Abstract

Meiosis is a fundamental process that sexually reproducing organisms undergo in order to reduce by half the chromosome number in germ cells. This reduction is necessary so that when two gametes fuse at fertilization the diploid chromosome number of the cell is reconstituted. When meiosis fails, chromosomally imbalanced gametes result. In mammals, the zygotes generated by fertilization of such chromosomally imbalanced gametes are frequently inviable and account for a large number of spontaneous abortions. In cases where viable offspring are produced, mental and morphological defects such as those seen for Trisomy 21 (Down's syndrome) are observed. Understanding how the meiotic process works to accurately segregate homologous chromosomes may ultimately provide the knowledge needed to monitor and prevent failures of the process. In order for homologous chromosomes to segregate properly at the first meiotic division, they must first become physically associated by formation of a multi-protein structure called the synaptonemal complex (SC). The focus of the proposed grant is to determine how the SC is assembled during meiosis and how it functions to direct the segregation of homologous chromosomes to opposite poles at Meiosis I in the yeast Saccharomyces cerevisiae. Two genes, RUM17 and RUM18, have been recently identified using a screen specific for genes involved in meiotic chromosome synapsis. Mutants in these genes exhibit reduced levels of interhomolog recombination and decreased spore viability. In addition, the mechanism by which an acyltransferase, HCS1-7, is able to specifically suppress a defect in the synaptonemal complex component HOPI, will be investigated. In order to find additional genes important for synapsis, two genetic screens, high copy suppression and synthetic spore lethality, will be performed using specially selected alleles of HOP1, RED1, MEK1 and HCS1-7. Mutations in genes arising from the genetic screens will analyzed for their effects on SC formation, recombination and chromosome segregation to assess their functions. Biochemical experiments using a combination of purified proteins and extracts will be performed to determine whether gene products which interact genetically do so by a direct physical interaction. Specifically the model that RED1 physically interacts with HOP1, as well as the model that HOPI is a substrate for the MEK1 kinase will be tested. By combining genetic, biochemical and cytological studies, a greater understanding of the function, structure and pathway of assembly of the SC will be obtained.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
5R01GM050717-04
Application #
2634743
Study Section
Genetics Study Section (GEN)
Project Start
1995-01-01
Project End
1999-12-31
Budget Start
1998-01-01
Budget End
1998-12-31
Support Year
4
Fiscal Year
1998
Total Cost
Indirect Cost

  Institution

Name
State University New York Stony Brook
Department
Biochemistry
Type
Schools of Arts and Sciences
DUNS #
804878247
City
Stony Brook
State
NY
Country
United States
Zip Code
11794

  Publications

Kniewel, Ryan; Murakami, Hajime; Liu, Yan et al. (2017) Histone H3 Threonine 11 Phosphorylation Is Catalyzed Directly by the Meiosis-Specific Kinase Mek1 and Provides a Molecular Readout of Mek1 Activity in Vivo. Genetics 207:1313-1333
Prugar, Evelyn; Burnett, Cameron; Chen, Xiangyu et al. (2017) Coordination of Double Strand Break Repair and Meiotic Progression in Yeast by a Mek1-Ndt80 Negative Feedback Loop. Genetics 206:497-512
Callender, Tracy L; Laureau, Raphaelle; Wan, Lihong et al. (2016) Correction: Mek1 Down Regulates Rad51 Activity during Yeast Meiosis by Phosphorylation of Hed1. PLoS Genet 12:e1006283
Suhandynata, Raymond T; Wan, Lihong; Zhou, Huilin et al. (2016) Identification of Putative Mek1 Substrates during Meiosis in Saccharomyces cerevisiae Using Quantitative Phosphoproteomics. PLoS One 11:e0155931
Hollingsworth, Nancy M (2016) Mek1/Mre4 is a master regulator of meiotic recombination in budding yeast. Microb Cell 3:129-131
Callender, Tracy L; Laureau, Raphaelle; Wan, Lihong et al. (2016) Mek1 Down Regulates Rad51 Activity during Yeast Meiosis by Phosphorylation of Hed1. PLoS Genet 12:e1006226
Park, Jae-Sook; Thorsness, Mary K; Policastro, Robert et al. (2016) Yeast Vps13 promotes mitochondrial function and is localized at membrane contact sites. Mol Biol Cell 27:2435-49
Chen, Xiangyu; Suhandynata, Ray T; Sandhu, Rima et al. (2015) Phosphorylation of the Synaptonemal Complex Protein Zip1 Regulates the Crossover/Noncrossover Decision during Yeast Meiosis. PLoS Biol 13:e1002329
Suhandynata, Ray; Liang, Jason; Albuquerque, Claudio P et al. (2014) A method for sporulating budding yeast cells that allows for unbiased identification of kinase substrates using stable isotope labeling by amino acids in cell culture. G3 (Bethesda) 4:2125-35
Liu, Yan; Gaines, William A; Callender, Tracy et al. (2014) Down-regulation of Rad51 activity during meiosis in yeast prevents competition with Dmc1 for repair of double-strand breaks. PLoS Genet 10:e1004005

Showing the most recent 10 out of 16 publications