An Activity in Rat Tissues That Modifies Nitrotyrosine-Containing Proteins
Homogenates from rat spleen and lung could modify nitrotyrosine-containing BSA. With incubation, nitrotyrosine-containing BSA lost its epitope to a monoclonal antibody that selectively recognized nitrotyrosine-containing proteins. In the presence of protease inhibitors, the loss of the nitrotyrosine...
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Published in | Proceedings of the National Academy of Sciences - PNAS Vol. 95; no. 20; pp. 11584 - 11589 |
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Main Authors | , , , , , , , , |
Format | Journal Article |
Language | English |
Published |
United States
National Academy of Sciences of the United States of America
29.09.1998
National Acad Sciences National Academy of Sciences |
Subjects | |
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Abstract | Homogenates from rat spleen and lung could modify nitrotyrosine-containing BSA. With incubation, nitrotyrosine-containing BSA lost its epitope to a monoclonal antibody that selectively recognized nitrotyrosine-containing proteins. In the presence of protease inhibitors, the loss of the nitrotyrosine epitope occurred without protein degradation and hydrolysis. This activity was found in supernatant but not particulate fractions of spleen homogenates. The factor was heat labile, was sensitive to trypsin treatment, and was retained after passage through a membrane with a 10-kDa retention. The activity was time- and protein-concentration dependent. The activity increased about 2-fold in spleen extracts with endotoxin (bacterial lipopolysaccharide) treatment of animals, suggesting that the activity is inducible or regulatable. Other nitrotyrosine-containing proteins also served as substrates, while free nitrotyrosine and some endogenous nitrotyrosine-containing proteins in tissue extracts were poor substrates. Although the product and possible cofactors for this reaction have not yet been identified, this activity may be a "nitrotyrosine denitrase" that reverses protein nitration and, thus, decreases peroxynitrite toxicity. This activity was not observed in homogenates from rat liver or kidney, suggesting that there may also be some tissue specificity for the apparent denitrase activity. |
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AbstractList | Homogenates from rat spleen and lung could modify nitrotyrosine-containing BSA. With incubation, nitrotyrosine-containing BSA lost its epitope to a monoclonal antibody that selectively recognized nitrotyrosine-containing proteins. In the presence of protease inhibitors, the loss of the nitrotyrosine epitope occurred without protein degradation and hydrolysis. This activity was found in supernatant but not particulate fractions of spleen homogenates. The factor was heat labile, was sensitive to trypsin treatment, and was retained after passage through a membrane with a 10-kDa retention. The activity was time- and protein-concentration dependent. The activity increased about 2-fold in spleen extracts with endotoxin (bacterial lipopolysaccharide) treatment of animals, suggesting that the activity is inducible or regulatable. Other nitrotyrosine-containing proteins also served as substrates, while free nitrotyrosine and some endogenous nitrotyrosine-containing proteins in tissue extracts were poor substrates. Although the product and possible cofactors for this reaction have not yet been identified, this activity may be a "nitrotyrosine denitrase" that reverses protein nitration and, thus, decreases peroxynitrite toxicity. This activity was not observed in homogenates from rat liver or kidney, suggesting that there may also