Abstract

Adenosine deaminase (ADA), an enzyme of the purine salvage pathway, is a ubiquitous enzyme in mammalian tissues. However the levels of expression are regulated in a tissue-specific manner with ADA activity spanning a range of several hundred-fold among various tissues. Expression of ADA is regulated temporally during development of certain tissues and ADA expression is also altered during the functional differentiation of specific cell types. Abnormal levels of expression of ADA are associated with disease states, with very low levels causing severe combined immunodeficiency disease and high levels resulting in hereditary hemolytic anemia. The long-term objective of this application is to define the mechanisms and elements involved in determining the level of tissue- specific ADA expression and eh variation of expression during normal development and differentiation. Recent isolation and characterization of DNA encompassing the ADA gene makes this feasible. The ADA gene contains a basic promoter comprised of G/C rich elements of the type that bind Spl. A unifying theme for regulatory elements that interact with Spl responsive promoters has not been identified tissue-specific pattern.
The specific aims of this application are to define and characterize positive regulatory elements identified in the first intron of the ADA gene, negative elements identified in the 5'-flanking region, and any additional elements in intragenic and specific and development expression of ADA. Primary methods will be construction and transfection of hybrid genes and production of transgenic mice with fragments of these constructions. Assays for gene expression, at the level of enzyme activity and mRNA, will allow evaluation of the significance of particular DNA elements and their interactions in regulation of expression of ADA. In concert deletional analysis, nuclease hypersensitivity, genomic footprinting, and competition studies will map and define the elements. These methods will also be used to determine the fine structure of the G/C rich basic promoter and elucidate its interaction with the defined regulatory elements. Knowledge of the elements necessary to specify proper ADA expression may be critical in therapeutic applications such as gene replacement therapy.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
5R01GM042969-04
Application #
3301923
Study Section
Mammalian Genetics Study Section (MGN)
Project Start
1990-07-01
Project End
1995-06-30
Budget Start
1993-07-01
Budget End
1994-06-30
Support Year
4
Fiscal Year
1993
Total Cost
Indirect Cost

  Institution

Name
Cincinnati Children's Hospital Medical Center
Department
Type
DUNS #
071284913
City
Cincinnati
State
OH
Country
United States
Zip Code
45229

  Publications

Brickner, A G; Koop, B F; Aronow, B J et al. (1999) Genomic sequence comparison of the human and mouse adenosine deaminase gene regions. Mamm Genome 10:95-101
Haynes, T L; Thomas, M B; Dusing, M R et al. (1996) An enhancer LEF-1/TCF-1 site is essential for insertion site-independent transgene expression in thymus. Nucleic Acids Res 24:5034-44
Brickner, A G; Gossage, D L; Dusing, M R et al. (1995) Identification of a murine homolog of the human adenosine deaminase thymic enhancer. Gene 167:261-6
Dusing, M R; Wiginton, D A (1994) Sp1 is essential for both enhancer-mediated and basal activation of the TATA-less human adenosine deaminase promoter. Nucleic Acids Res 22:669-77
Aronow, B J; Silbiger, R N; Dusing, M R et al. (1992) Functional analysis of the human adenosine deaminase gene thymic regulatory region and its ability to generate position-independent transgene expression. Mol Cell Biol 12:4170-85