Specific screening method for dextran and hydroxyethyl starch in human urine by size exclusion chromatography–in-source collision-induced dissociation–time-of-flight mass spectrometry

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作者
Marjo Kolmonen
Antti Leinonen
Tiia Kuuranne
Anna Pelander
Koen Deventer
Ilkka Ojanperä
机构
[1] University of Helsinki,Hjelt Institute, Department of Forensic Medicine, Forensic Toxicology Division
[2] United Medix Laboratories Ltd.,Doping Control Laboratory
[3] Ghent University (UGent),Department of Clinical Chemistry, Microbiology and Immunology, Doping Control Laboratory (DoCoLab)
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Dextran; Hydroxyethyl starch; Screening; Size exclusion chromatography; Time-of-flight mass spectrometry;
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摘要
The use of plasma volume expanders (PVE), such as dextran (DEX) and hydroxyethyl starch (HES), is prohibited in sports. DEX is a naturally occurring glucose polymer, whereas HES is synthetically produced from amylopectin starch by substitution with hydroxyethyl groups. In doping control, the commonly applied enzymatic and colorimetric screening methods are lacking adequate specificity for DEX and HES. Also, gas chromatographic–mass spectrometic (GC-MS) screening methods have specificity issues with DEX. In addition, due to the nature of the target compounds, time-consuming derivatisation steps are required in GC-MS. Based on the high molecular weight of carbohydrate polymers excreted in urine after administration of DEX and HES, a screening method was developed involving size exclusion chromatography (SEC) combined with time-of-flight mass spectrometry (TOFMS). By using solely a SEC guard column as an analytical column allowed sufficient chromatographic resolution in a minimal amount of time and with reasonable repeatability (average RSD of 10%). Detector response was linear throughout the measurement range with R2 > 0.99 for both analytes. Limits of detection were 100 and 250 μg mL−1 for DEX and HES, respectively. Ion suppression was found to be 52% at maximum. In-source collision-induced dissociation (ISCID) was used to produce characteristic fragments at a mass accuracy better than 2 mDa. The specificity of the SEC–ISCID–TOFMS method was demonstrated with 120 PVE negative doping control samples analyzed in parallel with a routine GC-MS screening method. In addition, seven urine samples from diabetic athletes, causing interpretation problems in routine GC-MS, showed here a definitely negative profile.
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页码:563 / 571
页数:8
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