be some tissue specificity for the apparent denitrase activity. Homogenates from rat spleen and lung could modify nitrotyrosine-containing BSA. With incubation, nitrotyrosine-containing BSA lost its epitope to a monoclonal antibody that selectively recognized nitrotyrosine-containing proteins. Homogenates from rat spleen and lung could modify nitrotyrosine-containing BSA. With incubation, nitrotyrosine-containing BSA lost its epitope to a monoclonal antibody that selectively recognized nitrotyrosine-containing proteins. In the presence of protease inhibitors, the loss of the nitrotyrosine epitope occurred without protein degradation and hydrolysis. This activity was found in supernatant but not particulate fractions of spleen homogenates. The factor was heat labile, was sensitive to trypsin treatment, and was retained after passage through a membrane with a 10-kDa retention. The activity was time- and protein-concentration dependent. The activity increased about 2-fold in spleen extracts with endotoxin (bacterial lipopolysaccharide) treatment of animals, suggesting that the activity is inducible or regulatable. Other nitrotyrosine-containing proteins also served as substrates, while free nitrotyrosine and some endogenous nitrotyrosine-containing proteins in tissue extracts were poor substrates. Although the product and possible cofactors for this reaction have not yet been identified, this activity may be a “nitrotyrosine denitrase” that reverses protein nitration and, thus, decreases peroxynitrite toxicity. This activity was not observed in homogenates from rat liver or kidney, suggesting that there may also be some tissue specificity for the apparent denitrase activity. nitric oxide/peroxynitrite/protein nitration/denitrase Homogenates from rat spleen and lung could modify nitrotyrosine-containing BSA. With incubation, nitrotyrosine-containing BSA lost its epitope to a monoclonal antibody that selectively recognized nitrotyrosine-containing proteins. In the presence of protease inhibitors, the loss of the nitrotyrosine epitope occurred without protein degradation and hydrolysis. This activity was found in supernatant but not particulate fractions of spleen homogenates. The factor was heat labile, was sensitive to trypsin treatment, and was retained after passage through a membrane with a 10-kDa retention. The activity was time- and protein-concentration dependent. The activity increased about 2-fold in spleen extracts with endotoxin (bacterial lipopolysaccharide) treatment of animals, suggesting that the activity is inducible or regulatable. Other nitrotyrosine-containing proteins also served as substrates, while free nitrotyrosine and some endogenous nitrotyrosine-containing proteins in tissue extracts were poor substrates. Although the product and possible cofactors for this reaction have not yet been identified, this activity may be a “nitrotyrosine denitrase” that reverses protein nitration and, thus, decreases peroxynitrite toxicity. This activity was not observed in homogenates from rat liver or kidney, suggesting that there may also be some tissue specificity for the apparent denitrase activity. |
Author | Behbod, Fariba Martin, Emil Wada, Kouichirou Davis, Karen Kamisaki, Yoshinori Balabanli, Barbaros Bian, Ka Lee, Yu-Chen Murad, Ferid |
AuthorAffiliation | Department of Integrative Biology and Pharmacology, University of Texas–Houston Medical School, 6431 Fannin, Houston, TX 77030 |
AuthorAffiliation_xml | – name: Department of Integrative Biology and Pharmacology, University of Texas–Houston Medical School, 6431 Fannin, Houston, TX 77030 |
