Your search keyword '"Sang S"' showing total 11 results

1. Ethanol increases cytochromes P450IIE, IIB1/2, and IIIA in cultured rat hepatocytes

Author

Jacqueline F. Sinclair, Sheryl G. Wood, E.Lucile Smith, Jennifer McCaffrey, John B. Schenkman, Sang S. Park, Harry V. Gelboin, Peter R. Sinclair, William J. Bement, Philip S. Guzelian, and Linda K. Lambrecht

Subjects

Male, Hemeprotein, Cytochrome, Biophysics, Biology, Hydroxylation, Biochemistry, Dexamethasone, Troleandomycin, Nitrophenols, chemistry.chemical_compound, Cytochrome P-450 Enzyme System, medicine, Animals, Molecular Biology, Cells, Cultured, Acetaminophen, Ethanol, Cytochrome P450, Rats, Inbred Strains, Glutathione, Molecular biology, Rats, Liver, chemistry, Cell culture, Phenobarbital, Cytochrome P-450 CYP2B1, biology.protein, Oxidoreductases, medicine.drug

Abstract

In intact rats, ethanol treatment has been associated with increases in hepatic levels of both P450IIB1/2 and P450IIE. When rat hepatocytes were cultured on an extracellular tumor matrix (Matrigel), exposure to ethanol from 48 to 96 h in culture resulted in increases in cytochromes P450IIE, IIB1/2, and IIIA. Cytochrome P450IIE was detected immunologically and enzymatically, using two activities associated with cytochrome P450IIE, p-nitrophenol hydroxylation, and acetaminophen activation to a metabolite that binds to glutathione. The content of cytochrome P450IIE in freshly isolated cells decreased when the cells were placed in culture. Exposure of the cultured hepatocytes to ethanol from 48 to 96 h after inoculation resulted in an increase in cytochrome P450IIE compared to untreated cultured cells. In addition, in culture, the amount of enzymatically active protein after ethanol treatment was equal to that in hepatocytes freshly isolated from intact animals. Ethanol treatment resulted in increases in cytochrome P450IIB1/2 compared to untreated cells, as shown immunologically and by increased benzyloxyresorufin dealkylase activity. However, phenobarbital induced cytochrome P450IIB1/2 to higher levels, compared to ethanol. Ethanol and phenobarbital treatments both increased P450IIIA, as determined immunologically and by the amount of propoxycoumarin depropylase activity that is inhibited by triacetyloleandomycin. However, the amount of P450IIIA increased after ethanol treatment was less than that increased after treatment with dexamethasone in these cells. The ethanol-mediated increases in all four forms of cytochrome P450 in culture suggest that these increases in the intact animal result from direct effects of ethanol on the liver.

Published

1991

2. Ethanol increases cytochromes P450IIE, IIB1/2, and IIIA in cultured rat hepatocytes

Author

Sinclair, Jacqueline F., primary, McCaffrey, Jennifer, additional, Sinclair, Peter R., additional, Bement, William J., additional, Lambrecht, Linda K., additional, Wood, Sheryl G., additional, Smith, E.Lucile, additional, Schenkman, John B., additional, Guzelian, Philip S., additional, Park, Sang S., additional, and Gelboin, Harry V., additional

Published

1991

3. Monoclonal antibody-directed characterization of rat hepatic P450 catalyzing the ω-1 and ω-2 hydroxylation of prostaglandins

Author

Sang S. Park, Harry V. Gelboin, Karsten A. Holm, and David Kupfer

Subjects

Male, Biophysics, Antigen-Antibody Complex, Reductase, Hydroxylation, Biochemistry, Isozyme, Chromatography, Affinity, Mixed Function Oxygenases, chemistry.chemical_compound, Cytochrome P-450 Enzyme System, Animals, Molecular Biology, chemistry.chemical_classification, biology, Antibodies, Monoclonal, Cytochrome P450, Rats, Inbred Strains, Monooxygenase, Rats, Kinetics, Enzyme, chemistry, Phenobarbital, Methylcholanthrene, Microsomes, Liver, Microsome, biology.protein

