Nitro-fatty acid metabolome: saturation, desaturation, beta-oxidation, and protein adduction

Volker Rudolph; Francisco J Schopfer; Nicholas K H Khoo; Tanja K Rudolph; Marsha P Cole; Steven R Woodcock; Gustavo Bonacci; Alison L Groeger; Franca Golin-Bisello; Chen-Shan Chen; Paul R S Baker; Bruce A Freeman

doi:10.1074/jbc.M802298200

Nitro-fatty acid metabolome: saturation, desaturation, beta-oxidation, and protein adduction

Standard

Nitro-fatty acid metabolome: saturation, desaturation, beta-oxidation, and protein adduction. / Rudolph, Volker; Schopfer, Francisco J; Khoo, Nicholas K H; Rudolph, Tanja K; Cole, Marsha P; Woodcock, Steven R; Bonacci, Gustavo; Groeger, Alison L; Golin-Bisello, Franca; Chen, Chen-Shan; Baker, Paul R S; Freeman, Bruce A.

In: J BIOL CHEM, Vol. 284, No. 3, 16.01.2009, p. 1461-1473.

Research output: SCORING: Contribution to journal › SCORING: Journal article › Research › peer-review

Harvard

Rudolph, V, Schopfer, FJ, Khoo, NKH, Rudolph, TK, Cole, MP, Woodcock, SR, Bonacci, G, Groeger, AL, Golin-Bisello, F, Chen, C-S, Baker, PRS & Freeman, BA 2009, 'Nitro-fatty acid metabolome: saturation, desaturation, beta-oxidation, and protein adduction', J BIOL CHEM, vol. 284, no. 3, pp. 1461-1473. https://doi.org/10.1074/jbc.M802298200

APA

Rudolph, V., Schopfer, F. J., Khoo, N. K. H., Rudolph, T. K., Cole, M. P., Woodcock, S. R., Bonacci, G., Groeger, A. L., Golin-Bisello, F., Chen, C-S., Baker, P. R. S., & Freeman, B. A. (2009). Nitro-fatty acid metabolome: saturation, desaturation, beta-oxidation, and protein adduction. J BIOL CHEM, 284(3), 1461-1473. https://doi.org/10.1074/jbc.M802298200

Vancouver

Rudolph V, Schopfer FJ, Khoo NKH, Rudolph TK, Cole MP, Woodcock SR et al. Nitro-fatty acid metabolome: saturation, desaturation, beta-oxidation, and protein adduction. J BIOL CHEM. 2009 Jan 16;284(3):1461-1473. https://doi.org/10.1074/jbc.M802298200

Bibtex

@article{f851c366f8014458828487d574adb567,

title = "Nitro-fatty acid metabolome: saturation, desaturation, beta-oxidation, and protein adduction",

abstract = "Nitrated derivatives of fatty acids (NO2-FA) are pluripotent cell-signaling mediators that display anti-inflammatory properties. Current understanding of NO2-FA signal transduction lacks insight into how or if NO2-FA are modified or metabolized upon formation or administration in vivo. Here the disposition and metabolism of nitro-9-cis-octadecenoic (18:1-NO2) acid was investigated in plasma and liver after intravenous injection in mice. High performance liquid chromatography-tandem mass spectrometry analysis showed that no 18:1-NO2 or metabolites were detected under basal conditions, whereas administered 18:1-NO2 is rapidly adducted to plasma thiol-containing proteins and glutathione. NO2-FA are also metabolized via beta-oxidation, with high performance liquid chromatography-tandem mass spectrometry analysis of liver lipid extracts of treated mice revealing nitro-7-cis-hexadecenoic acid, nitro-5-cis-tetradecenoic acid, and nitro-3-cis-dodecenoic acid and corresponding coenzyme A derivatives of 18:1-NO2 as metabolites. Additionally, a significant proportion of 18:1-NO2 and its metabolites are converted to nitroalkane derivatives by saturation of the double bond, and to a lesser extent are desaturated to diene derivatives. There was no evidence of the formation of nitrohydroxyl or conjugated ketone derivatives in organs of interest, metabolites expected upon 18:1-NO2 hydration or nitric oxide (*NO) release. Plasma samples from treated mice had significant extents of protein-adducted 18:1-NO2 detected by exchange to added beta-mercaptoethanol. This, coupled with the observation of 18:1-NO2 release from glutathione-18:1-NO2 adducts, supports that reversible and exchangeable NO2-FA-thiol adducts occur under biological conditions. After administration of [3H]18:1-NO2, 64% of net radiolabel was recovered 90 min later in plasma (0.2%), liver (18%), kidney (2%), adipose tissue (2%), muscle (31%), urine (6%), and other tissue compartments, and may include metabolites not yet identified. In aggregate, these findings show that electrophilic FA nitroalkene derivatives (a) acquire an extended half-life by undergoing reversible and exchangeable electrophilic reactions with nucleophilic targets and (b) are metabolized predominantly via saturation of the double bond and beta-oxidation reactions that terminate at the site of acyl-chain nitration.",