Author_xml | – sequence: 1 givenname: Yoshinori surname: Kamisaki fullname: Kamisaki, Yoshinori – sequence: 2 givenname: Kouichirou surname: Wada fullname: Wada, Kouichirou – sequence: 3 givenname: Ka surname: Bian fullname: Bian, Ka – sequence: 4 givenname: Barbaros surname: Balabanli fullname: Balabanli, Barbaros – sequence: 5 givenname: Karen surname: Davis fullname: Davis, Karen – sequence: 6 givenname: Emil surname: Martin fullname: Martin, Emil – sequence: 7 givenname: Fariba surname: Behbod fullname: Behbod, Fariba – sequence: 8 givenname: Yu-Chen surname: Lee fullname: Lee, Yu-Chen – sequence: 9 givenname: Ferid surname: Murad fullname: Murad, Ferid |
BackLink | https://www.ncbi.nlm.nih.gov/pubmed/9751709$$D View this record in MEDLINE/PubMed |
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References | e_1_3_2_9_2 e_1_3_2_15_2 e_1_3_2_8_2 e_1_3_2_16_2 e_1_3_2_7_2 e_1_3_2_17_2 e_1_3_2_18_2 e_1_3_2_19_2 Murad F (e_1_3_2_3_2) 1978; 9 e_1_3_2_20_2 Katsuki S (e_1_3_2_1_2) 1977; 3 e_1_3_2_10_2 e_1_3_2_21_2 e_1_3_2_5_2 e_1_3_2_11_2 e_1_3_2_22_2 e_1_3_2_12_2 e_1_3_2_23_2 e_1_3_2_13_2 e_1_3_2_2_2 e_1_3_2_14_2 Murad F (e_1_3_2_6_2) 1998; 53 Ignarro L (e_1_3_2_4_2) 1995 |
References_xml | – ident: e_1_3_2_9_2 doi: 10.1515/bchm3.1994.375.2.81 – volume: 9 start-page: 145 year: 1978 ident: e_1_3_2_3_2 publication-title: Adv Cyclic Nucleotide Res contributor: fullname: Murad F – start-page: 1 volume-title: Advances in Pharmacology year: 1995 ident: e_1_3_2_4_2 contributor: fullname: Ignarro L – ident: e_1_3_2_23_2 doi: 10.1038/227680a0 – volume: 3 start-page: 23 year: 1977 ident: e_1_3_2_1_2 publication-title: J Cyclic Nucleotide Res contributor: fullname: Katsuki S – ident: e_1_3_2_18_2 doi: 10.1016/S0021-9258(19)39084-2 – ident: e_1_3_2_21_2 doi: 10.1006/abio.1997.2281 – ident: e_1_3_2_19_2 doi: 10.1016/0003-2697(76)90527-3 – ident: e_1_3_2_5_2 doi: 10.1001/jama.1996.03540140077033 – ident: e_1_3_2_14_2 doi: 10.1016/S0021-9258(18)43894-X – ident: e_1_3_2_22_2 doi: 10.1006/abbi.1997.0114 – ident: e_1_3_2_7_2 doi: 10.1073/pnas.87.4.1620 – ident: e_1_3_2_20_2 doi: 10.1016/S0076-6879(96)69020-X – ident: e_1_3_2_10_2 doi: 10.1016/0014-5793(94)00722-5 – ident: e_1_3_2_11_2 doi: 10.1038/364584a0 – ident: e_1_3_2_13_2 doi: 10.1073/pnas.92.26.12041 – ident: e_1_3_2_17_2 doi: 10.1073/pnas.93.8.3377 – ident: e_1_3_2_15_2 doi: 10.1073/pnas.93.5.1776 – volume: 53 start-page: 43 year: 1998 ident: e_1_3_2_6_2 publication-title: Rec Prog Horm Res contributor: fullname: Murad F – ident: e_1_3_2_16_2 doi: 10.1016/0014-5793(96)00347-X – ident: e_1_3_2_12_2 doi: 10.1038/34923 – ident: e_1_3_2_2_2 doi: 10.1073/pnas.74.8.3203 – ident: e_1_3_2_8_2 doi: 10.1016/0003-9861(92)90432-V |
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Snippet | Homogenates from rat spleen and lung could modify nitrotyrosine-containing BSA. With incubation, nitrotyrosine-containing BSA lost its epitope to a monoclonal... Homogenates from rat spleen and lung could modify nitrotyrosine-containing BSA. With incubation, nitrotyrosine-containing BSA lost its epitope to a monoclonal... |
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SubjectTerms | Animals Antibodies Biochemistry Biological Sciences Cattle Endotoxins Epitopes In Vitro Techniques Kidneys Lipopolysaccharides - pharmacology Liver Lungs Male Nitration Oxides Protein Processing, Post-Translational Proteins Proteins - chemistry Proteins - metabolism Rats Rats, Sprague-Dawley Rodents Serum Albumin, Bovine - chemistry Serum Albumin, Bovine - metabolism Spleen Spleen - drug effects Spleen - enzymology Substrate Specificity Tyrosine - analogs & derivatives Tyrosine - chemistry Tyrosine - metabolism |
Title | An Activity in Rat Tissues That Modifies Nitrotyrosine-Containing Proteins |
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