Abstract

Previous studies have demonstrated that methylcholanthrene (MC) treatment of rats increases 10-fold the ω-2 hydroxylation of prostaglandin E 2 (PGE 2 ) by liver microsomes ( K. A. Holm, R. J. Engell, and D. Kupfer (1985) Arch. Biochem. Biophys. 237 , 477–489 ). The current study identifies the cytochrome P450 form, which catalyzes a major portion of the ω-2 hydroxylation of prostaglandins in liver microsomes of MC-treated rats (MC-microsomes) and examines whether the same enzyme catalyzes this reaction in microsomes from untreated rats (control microsomes). Three monoclonal antibodies (MAbs), MC 1-7-1,1-31-2, and 1-36-1, raised against the major liver P450 from MC-treated rats were used. MAb 1-7-1 binds P450 57K and P450 56K (P450c and P450d, respectively); MAb 1-31-2 binds primarily P450 57K ; and 1-36-1 binds solely P450 57K . MAb 1-7-1 inhibited ω-2 and ω-1 PGE 2 hydroxylations in MC-microsomes by 70 and 45%, respectively. By contrast, MAb 1-31-2 and 1-36-1 were not inhibitory. MAb 1-7-1 did not inhibit PGE 2 ω-2 hydroxylation in control or in microsomes from phenobarbital-treated rats (PB-microsomes). Since MAb 1-7-1 binds to both P450c and P450d, and 1-31-2 and 1-36-1 bind to P450c but are not inhibitory, these findings did not permit the determination of whether in MC microsomes a single isozyme (P450c or P450d) or both isozymes catalyze the ω-2 hydroxylation. This question was partially resolved by the observation that immunoaffinity-isolated P450c, supplemented with purified NADPH-P450 reductase, catalyzes effectively the ω-2 hydroxylation and to a lesser extent the ω-1 hydroxylation. There was no activity in the absence of reductase. The P450 antibody complex exhibits characteristics similar to those of the ω-2 hydroxylating activity in intact MC-microsomes supported by H 2 O 2 , by demonstrating a much higher activity when H 2 O 2 is used instead of reductase and NADPH. Furthermore, a reconstituted monooxygenase composed of rat liver reductase and P450c, purified by conventional means, hydroxylated PGE 2 at the ω-2 and ω-1 sites at a ratio of 2.8, similar to that obtained with the P450-antibody complex. These findings demonstrate that a major portion of the ω-2 hydroxylation of PGs in MC-microsomes is catalyzed by P450c; however, the possibility that some ω-2 hydroxylating activity is due to P450d was not ruled out. Certain purified P450s (RLM 5 and 5a) from untreated rat liver catalyze the ω-2 hydroxylation of PGE 2 (D. Kupfer et al. (1988) Arch. Biochem. Biophys. 261 , 186–195). The current findings demonstrate that all the ω-2 hydroxylation in control microsomes and about 25% of the activity in MC-microsomes is by P450s which are not inhibited by MAb 1-7-1. It is not known whether these resistant P450s are RLM 5, 5a, or different constitutive P450s.

Published

1989

4. Monoclonal antibodies to liver microsomal cytochrome P-450E of the marine fish Stenotomus chrysops (scup): Cross reactivity with 3-methylcholanthrene induced rat cytochrome P-450

Author

Haruko Miller, Harry V. Gelboin, John J. Stegeman, Alan V. Klotz, Sang S. Park, and Pamela J. Kloepper-Sams

Subjects

Immunodiffusion, Cytochrome, Scup, medicine.drug_class, Radioimmunoassay, Biophysics, Cross Reactions, Monoclonal antibody, Biochemistry, Isozyme, Epitope, Epitopes, Mice, chemistry.chemical_compound, Cytochrome P-450 Enzyme System, medicine, Animals, Molecular Biology, biology, Fishes, Antibodies, Monoclonal, biology.organism_classification, Molecular biology, Rats, Isoenzymes, chemistry, Enzyme Induction, Methylcholanthrene, Microsomes, Liver, biology.protein, Microsome, Rabbits

