Abstract

The enzyme prostaglandin H (PGH) synthase catalyzes the oxidation of arachidonic acid to the hydroperoxy endoperoxide, PGG2, and the reduction of PGG2 to the hydroxy endoperoxide, PGH2. The enzyme has an important role in numerous physiological and pathophysiological processes including inflammation, thrombosis, carcinogenesis, and metastasis. Recent results suggest it is induced in response to treatment of cells with tumor promoters. The hydroperoxide intermediate, PGG2, triggers the oxidative inactivation of PGH synthase, which limits its ability to make bioactive arachidonic acid metabolites. Reducing substrates for the peroxidase activity of PHG synthase lower the steady-state level of PGG2, protect the enzyme from inactivation, and enhance the conversion of arachidonate to PGH2. This may account for the ability of certain drugs to stimulate biosynthesis of the antithrombotic and antimetastatic agent, prostacyclin, by vascular endothelium. Relatively little is known of the structure of PGH synthase and its relation to function. We propose a series of investigations to determine the primary structure of PGH synthase, elucidate the biochemical basis of hydroperoxide-dependent inactivation of PGH synthase, isolate the active site domain of PGH synthase, and design maximally effective peroxidase reducing substrates. Recombinant DNA technology will be used to determine the DNA sequence of a molecular clone of cDNA for ram seminal vesicle PGH synthase. Exhaustive tryptic digestion, mapping, and sequencing will be employed to detect peptides containing amino acid residues oxidized as a result of self-inactivation. The location of oxidized residues in the sequence should be useful in establishing the location of the active site(s) of the cyclooxygenase and peroxidase of PGH synthase. A series of aralkyl sulfides will be constructed that possess high peroxidase reducing substrate activity in order to maximize pharmacological protection of PGH synthase from oxidative inactivation. Literature precedents suggest that such compounds should be effective antithrombotic and antimetastatic agents. Controlled proteolysis of PGH synthase appears to generate a membrane- binding domain and an active site domain. Techniques will be developed to purify the active site domain in order to characterize its cyclooxygenase and peroxidase activities for comparison to the intact enzyme. The proposed experiments should significantly advance our knowledge of structure-function relationships for PGH synthase, reveal the biochemical basis for self-catalyzed inactivation, and provide new strategies for the development of antithrombotic and antimetastatic agents.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
5R01GM023642-11
Application #
3271810
Study Section
Biochemistry Study Section (BIO)
Project Start
1977-01-01
Project End
1990-06-30
Budget Start
1988-07-01
Budget End
1989-06-30
Support Year
11
Fiscal Year
1988
Total Cost
Indirect Cost

  Institution

Name
Wayne State University
Department
Type
Schools of Arts and Sciences
DUNS #
City
Detroit
State
MI
Country
United States
Zip Code
48202

  Publications

Marnett, L J (1990) Prostaglandin synthase-mediated metabolism of carcinogens and a potential role for peroxyl radicals as reactive intermediates. Environ Health Perspect 88:5-12
Odenwaller, R; Chen, Y N; Marnett, L J (1990) Preparation and proteolytic cleavage of apoprostaglandin endoperoxide synthase. Methods Enzymol 187:479-85
Chen, Y N; Marnett, L J (1989) Heme prosthetic group required for acetylation of prostaglandin H synthase by aspirin. FASEB J 3:2294-7
Ple, P; Marnett, L J (1989) Alkylaryl sulfides as peroxidase reducing substrates for prostaglandin H synthase. Probes for the reactivity and environment of the ferryl-oxo complex. J Biol Chem 264:13983-93
Marnett, L J; Chen, Y N; Maddipati, K R et al. (1989) Localization of the peroxidase active site of PGH synthase. Adv Prostaglandin Thromboxane Leukot Res 19:458-61
Marnett, L J; Chen, Y N; Maddipati, K R et al. (1988) Functional differentiation of cyclooxygenase and peroxidase activities of prostaglandin synthase by trypsin treatment. Possible location of a prosthetic heme binding site. J Biol Chem 263:16532-5
Chen, Y N; Bienkowski, M J; Marnett, L J (1987) Controlled tryptic digestion of prostaglandin H synthase. Characterization of protein fragments and enhanced rate of proteolysis of oxidatively inactivated enzyme. J Biol Chem 262:16892-9
Marnett, L J (1987) Peroxyl free radicals: potential mediators of tumor initiation and promotion. Carcinogenesis 8:1365-73
Lambeir, A M; Markey, C M; Dunford, H B et al. (1987) Spectral properties of the higher oxidation states of prostaglandin H synthase. Adv Prostaglandin Thromboxane Leukot Res 17A:25-8
Markey, C M; Alward, A; Weller, P E et al. (1987) Quantitative studies of hydroperoxide reduction by prostaglandin H synthase. Reducing substrate specificity and the relationship of peroxidase to cyclooxygenase activities. J Biol Chem 262:6266-79

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