Abstract

Cancer arises from cells that escape normal growth regulation through mutations that activate growth-promoting protooncogenes and inactivate tumor suppressor genes. Most often, these genetic alterations are somatic events, but rare individuals are born with heritable, germline mutations of tumor-related genes that make them extremely prone to cancer. Analysis of hereditary cancer predisposition syndromes has been critically important in delineating the role of tumor suppressor genes. Basal cell carcinomas of the skin (BCCs) are the most common malignancies in humans, accounting for approximately one third of all cancers in the U.S. There are slow growing tumors that rarely metastasize, but which can cause significant morbidity and occasional mortality from local invasion. Environmental mutagens, such as ultraviolet and ionizing radiation, are strong risk factors; but little is known about the specific genetic alterations involved in basal cell carcinogenesis. Occasionally these neoplasms arise in an hereditary setting, most commonly in association with Gorlin syndrome. This autosomal dominant disorder is characterized by multiple BCCs, ovarian fibromas, medulloblastomas, meningiomas, fibrosarcomas, and widespread developmental anomalies. In preliminary studies, we showed that the Gorlin syndrome gene maps to chromosome 9q22.3-31 and is deleted in nearly all hereditary and sporadic BCCs. Presumably the gene is a novel tumor suppressor with a critically important role in both carcinogenesis and embryogenesis. Analyzing the function of this gene will help delineate the molecular basis for neoplasia in a variety of solid tumors and, in addition, the role of tumor suppressors in normal development. The purpose of this study is to refine the map location of the gene and to isolate it using positional cloning techniques. A 9q22.3-31 microdissected library will be screened for new STRs, and the map location of the gene will be refined by tumor deletion and linkage studies. Existing YAC contigs that have been constructed by random L1 fingerprinting of the CEPH large-insert library will be tested for the presence of markers in the Gorlin syndrome region and will be further analyzed and extended by content mapping with the new STRs. Simultaneously pools of single copy clones from the microdissected library will be used to directly screen cDNA libraries from tissues in which the gene is likely to be expressed. Those cDNAs that lie in the region of the YAC contig between the closest flanking markers will be analyzed for expression in normal skin cells versus basal cell carcinomas and for mutations in Gorlin syndrome patients. If none of these candidates proves to be the Gorlin syndrome gene, direct cDNA selection from YACs will be used as a complementary and more comprehensive method of identifying additional candidates.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Cancer Institute (NCI)
Type
Research Project (R01)
Project #
5R01CA057605-02
Application #
2098343
Study Section
Mammalian Genetics Study Section (MGN)
Project Start
1994-03-10
Project End
1997-02-28
Budget Start
1995-03-01
Budget End
1996-02-29
Support Year
2
Fiscal Year
1995
Total Cost
Indirect Cost

  Institution

Name
Yale University
Department
Genetics
Type
Schools of Medicine
DUNS #
082359691
City
New Haven
State
CT
Country
United States
Zip Code
06520

  Publications

Cooper, Ayanna F; Yu, Kuan Ping; Brueckner, Martina et al. (2005) Cardiac and CNS defects in a mouse with targeted disruption of suppressor of fused. Development 132:4407-17
Barreto, D C; Bale, A E; De Marco, L et al. (2002) Immunolocalization of PTCH protein in odontogenic cysts and tumors. J Dent Res 81:757-60
Dong, J; Gailani, M R; Pomeroy, S L et al. (2000) Identification of PATCHED mutations in medulloblastomas by direct sequencing. Hum Mutat 16:89-90
Barreto, D C; Gomez, R S; Bale, A E et al. (2000) PTCH gene mutations in odontogenic keratocysts. J Dent Res 79:1418-22
Petroianu, A; Boson, W L; Bale, A E et al. (1999) Mutational analyses of candidate genes in human squamous cell carcinomas. Laryngoscope 109:661-3
Levanat, S; Chidambaram, A; Wicking, C et al. (1997) Pulsed-field gel electrophoresis and FISH mapping of chromosome 9q22: placement of a novel zinc finger gene within the NBCCS and ESS1 region. Cytogenet Cell Genet 76:208-13
Walter, A W; Pivnick, E K; Bale, A E et al. (1997) Complications of the nevoid basal cell carcinoma syndrome: a case report. J Pediatr Hematol Oncol 19:258-62
Chidambaram, A; Goldstein, A M; Gailani, M R et al. (1996) Mutations in the human homologue of the Drosophila patched gene in Caucasian and African-American nevoid basal cell carcinoma syndrome patients. Cancer Res 56:4599-601
Levanat, S; Gorlin, R J; Fallet, S et al. (1996) A two-hit model for developmental defects in Gorlin syndrome. Nat Genet 12:85-7
Hahn, H; Wicking, C; Zaphiropoulous, P G et al. (1996) Mutations of the human homolog of Drosophila patched in the nevoid basal cell carcinoma syndrome. Cell 85:841-51

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