Analysis of methyloxime derivatives of intact esters of testosterone and boldenone in equine plasma using ultra high performance liquid chromatography tandem mass spectrometry

Analysis of methyloxime derivatives of intact esters of testosterone and boldenone in equine plasma using ultra high performance liquid chromatography tandem mass spectrometry

Analysis of equine plasma samples to detect the abuse of anabolic steroids can be complicated when the parent steroid is endogenous to the animal. Anabolic steroids are usually administered intramuscularly as synthetic esters and therefore detection of the exogenous esters provides unequivocal proof...

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Bibliographic Details
Published in:Drug testing and analysis Vol. 3; no. 4; pp. 206 - 213
Main Authors: Gray, Bobby P., Teale, Phil, Pearce, Clive M.
Format: Journal Article
Language:English
Published: Chichester, UK John Wiley & Sons, Ltd 01-04-2011
Subjects:
Anabolic Agents - administration & dosage
Anabolic Agents - blood
Animals
Chromatography, High Pressure Liquid - methods
Chromatography, High Pressure Liquid - standards
Doping in Sports - prevention & control
equine
Esters
Horses - blood
Injections, Intramuscular
methyloxime
Oximes - blood
plasma
Reproducibility of Results
steroids
Tandem Mass Spectrometry - methods
Tandem Mass Spectrometry - standards
Testosterone - administration & dosage
Testosterone - analogs & derivatives
Testosterone - blood
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Summary:Analysis of equine plasma samples to detect the abuse of anabolic steroids can be complicated when the parent steroid is endogenous to the animal. Anabolic steroids are usually administered intramuscularly as synthetic esters and therefore detection of the exogenous esters provides unequivocal proof of illegal administration. An ultra high performance liquid chromatography tandem mass spectrometric (UPLC‐MSMS) method for the analysis of esters of testosterone (propionate, phenylpropionate, isocaproate, and decanoate) and boldenone (undecylenate) in equine plasma has been developed. Esters were extracted from equine plasma using a mixture of hexane and ethyl acetate and treated with methoxyamine hydrochloride to form methyloxime derivatives. Metenolone enanthate was used as an internal standard. After chromatographic separation, the derivatized steroid esters were quantified using selected reaction monitoring (SRM). The limit of detection for all of the steroid esters, based on a signal to noise ratio (S/N) of 3:1, was 1–3 pg/mL. The lower limit of quantification (LLOQ) for the all of the steroid esters was 5 pg/mL when 2 mL of plasma was extracted. Recovery of the steroid esters was 85–97% for all esters except for testosterone decanoate which was recovered at 62%. The intra‐day coefficient of variation (CV) for the analysis of plasma quality control (QC) samples was less than 9.2% at 40 pg/mL and less than 6.0% at 400 pg/mL. The developed assay was used to successfully confirm the presence of intact testosterone esters in equine plasma samples following intramuscular injection of Durateston® (mixed testosterone esters). Copyright © 2011 John Wiley & Sons, Ltd. Detection of intact steroid esters in doping control samples provides unequivocal proof of their exogenous nature. Results are presented from the validation of a method for the analysis of esters of testosterone and boldenone in equine plasma. The developed assay was used to successfully confirm the presence of intact testosterone esters in equine plasma samples following intramuscular injection of Durateston® (mixed testosterone esters).
Bibliography:ArticleID:DTA237
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ObjectType-Article-1
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content type line 23
ISSN:1942-7603
1942-7611
DOI:10.1002/dta.237