrowth in zebrafish. Nucleic Acids Res 43:3208-18
Yu, Yong; Reed, Robin (2015) FUS functions in coupling transcription to splicing by mediating an interaction between RNAP II and U1 snRNP. Proc Natl Acad Sci U S A 112:8608-13
Folco, Eric G; Reed, Robin (2014) In vitro systems for coupling RNAP II transcription to splicing and polyadenylation. Methods Mol Biol 1126:169-77

Showing the most recent 10 out of 24 publications