Abstract

The goal of the international human genome effort is to identify all of the genes encoded by the genome and map them to specific regions of individual chromosomes. The advent of efficient methods to construct physical maps of the genome and the successful completion of physical maps for chromosomes 21 and Y underscore the need to accelerate efforts to isolate and map coding sequences. In this project of the program, we propose to isolate cDNAs corresponding to genes encoded by chromosome 12. The first step of this program is to construct a highly representative, short fragment cDNA library which is normalized so that each member of the library is represented equally. Highly purified poly(A)+ RNA from a large number of adult and developing human tissues will be used as substrates for preparation of short fragment cDNA libraries using random oligomers as primers. Individual size selected libraries will be cloned into phage vectors and each of the libraries will be normalized by hybridization procedures which we have developed. Different libraries will be mixed and renormalized to generate a comprehensive normalized library. We expect this library to represent at least 75-80% of the genes encoded by the human genome. DNA from individual or small groups of non-chimeric YACs which have been physically mapped in Projects 1 and 2 will be immobilized on nylon membranes and hybridized with PCR amplified short fragment cDNA library. The cDNAs which hybridize to the YACs will be isolated by PCR and cloned. This procedure is expected to enable us to isolate cDNAs corresponding to one megabase of chromosome 12 DNA at a time. Several members of each of these cDNA packets will be sequenced by the cycle sequencing procedure to examine the quality and integrity of the cDNA packets isolated. In addition, these sequences can yield a low resolution expressed sequence tag (EST) map of chromosome 12. The availability of cDNA packets corresponding to specific, highly defined regions of the chromosome would be a starting point to isolate individual genes from those regions or to initiate a larger scale sequencing effort to define all of the genes encoded by chromosome 12.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Human Genome Research Institute (NHGRI)
Type
Research Program Projects (P01)
Project #
1P01HG000965-01
Application #
3779464
Study Section
Project Start
Project End
Budget Start
Budget End
Support Year
1
Fiscal Year
1993
Total Cost
Indirect Cost

  Institution

Name
Albert Einstein College of Medicine
Department
Type
DUNS #
009095365
City
Bronx
State
NY
Country
United States
Zip Code
10461

  Publications

Renault, B; Hovnanian, A; Bryce, S et al. (1997) A sequence-ready physical map of a region of 12q24.1. Genomics 45:271-8
Nadkarni, P M (1997) Concept locator: a client-server application for retrieval of UMLS metathesaurus concepts through complex boolean query. Comput Biomed Res 30:323-36
Merscher, S; Marondel, I; Pedeutour, F et al. (1997) Identification of new translocation breakpoints at 12q13 in lipomas. Genomics 46:70-7
Nadkarni, P M (1997) QAV: querying entity-attribute-value metadata in a biomedical database. Comput Methods Programs Biomed 53:93-103
Nadkarni, P M (1997) Mapdiff: determining differences between two genomic maps. Comput Appl Biosci 13:217-25
Basson, C T; Bachinsky, D R; Lin, R C et al. (1997) Mutations in human TBX5 [corrected] cause limb and cardiac malformation in Holt-Oram syndrome. Nat Genet 15:30-5
Nadkarni, P M; Banks, A; Montgomery, K et al. (1996) CONTIG EXPLORER: interactive marker-content map assembly. Genomics 31:301-10
Marondel, I; Renault, B; Lieman, J et al. (1996) Physical mapping of the human neurotensin gene (NTS) between markers D12S1444 and D12S81 on chromosome 12q21. Genomics 38:243-5
Cupelli, L; Renault, B; Leblanc-Straceski, J et al. (1996) Assignment of the human myogenic factors 5 and 6 (MYF5, MYF6) gene cluster to 12q21 by in situ hybridization and physical mapping of the locus between D12S350 and D12S106. Cytogenet Cell Genet 72:250-1
Schoenberg Fejzo, M; Ashar, H R; Krauter, K S et al. (1996) Translocation breakpoints upstream of the HMGIC gene in uterine leiomyomata suggest dysregulation of this gene by a mechanism different from that in lipomas. Genes Chromosomes Cancer 17:1-6

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