Abstract

Proteins are targets of reactive oxygen species (ROS) that are produced in the environment and in the course of normal and xenobiotic metabolism. Protein oxidation is often detrimental, but it may be involved in normal biological processes. Hydrogen peroxide is a common ROS produced in the environment and in the cell, e.g. the mitochondrion. Hydrogen peroxide is the mildest of the ROS and is the most likely to act at sites distant from it's generation. Rhodanese, a sulfur-transfer enzyme in the mitochondrial matrix, can regulate iron-sulfur centers, and it may be controlled by oxidation. Rhodanese can be reversibly and irreversibly modified by hydrogen peroxide. Properties of modified rhodanese are those reported to be involved in damage, aging and turnover. This research program will characterize the altered forms and will determine the mechanism for conformational changes triggered by oxidation. Analyses can be pursued in unprecedented detail because of extensive kinetic and X-ray information already available for rhodanese. Our working hypotheses are: a) oxidation can be considered as a post- translational protein modification; b) oxidative damage is progressive and can be initiated by reaction at specific sites; c) oxidative effects can be propagated to distant regions of the protein; and d) oxidation and conformational changes are reciprocally linked, each facilitating the other. The specific approaches would be as follows: I. Oxidized amino acids will be located in the sequence of reversibly and irreversibly oxidized rhodanese. Oxidation states of sulfhydryl groups will be determined. II. Sequencing methods will be used to determine regions of the protein, not directly oxidized, that respond to oxidation. This is possible because oxidation reveal new antigenic determinants and exposes sites of proteolysis. III. Non-covalent conformational consequences of oxidation will be probed by physico-chemical methods. Changes in conformation, flexibility and domain interactions will be measured using: fluorescence, circular dichroism, tritium exchange, light scattering and hydrophobic chromatography. IV. Directed mutagenesis will modify regions of rhodanese suggested to either trigger or respond to oxidative changes. Site directed mutagenesis will change cys to ser and remove prolines in the interdomain tether. The N-terminal residues 1-23 will be deleted. C-terminal deletions will be produced by treating recombinant rhodanese with carboxypeptidase. These species will be studied as above.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Environmental Health Sciences (NIEHS)
Type
Research Project (R01)
Project #
1R01ES005729-01
Application #
3254023
Study Section
Toxicology Subcommittee 2 (TOX)
Project Start
1991-08-01
Project End
1996-07-31
Budget Start
1991-08-01
Budget End
1992-07-31
Support Year
1
Fiscal Year
1991
Total Cost
Indirect Cost

  Institution

Name
University of Texas Health Science Center San Antonio
Department
Type
Schools of Medicine
DUNS #
800772162
City
San Antonio
State
TX
Country
United States
Zip Code
78229

  Publications

Mendoza, J A; Horowitz, P M (1994) The chaperonin assisted and unassisted refolding of rhodanese can be modulated by its N-terminal peptide. J Protein Chem 13:15-22
Zardeneta, G; Horowitz, P M (1994) Protein refolding at high concentrations using detergent/phospholipid mixtures. Anal Biochem 218:392-8
Luo, G X; Horowitz, P M (1994) The stability of the molecular chaperonin cpn60 is affected by site-directed replacement of cysteine 518. J Biol Chem 269:32151-4
Luo, G X; Horowitz, P M (1994) The sulfurtransferase activity and structure of rhodanese are affected by site-directed replacement of Arg-186 or Lys-249. J Biol Chem 269:8220-5
Miller-Martini, D M; Chirgwin, J M; Horowitz, P M (1994) Mutations of noncatalytic sulfhydryl groups influence the stability, folding, and oxidative susceptibility of rhodanese. J Biol Chem 269:3423-8
Sloan, I S; Horowitz, P M; Chirgwin, J M (1994) Rapid secretion by a nonclassical pathway of overexpressed mammalian mitochondrial rhodanese. J Biol Chem 269:27625-30
Islam, T A; Miller-Martini, D M; Horowitz, P M (1994) Mutation of cysteine 254 facilitates the conformational changes accompanying the interconversion of persulfide-substituted and persulfide-free rhodanese. J Biol Chem 269:7903-13
Mendoza, J A; Demeler, B; Horowitz, P M (1994) Alteration of the quaternary structure of cpn60 modulates chaperonin-assisted folding. Implications for the mechanism of chaperonin action. J Biol Chem 269:2447-51
Miller-Martini, D M; Hua, S; Horowitz, P M (1994) Cysteine 254 can cooperate with active site cysteine 247 in reactivation of 5,5'-dithiobis(2-nitrobenzoic acid)-inactivated rhodanese as determined by site-directed mutagenesis. J Biol Chem 269:12414-8
Luo, G X; Horowitz, P M (1993) The folding and stability of rhodanese are influenced by the replacement of glutamic acid 17 in the NH2-terminal helix by proline but not by glutamine. J Biol Chem 268:10246-51

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