Abstract

This project investigates the function of the homeodomain-containing transcription repressors Engrailed (En) and Even-skipped (Eve). How does En locate its target genes within the nucleus? To do so, it appears to interact with the Hox protein cofactors Extradenticle and Homothorax. Each of these cofactors has been shown to be important for the activity of En in repressing a direct target gene in Drosophila embryos. The project will identify the mechanistic basis of these functional interactions in vivo. Studies of cooperative interactions on the DNA will be facilitated by the identification of direct binding sites in the target gene sloppy paired. In order to carry out its function, En has been shown to interact with corepressors, including Groucho (Gro). Like En, Eve has both a Gro interaction region and a Gro-independent repression domain. Why are two repression domains with different functional properties found in both of these developmental regulators? A transgene capable of completely rescuing eve null mutants has been constructed. Since Eve plays a major role in establishing cell fates during several stages of embryogenesis, and target genes have been well characterized, this transgene will be used to study functional distinctions among different classes of repression domain in vivo. What other partner proteins does En interact with to carry out its function? Several proteins have been identified that interact with specific functional domains of En. One interacts with the second class of repression domain in En, and genetic studies indicate that the two proteins have a close functional relationship in vivo. What other partner proteins does Ev interact with to carry out its function? Several proteins have been identified that interact with specific functional domains of En. One interacts with the second class of repression domain in Ev, and genetic studies indicate that the two proteins have a close functional relationship in vivo. Intriguingly, it is the cell cycle regulator cyclin E. This relationship may prove to be an important connection between regulation of transcription and the cell cycle. Analysis of the interaction will serve as a model for testing this hypothesis. This project will utilize genetic, cell culture, and biochemical means to study this and other novel interactions. For those interacting proteins that represent new genes, specific mutations will be identified and analyzed for their effects on the target genes of En, as well as on development generally. These studies will thus lead to a greater understanding of the regulatory mechanisms of homeodomain protein function in development and disease.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
2R01GM050231-05A2
Application #
6046243
Study Section
Cell Development and Function Integrated Review Group (CDF)
Program Officer
Greenberg, Judith H
Project Start
1995-05-01
Project End
2003-12-31
Budget Start
2000-01-01
Budget End
2000-12-31
Support Year
5
Fiscal Year
2000
Total Cost
$214,235
Indirect Cost

  Institution

Name
Thomas Jefferson University
Department
Internal Medicine/Medicine
Type
Schools of Medicine
DUNS #
061197161
City
Philadelphia
State
PA
Country
United States
Zip Code
19107

  Publications

Chetverina, Darya; Fujioka, Miki; Erokhin, Maksim et al. (2017) Boundaries of loop domains (insulators): Determinants of chromosome form and function in multicellular eukaryotes. Bioessays 39:
Peacock, Jacob; Jaynes, James B (2017) Using competition assays to quantitatively model cooperative binding by transcription factors and other ligands. Biochim Biophys Acta Gen Subj 1861:2789-2801
Fujioka, Miki; Mistry, Hemlata; Schedl, Paul et al. (2016) Determinants of Chromosome Architecture: Insulator Pairing in cis and in trans. PLoS Genet 12:e1005889
Lacin, Haluk; Rusch, Jannette; Yeh, Raymond T et al. (2014) Genome-wide identification of Drosophila Hb9 targets reveals a pivotal role in directing the transcriptome within eight neuronal lineages, including activation of nitric oxide synthase and Fd59a/Fox-D. Dev Biol 388:117-33
Fujioka, Miki; Sun, Guizhi; Jaynes, James B (2013) The Drosophila eve insulator Homie promotes eve expression and protects the adjacent gene from repression by polycomb spreading. PLoS Genet 9:e1003883
Fujioka, Miki; Jaynes, James B (2012) Regulation of a duplicated locus: Drosophila sloppy paired is replete with functionally overlapping enhancers. Dev Biol 362:309-19
Fujioka, Miki; Gebelein, Brian; Cofer, Zenobia C et al. (2012) Engrailed cooperates directly with Extradenticle and Homothorax on a distinct class of homeodomain binding sites to repress sloppy paired. Dev Biol 366:382-92
Johnston, Danika M; Sedkov, Yurii; Petruk, Svetlana et al. (2011) Ecdysone- and NO-mediated gene regulation by competing EcR/Usp and E75A nuclear receptors during Drosophila development. Mol Cell 44:51-61
Prazak, Lisa; Fujioka, Miki; Gergen, J Peter (2010) Non-additive interactions involving two distinct elements mediate sloppy-paired regulation by pair-rule transcription factors. Dev Biol 344:1048-59
Fujioka, Miki; Wu, Xian; Jaynes, James B (2009) A chromatin insulator mediates transgene homing and very long-range enhancer-promoter communication. Development 136:3077-87

Showing the most recent 10 out of 36 publications