Abstract

Hybridomas were prepared from myeloma cells and spleen cells of BALB/c female mice immunized with hepatic cytochrome P-450E purified from the marine fish, Stenotomus chrysops (scup). Nine independent hybrid clones produced MAbs, either IgG1, IgG2b, or IgM, that bound to purified cytochrome P-450E in radioimmunoassay. Antibodies from one clone MAb (1-12-3), also strongly recognized rat cytochrome P-450MC-B (P-450BNF-B; P-450c). The nine antibodies inhibited reconstituted aryl hydrocarbon hydroxylase (AHH) and ethoxycoumarin O-deethylase of scup cytochrome P-450E to varying degrees, and inhibited AHH activity of beta-naphthoflavone-induced scup liver microsomes in a pattern similar to that in reconstitutions, indicating that cytochrome P-450E is identical to the AHH catalyst induced in this fish by beta-naphthoflavone. MAb 1-12-3 also inhibited the reconstituted AHH activity of the major BNF-induced rat isozyme. Conversely, MAb 1-7-1 to rat cytochrome P-450MC-B had little effect on AHH activity of scup cytochrome P-450E, and did not recognize cytochrome P-450E in radioimmunoassay nor in an immunoblot. Scup cytochrome P-450E and rat cytochrome P-450MC-B thus have at least one common epitope recognized by MAb 1-12-3, but the epitope recognized by Mab 1-7-1 is absent or recognized with low affinity in cytochrome P-450E. The various assays indicate that the nine MAbs against cytochrome P-450E are directed to different epitopes of the molecule. These MAbs should be useful in determining phylogenetic relationships of the BNF- or MC-inducible isozymes and their regulation by other environmental factors.

Published

1986

5. Specificity and cross-reactivity of monoclonal and polyclonal antibodies against cytochrome P-450E of the marine fish scup

Author

Harry V. Gelboin, John J. Stegeman, Sang S. Park, and Pamela J. Kloepper-Sams

Subjects

Cytochrome, medicine.drug_class, Scup, Biophysics, Cross Reactions, Monoclonal antibody, Biochemistry, Isozyme, Cytochrome P-450 Enzyme System, Antibody Specificity, Microsomes, medicine, Animals, Killifish, Molecular Biology, Immunosorbent Techniques, biology, Fishes, Antibodies, Monoclonal, biology.organism_classification, Molecular biology, Rats, Isoenzymes, Molecular Weight, Trout, Polyclonal antibodies, biology.protein, Microsome

Abstract

Monoclonal antibody (MAb) 1-12-3 generated against liver cytochrome P-450E (P-450E), an aryl hydrocarbon hydroxylase of the marine fish Stenotomus chrysops (scup), reacted only with P-450E when tested in immunoblot analysis with five P-450 fractions from scup liver. This and six other MAbs against P-450E recognized purified P-450E, as well as a single band in β-naphthoflavone (BNF)-induced scup microsomes that comigrated with authentic P-450E. Like MAb 1-12-3, polyclonal anti-P-450E reacted with P-450Ebut not with other scup P-450 fractions and reacted strongly with a band coincident to P-450E in BNF-treated scup microsomes. However, the polyclonal antibody (PAb) also faintly recognized additional microsomal proteins. MAb 1-12-3 recognized P-450Einduced by 3,3′,4,4′,5,5′-hexachlorobiphenyl and by polychlorinated biphenyl mixtures in scup, and a single band induced by BNF or 3-methylcholanthrene (MC) in microsomes of other teleosts, including two trout species, killifish and winter flounder. The content of the P-450E counterpart in these fish and also in untreated scup coincided with induced ethoxyresorufin O-deethylase (EROD) activity. Induced EROD activity in scup and trout was strongly inhibited by MAb 1-12-3, further demonstrating the relationship between P-450E and inducedP-450in trout. MAb 1-12-3, two other MAbs, and anti-P-450E PAb recognized a band comigrating with P-450c in BNF-induced rat microsomes. MAb 1-12-3 also recognized purified rat P-450c. MAb 1-12-3 and anti-P-450E PAb recognized a second band of lower molecular weight than P-450c in BNF rat microsomes which may correspond to P-450d, the MC- and isosafrole-inducible rat isozyme. The results firmly establish the identity of scup P-450E, the relationship of BNF-induced P-450 in other teleosts with P-450E, and the immunochemical relationship of P-450E with rat P-450c. Furthermore, results with untreated fish suggest that effects of environmental chemicals may be detected by immunoblotting with monoclonal anti-P-450E.

