Abstract

Our ability to smell thousands of different odors is mediated by a large repertoire of odorant receptors (OR) expressed on sensory neurons in the nose. The Ors bind odorous molecules and transmit this information to the brain. During development, Ors also guide neurons to spatially fixed relay stations in the olfactory bulb. Ors form one of the largest gene families in the mammalian genome, with at least 1000 members. OR genes are distributed on many chromosomes in clusters that may occupy as much as 1 percent of the genome. The family also includes many pseudogenes and OR- like genes that may perform other chemosensory functions, such as cell-cell recognition or sperm chemotaxis. This project s goal is to learn (A) how the diversity of the expressed repertoire of Ors has evolved to meet the differing demands for olfaction in mouse and human; (B) how transcription of these genes is controlled such that each sensory neuron expresses a single OR, while a diverse repertoire is displayed in the nose as a whole; (C) how the specificity of ligand-binding and neuronal-targeting is embodied in the structure of the OR proteins; (D) whether the complex genomic organization of Ors is based on functional considerations; (E) how the OR genes responsible for the sense of smell are distinguished from and organized relative to other members of the family; (F) how the evolutionary dynamic nature of the OR subgenome impacts the functional repertoire; and (G) how the repertoire varies among individuals or with age exposure to odors. We therefore propose to conduct a comprehensive and detailed genomic analysis of the OR families in mouse and human and to integrate these genomic data with assays of gene function and regulation.
Aim 1 is to characterize nearly the full repertoire of Ors active in the olfactory tissue of mouse and human.
Aim 2 is to map the locations of these active Ors and to sequence all OR-like sequences, including pseudogenes and ones functioning outside the nose, at each chromosomal location.
Aim 3 is to characterize genomic sequence encompassing approximately 20 percent of the active OR genes to make paralogous and orthologous comparisons of gene structure and cluster organization.
Aim 4 is to characterize the 5'UTRs and expression patterns of OR genes and to perform functional assays in mice to identify regulatory motifs and structural elements key for ligand-binding and neuron-targeting.
Aim 5 is to develop technology to use cDNA arrays to examine expression profiles of 100's of OR genes at once. This partnership between the Axel group, with expertise in transgenics and olfactory biology, and the Trask and Hood groups, with experience in sequencing, genomic evolution, and cDNA-array technology, represents a unique opportunity to unite the worlds of large-scale genomics and functional biology. It is our belief that this sort of partnership in functional genomics represents a model for future collaborative efforts to characterize complex neurobiological systems and large gene families.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute on Deafness and Other Communication Disorders (NIDCD)
Type
Research Project (R01)
Project #
5R01DC004209-02
Application #
6176115
Study Section
Genome Study Section (GNM)
Program Officer
Davis, Barry
Project Start
1999-09-01
Project End
2000-09-27
Budget Start
2000-09-01
Budget End
2000-09-27
Support Year
2
Fiscal Year
2000
Total Cost
$20,274
Indirect Cost

  Institution

Name
University of Washington
Department
Biochemistry
Type
Schools of Medicine
DUNS #
135646524
City
Seattle
State
WA
Country
United States
Zip Code
98195

  Publications

Young, Janet M; Luche, Ralf M; Trask, Barbara J (2011) Rigorous and thorough bioinformatic analyses of olfactory receptor promoters confirm enrichment of O/E and homeodomain binding sites but reveal no new common motifs. BMC Genomics 12:561
Karn, Robert C; Young, Janet M; Laukaitis, Christina M (2010) A candidate subspecies discrimination system involving a vomeronasal receptor gene with different alleles fixed in M. m. domesticus and M. m. musculus. PLoS One 5:
Young, Janet M; Massa, Hillary F; Hsu, Li et al. (2010) Extreme variability among mammalian V1R gene families. Genome Res 20:10-8
Holcomb, Ilona N; Young, Janet M; Coleman, Ilsa M et al. (2009) Comparative analyses of chromosome alterations in soft-tissue metastases within and across patients with castration-resistant prostate cancer. Cancer Res 69:7793-802
Rudd, M Katharine; Endicott, Raelynn M; Friedman, Cynthia et al. (2009) Comparative sequence analysis of primate subtelomeres originating from a chromosome fission event. Genome Res 19:33-41
Holcomb, Ilona N; Grove, Douglas I; Kinnunen, Martin et al. (2008) Genomic alterations indicate tumor origin and varied metastatic potential of disseminated cells from prostate cancer patients. Cancer Res 68:5599-608
Young, Janet M; Endicott, Raelynn M; Parghi, Sean S et al. (2008) Extensive copy-number variation of the human olfactory receptor gene family. Am J Hum Genet 83:228-42
Young, Janet M; Trask, Barbara J (2007) V2R gene families degenerated in primates, dog and cow, but expanded in opossum. Trends Genet 23:212-5
Young, Janet M; Waters, Hang; Dong, Cora et al. (2007) Degeneration of the olfactory guanylyl cyclase D gene during primate evolution. PLoS One 2:e884
Lomvardas, Stavros; Barnea, Gilad; Pisapia, David J et al. (2006) Interchromosomal interactions and olfactory receptor choice. Cell 126:403-13

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