keywords = "Animals, Fatty Acids/metabolism, Glutathione/metabolism, Humans, Liver/metabolism, Mice, Nitro Compounds/metabolism, Organ Specificity/drug effects, Oxidation-Reduction/drug effects, Plasma/metabolism, Proteins/metabolism, Signal Transduction/drug effects",

author = "Volker Rudolph and Schopfer, {Francisco J} and Khoo, {Nicholas K H} and Rudolph, {Tanja K} and Cole, {Marsha P} and Woodcock, {Steven R} and Gustavo Bonacci and Groeger, {Alison L} and Franca Golin-Bisello and Chen-Shan Chen and Baker, {Paul R S} and Freeman, {Bruce A}",

year = "2009",

month = jan,

day = "16",

doi = "10.1074/jbc.M802298200",

language = "English",

volume = "284",

pages = "1461--1473",

journal = "J BIOL CHEM",

issn = "0021-9258",

publisher = "American Society for Biochemistry and Molecular Biology Inc.",

number = "3",

}

RIS

TY - JOUR

T1 - Nitro-fatty acid metabolome: saturation, desaturation, beta-oxidation, and protein adduction

AU - Rudolph, Volker

AU - Schopfer, Francisco J

AU - Khoo, Nicholas K H

AU - Rudolph, Tanja K

AU - Cole, Marsha P

AU - Woodcock, Steven R

AU - Bonacci, Gustavo

AU - Groeger, Alison L

AU - Golin-Bisello, Franca

AU - Chen, Chen-Shan

AU - Baker, Paul R S

AU - Freeman, Bruce A

PY - 2009/1/16

Y1 - 2009/1/16

N2 - Nitrated derivatives of fatty acids (NO2-FA) are pluripotent cell-signaling mediators that display anti-inflammatory properties. Current understanding of NO2-FA signal transduction lacks insight into how or if NO2-FA are modified or metabolized upon formation or administration in vivo. Here the disposition and metabolism of nitro-9-cis-octadecenoic (18:1-NO2) acid was investigated in plasma and liver after intravenous injection in mice. High performance liquid chromatography-tandem mass spectrometry analysis showed that no 18:1-NO2 or metabolites were detected under basal conditions, whereas administered 18:1-NO2 is rapidly adducted to plasma thiol-containing proteins and glutathione. NO2-FA are also metabolized via beta-oxidation, with high performance liquid chromatography-tandem mass spectrometry analysis of liver lipid extracts of treated mice revealing nitro-7-cis-hexadecenoic acid, nitro-5-cis-tetradecenoic acid, and nitro-3-cis-dodecenoic acid and corresponding coenzyme A derivatives of 18:1-NO2 as metabolites. Additionally, a significant proportion of 18:1-NO2 and its metabolites are converted to nitroalkane derivatives by saturation of the double bond, and to a lesser extent are desaturated to diene derivatives. There was no evidence of the formation of nitrohydroxyl or conjugated ketone derivatives in organs of interest, metabolites expected upon 18:1-NO2 hydration or nitric oxide (*NO) release. Plasma samples from treated mice had significant extents of protein-adducted 18:1-NO2 detected by exchange to added beta-mercaptoethanol. This, coupled with the observation of 18:1-NO2 release from glutathione-18:1-NO2 adducts, supports that reversible and exchangeable NO2-FA-thiol adducts occur under biological conditions. After administration of [3H]18:1-NO2, 64% of net radiolabel was recovered 90 min later in plasma (0.2%), liver (18%), kidney (2%), adipose tissue (2%), muscle (31%), urine (6%), and other tissue compartments, and may include metabolites not yet identified. In aggregate, these findings show that electrophilic FA nitroalkene derivatives (a) acquire an extended half-life by undergoing reversible and exchangeable electrophilic reactions with nucleophilic targets and (b) are metabolized predominantly via saturation of the double bond and beta-oxidation reactions that terminate at the site of acyl-chain nitration.