Published

1987

6. Mechanism of induction of cytochrome P-450ac (P-450j) in chemically induced and spontaneously diabetic rats

Author

Qiang Ma, Harry V. Gelboin, Sang S. Park, Dechun Li, Zigong Dong, Chung S. Yang, Frank J. Gonzalez, John Bullock, and Junyan Hong

Subjects

medicine.medical_specialty, Cytochrome, medicine.medical_treatment, Biophysics, Biochemistry, Diabetes Mellitus, Experimental, chemistry.chemical_compound, Cytochrome P-450 Enzyme System, Alloxan, Diabetes mellitus, Internal medicine, Demethylase activity, medicine, Animals, Insulin, RNA, Messenger, Enzyme inducer, Molecular Biology, biology, Body Weight, Cytochrome P450, Antibodies, Monoclonal, Rats, Inbred Strains, Organ Size, Streptozotocin, medicine.disease, Rats, Isoenzymes, Endocrinology, chemistry, Enzyme Induction, biology.protein, medicine.drug

Abstract

Previous studies demonstrated that a microsomal high-affinity N-nitrosodimethylamine demethylase activity and cytochrome P-450ac (an acetone/ethanol-inducible form) were induced by streptozotocin-induced diabetes in rats. In the present work, the induction was studied in detail in two chemically induced (by streptozotocin and alloxan) diabetic rat models and one spontaneously (BB/Wor) diabetic rat model. All the diabetic conditions caused increases in three parameters: (a) microsomal N-nitrosodimethylamine demethylase activity which is known to be a good indicator of the level of P-450ac; (b) the levels of P-450ac as determined by immunoblot analysis; and (c) the levels of mRNA of P-450ac as determined by hybridization assays with a cDNA probe for this enzyme. These increases were abolished by treatment of the diabetic rats with insulin. The results suggest that the pathophysiological condition of diabetes is responsible for the induction of P-450ac and elevation of mRNA is involved in all of the three diabetic models investigated.

Published

1988

7. Monoclonal antibodies to liver microsomal cytochrome P-450E of the marine fish Stenotomus chrysops (scup): Cross reactivity with 3-methylcholanthrene induced rat cytochrome P-450

Author

Park, Sang S., primary, Miller, Haruko, additional, Klotz, Alan V., additional, Kloepper-Sams, Pamela J., additional, Stegeman, John J., additional, and Gelboin, Harry V., additional

Published

1986

8. Mechanism of induction of cytochrome P-450ac (P-450j) in chemically induced and spontaneously diabetic rats

Author

Dong, Zigong, primary, Hong, Junyan, additional, Ma, Qiang, additional, Li, Dechun, additional, Bullock, John, additional, Gonzalez, Frank J., additional, Park, Sang S., additional, Gelboin, Harry V., additional, and Yang, Chung S., additional

Published

1988

9. Monoclonal antibody-directed characterization of rat hepatic P450 catalyzing the ω-1 and ω-2 hydroxylation of prostaglandins

Author

Holm, Karsten A., primary, Park, Sang S., additional, Gelboin, Harry V., additional, and Kupfer, David, additional

Published

1989

10. Specificity and cross-reactivity of monoclonal and polyclonal antibodies against cytochrome P-450E of the marine fish scup

Author

Kloepper-Sams, Pamela J., primary, Park, Sang S., additional, Gelboin, Harry V., additional, and Stegeman, John J., additional

Published

1987

11. Mechanism of induction of cytochrome P-450 ac ( P-450 j) in chemically induced and spontaneously diabetic rats

Author

Dong, Zigong, Hong, Junyan, Ma, Qiang, Li, Dechun, Bullock, John, Gonzalez, Frank J., Park, Sang S., Gelboin, Harry V., and Yang, Chung S.

Published

1988