Abstract

The pathway of AMP degradation in prokaryotic organisms involves AMP nucleosidases, which are N-glycohydrolases. AMP nucleosidases exhibit allosteric activation by MgATP and inhibition by Pi. The pathway for AMP degradation in eukaryotes involves AMP deaminase. Regulation of AMP deaminase is similar to AMP nucleosidase by allosteric activation with ALP and inhibition by Pi. No prokaryotes have been found to contain AMP nucleosidase. The purpose of this proposal is to establish structure, catalytic mechanism, allosteric regulatory mechanism and genetic regulation for enzymes in this family of AMP degrading enzymes. The catalytic and allosteric mechanisms of AMP nucleosidase and AMP deaminase will be investigated by heavy-atom kinetic isotope effects in the presence and absence of allosteric activators. Transition state structures can be established for both of these enzymes. The role of specific amino acids in stabilizing the transition state will be investigated by determination of transition state structure in site- directed enzyme mutants. The amino acid sequences of E. coli AMP nucleosidase and yeast AMP deaminase have been established from the deoxynucleotide sequence of the genomic DNA. X-ray crystal structure will be determined for AMP nucleosidase and will be initiated for yeast AMP deaminase. Crystal structure and chemical modification will e used to establish the amino acids involved in catalysis and in allosteric regulation. The role of enzyme-bound zinc in AMP deaminase will be investigated by EPR studies in which Zn(II) is replaced by Mn(II). Expression of AMP nucleosidase in E. coli is regulated by cAMP and inorganic phosphate levels. The promoter region contains overlapping consensus sequences for phosphate regulatory protein and cAMP receptor protein. Experiments are designed to isolate the phosphate regulatory protein and to quantitate its interaction with phosphate and promoter region of the AMP nucleosidase gene. Competition studies with cyclic receptor protein will establish the nature of the overlapping regulatory regions.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
5R01GM021083-16
Application #
3270237
Study Section
Physiological Chemistry Study Section (PC)
Project Start
1988-02-01
Project End
1993-11-30
Budget Start
1990-12-01
Budget End
1991-11-30
Support Year
16
Fiscal Year
1991
Total Cost
Indirect Cost

  Institution

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

  Publications

Kline, P C; Schramm, V L (1994) Electrostatic potential surfaces of the transition state for AMP deaminase and for (R)-coformycin, a transition state inhibitor. J Biol Chem 269:22385-90
Ehrlich, J I; Schramm, V L (1994) Electrostatic potential surface analysis of the transition state for AMP nucleosidase and for formycin 5'-phosphate, a transition-state inhibitor. Biochemistry 33:8890-6
Schramm, V L; Horenstein, B A; Kline, P C (1994) Transition state analysis and inhibitor design for enzymatic reactions. J Biol Chem 269:18259-62
Sollitti, P; Merkler, D J; Estupinan, B et al. (1993) Yeast AMP deaminase. Catalytic activity in Schizosaccharomyces pombe and chromosomal location in Saccharomyces cerevisiae. J Biol Chem 268:4549-55
Merkler, D J; Schramm, V L (1993) Catalytic mechanism of yeast adenosine 5'-monophosphate deaminase. Zinc content, substrate specificity, pH studies, and solvent isotope effects. Biochemistry 32:5792-9
Merkler, D J; Kline, P C; Weiss, P et al. (1993) Transition-state analysis of AMP deaminase. Biochemistry 32:12993-3001
Horenstein, B A; Schramm, V L (1993) Correlation of the molecular electrostatic potential surface of an enzymatic transition state with novel transition-state inhibitors. Biochemistry 32:9917-25
Horenstein, B A; Schramm, V L (1993) Electronic nature of the transition state for nucleoside hydrolase. A blueprint for inhibitor design. Biochemistry 32:7089-97
Kline, P C; Schramm, V L (1992) Purine nucleoside phosphorylase. Inosine hydrolysis, tight binding of the hypoxanthine intermediate, and third-the-sites reactivity. Biochemistry 31:5964-73
Horenstein, B A; Parkin, D W; Estupinan, B et al. (1991) Transition-state analysis of nucleoside hydrolase from Crithidia fasciculata. Biochemistry 30:10788-95

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