Development of an LC-MS/MS method for the determination of endogenous cortisol in hair using (13)C3-labeled cortisol as surrogate analyte

Tina M Binz; Ueli Braun; Markus R Baumgartner; Thomas Kraemer

doi:10.1016/j.jchromb.2016.07.041

Development of an LC-MS/MS method for the determination of endogenous cortisol in hair using (13)C3-labeled cortisol as surrogate analyte

J Chromatogr B Analyt Technol Biomed Life Sci. 2016 Oct 15:1033-1034:65-72. doi: 10.1016/j.jchromb.2016.07.041. Epub 2016 Jul 22.

Authors

Tina M Binz¹, Ueli Braun², Markus R Baumgartner³, Thomas Kraemer⁴

Affiliations

¹ University of Zurich, Zurich Institute of Forensic Medicine, Center for Forensic Hair Analytics, Zurich, Switzerland. Electronic address: TinaMaria.Binz@irm.uzh.ch.
² University of Zurich, Vetsuisse Faculty, Department of Farm Animals, Clinic of Ruminants, Zurich, Switzerland.
³ University of Zurich, Zurich Institute of Forensic Medicine, Center for Forensic Hair Analytics, Zurich, Switzerland.
⁴ University of Zurich, Zurich Institute of Forensic Medicine, Forensic Pharmacology and Toxicology, Zurich, Switzerland.

PMID: 27522172
DOI: 10.1016/j.jchromb.2016.07.041

Abstract

Hair cortisol levels are increasingly applied as a measure for stress in humans and mammals. Cortisol is an endogenous compound and is always present within the hair matrix. Therefore, "cortisol-free hair matrix" is a critical point for any analytical method to accurately quantify especially low cortisol levels. The aim of this project was to modify current methods used for hair cortisol analysis to more accurately determine low endogenous cortisol concentrations in hair. For that purpose, (13)C3-labeled cortisol, which is not naturally present in hair (above 13C natural abundance levels), was used for calibration and comparative validation applying cortisol versus (13)C3-labeled cortisol. Cortisol was extracted from 20mg hair (standard sample amount) applying an optimized single step extraction protocol. An LC-MS/MS method was developed for the quantitative analysis of cortisol using either cortisol or (13)C3-cortisol as calibrators and D7-cortisone as internal standard (IS). The two methods (cortisol/(13)C3-labeled cortisol) were validated in a concentration range up to 500pg/mg and showed good linearity for both analytes (cortisol: R(2)=0.9995; (13)C3-cortisol R(2)=0.9992). Slight differences were observed for limit of detection (LOD) (0.2pg/mg/0.1pg/mg) and limit of quantification (LOQ) (1pg/mg/0.5pg/mg). Precision was good with a maximum deviation of 8.8% and 10% for cortisol and (13)C3-cortisol respectively. Accuracy and matrix effects were good for both analytes except for the quality control (QC) low cortisol. QC low (2.5pg/mg) showed matrix effects (126.5%, RSD 35.5%) and accuracy showed a deviation of 26% when using cortisol to spike. These effects are likely to be caused by the unknown amount of endogenous cortisol in the different hair samples used to determine validation parameters like matrix effect, LOQ and accuracy. No matrix effects were observed for the high QC (400pg/mg) samples. Recovery was good with 92.7%/87.3% (RSD 9.9%/6.2%) for QC low and 102.3%/82.1% (RSD 5.8%/11.4%) for QC high. After successful validation the applicability of the method could be proven. The study shows that the method is especially useful for determining low endogenous cortisol concentrations as they occur in cow hair for example.

Keywords: (13)C(3)-labeled cortisol; Endogenous cortisol; Hair; LC–MS/MS; Stress.

MeSH terms

Carbon Isotopes / analysis*
Chromatography, Liquid / methods*
Hair / chemistry*
Humans
Hydrocortisone / analysis*
Linear Models
Reproducibility of Results
Sensitivity and Specificity
Tandem Mass Spectrometry / methods*

Substances

Carbon Isotopes
Hydrocortisone