Abstract
We developed a sensitive method to quantitate the tyrosine metabolites maleylacetone (MA) and succinylacetone (SA) and the tyrosine metabolism inhibitor dichloroacetate (DCA) in biological specimens. Accumulation of these metabolites may be responsible for the toxicity observed when exposed to DCA. Detection limits of previous methods are 200 ng/mL (1.2 pmol/microL) (MA) and 2.6 microg/mL (16.5 pmol/microL) (SA) but the metabolites are likely present in lower levels in biological specimens. To increase sensitivity, analytes were extracted from liver, urine, plasma and cultured nerve cells before and after dosing with DCA, derivatized to their pentafluorobenzyl esters, and analyzed via GC-MS/MS.
Publication types
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Research Support, N.I.H., Extramural
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Validation Study
MeSH terms
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Acetone / analogs & derivatives*
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Acetone / blood
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Acetone / metabolism
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Acetone / urine
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Animals
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Blotting, Western
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Dichloroacetic Acid / blood
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Dichloroacetic Acid / metabolism*
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Dichloroacetic Acid / urine
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Gas Chromatography-Mass Spectrometry / methods*
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Heptanoates / blood
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Heptanoates / metabolism*
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Heptanoates / urine
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Humans
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Liver / metabolism
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Male
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Maleates / blood
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Maleates / metabolism*
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Maleates / urine
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Rats
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Sensitivity and Specificity
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Tyrosine / antagonists & inhibitors
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Tyrosine / blood
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Tyrosine / metabolism*
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Tyrosine / urine
Substances
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Heptanoates
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Maleates
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maleylacetone
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Acetone
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Tyrosine
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succinylacetone
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Dichloroacetic Acid