Abstract

Our goal is to understand the mechanism of chromosome segregation during meiosis, particularly how homologous chromosomes pair and synapse. The maize male meiocyte is the only system where there is a large collection of mutants that affect meiosis, and it is possible to do superb cytology. We have collected 3-D images on a deconvolution light microscope system using fluorescence in situ hybridization (FISH) probes and antibodies against RAD51 to describe the rearrangements of telomeres, chromosomes and the recombination machinery during the homology search. There is no premeiotic association of homologs; rather, homologous chromosomes approach each other at the end of leptotene as telomeres associate with the nuclear envelope (NE) and cluster (bouqet formation). We will use FISH probes which light up multiple spots on one specific chromosome arm, FISH centromere specific probes, and antibodies against the recombination machinery (RAD51, MSH2/6) to analyze in 3-D homolog alignment as pairing is initiated. Analysis of the pairing behavior of chromosomal derivatives deficient in synapsis such as rings, deficiency heterozygotes, ditelocentrics and reciprocal translocations will allow us to test the requirements for chromosome ends, telomeric sequences, and subtelomeric or internal homology, for successful pairing. We will analyze the pairing behavior of chromosomes in mutants known to be deficient in the early stages of the homology search (afd, dsy1) or in later stages (as1, dy1, dsy2, etc.). We are developing novel screens based on partial pollen abortion or altered recombination rates to find new meiotic mutants. We are using directed transposon tagging to clone new mutants or existing mutants which are defective in pairing. We assume that the homology search is dependent on the active movement of chromosomes, mediated by telomere-NE associations. We will analyze homolog alignment and telomere clustering in living meiocytes using large blocks of heterochromatin (knobs) as markers. Colchicine blocks telomere interactions with the NE in vitro. We will analyze how colchicine disrupts other aspects on nuclear organization such as nuclear pore distribution. Meiosis is essential for all sexually reproducing organisms and the studies described here will further our understanding of this process not only in maize but in all organisms. The mechanism of meiosis is a topic of major medical interest inaccurate chromosome segregation (aneuploidy) during meiosis is casual in several congenital malformations, a major cause of premature termination of pregnancy, and of poor gamete production in humans.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
5R01GM048547-06
Application #
6180094
Study Section
Special Emphasis Panel (ZRG1-SSS-I (03))
Program Officer
Carter, Anthony D
Project Start
1994-08-01
Project End
2003-06-30
Budget Start
2000-07-01
Budget End
2001-06-30
Support Year
6
Fiscal Year
2000
Total Cost
$269,378
Indirect Cost

  Institution

Name
University of California Berkeley
Department
Biochemistry
Type
Schools of Arts and Sciences
DUNS #
094878337
City
Berkeley
State
CA
Country
United States
Zip Code
94704

  Publications

Golubovskaya, Inna N; Wang, C J Rachel; Timofejeva, Ljudmilla et al. (2011) Maize meiotic mutants with improper or non-homologous synapsis due to problems in pairing or synaptonemal complex formation. J Exp Bot 62:1533-44
Wang, Chung-Ju Rachel; Carlton, Peter M; Golubovskaya, Inna N et al. (2009) Interlock formation and coiling of meiotic chromosome axes during synapsis. Genetics 183:905-15
Gustafsson, Mats G L; Shao, Lin; Carlton, Peter M et al. (2008) Three-dimensional resolution doubling in wide-field fluorescence microscopy by structured illumination. Biophys J 94:4957-70
Golubovskaya, Inna N; Hamant, Olivier; Timofejeva, Ljuda et al. (2006) Alleles of afd1 dissect REC8 functions during meiotic prophase I. J Cell Sci 119:3306-15
Jin, Ye; Mancuso, Joel J; Uzawa, Satoru et al. (2005) The fission yeast homolog of the human transcription factor EAP30 blocks meiotic spindle pole body amplification. Dev Cell 9:63-73
Hamant, Olivier; Golubovskaya, Inna; Meeley, Robert et al. (2005) A REC8-dependent plant Shugoshin is required for maintenance of centromeric cohesion during meiosis and has no mitotic functions. Curr Biol 15:948-54
Franklin, Amie E; Golubovskaya, Inna N; Bass, Hank W et al. (2003) Improper chromosome synapsis is associated with elongated RAD51 structures in the maize desynaptic2 mutant. Chromosoma 112:17-25
Jin, Ye; Uzawa, Satoru; Cande, W Z (2002) Fission yeast mutants affecting telomere clustering and meiosis-specific spindle pole body integrity. Genetics 160:861-76
Bass, H W; Riera-Lizarazu, O; Ananiev, E V et al. (2000) Evidence for the coincident initiation of homolog pairing and synapsis during the telomere-clustering (bouquet) stage of meiotic prophase. J Cell Sci 113 ( Pt 6):1033-42
Kaszas, E; Cande, W Z (2000) Phosphorylation of histone H3 is correlated with changes in the maintenance of sister chromatid cohesion during meiosis in maize, rather than the condensation of the chromatin. J Cell Sci 113 ( Pt 18):3217-26

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