AB - Nitrated derivatives of fatty acids (NO2-FA) are pluripotent cell-signaling mediators that display anti-inflammatory properties. Current understanding of NO2-FA signal transduction lacks insight into how or if NO2-FA are modified or metabolized upon formation or administration in vivo. Here the disposition and metabolism of nitro-9-cis-octadecenoic (18:1-NO2) acid was investigated in plasma and liver after intravenous injection in mice. High performance liquid chromatography-tandem mass spectrometry analysis showed that no 18:1-NO2 or metabolites were detected under basal conditions, whereas administered 18:1-NO2 is rapidly adducted to plasma thiol-containing proteins and glutathione. NO2-FA are also metabolized via beta-oxidation, with high performance liquid chromatography-tandem mass spectrometry analysis of liver lipid extracts of treated mice revealing nitro-7-cis-hexadecenoic acid, nitro-5-cis-tetradecenoic acid, and nitro-3-cis-dodecenoic acid and corresponding coenzyme A derivatives of 18:1-NO2 as metabolites. Additionally, a significant proportion of 18:1-NO2 and its metabolites are converted to nitroalkane derivatives by saturation of the double bond, and to a lesser extent are desaturated to diene derivatives. There was no evidence of the formation of nitrohydroxyl or conjugated ketone derivatives in organs of interest, metabolites expected upon 18:1-NO2 hydration or nitric oxide (*NO) release. Plasma samples from treated mice had significant extents of protein-adducted 18:1-NO2 detected by exchange to added beta-mercaptoethanol. This, coupled with the observation of 18:1-NO2 release from glutathione-18:1-NO2 adducts, supports that reversible and exchangeable NO2-FA-thiol adducts occur under biological conditions. After administration of [3H]18:1-NO2, 64% of net radiolabel was recovered 90 min later in plasma (0.2%), liver (18%), kidney (2%), adipose tissue (2%), muscle (31%), urine (6%), and other tissue compartments, and may include metabolites not yet identified. In aggregate, these findings show that electrophilic FA nitroalkene derivatives (a) acquire an extended half-life by undergoing reversible and exchangeable electrophilic reactions with nucleophilic targets and (b) are metabolized predominantly via saturation of the double bond and beta-oxidation reactions that terminate at the site of acyl-chain nitration.

KW - Animals

KW - Fatty Acids/metabolism

KW - Glutathione/metabolism

KW - Humans

KW - Liver/metabolism

KW - Mice

KW - Nitro Compounds/metabolism

KW - Organ Specificity/drug effects

KW - Oxidation-Reduction/drug effects

KW - Plasma/metabolism

KW - Proteins/metabolism

KW - Signal Transduction/drug effects

U2 - 10.1074/jbc.M802298200

DO - 10.1074/jbc.M802298200

M3 - SCORING: Journal article

C2 - 19015269

VL - 284

SP - 1461

EP - 1473

JO - J BIOL CHEM

JF - J BIOL CHEM

SN - 0021-9258

IS - 3

ER -