Preanalytical standardization for reactive oxygen species derived oxysterol analysis in human plasma by liquid chromatography-tandem mass spectrometry

C Helmschrodt; S Becker; J Thiery; U Ceglarek

doi:10.1016/j.bbrc.2013.12.087

Preanalytical standardization for reactive oxygen species derived oxysterol analysis in human plasma by liquid chromatography-tandem mass spectrometry

Biochem Biophys Res Commun. 2014 Apr 11;446(3):726-30. doi: 10.1016/j.bbrc.2013.12.087. Epub 2013 Dec 25.

Authors

C Helmschrodt¹, S Becker², J Thiery², U Ceglarek²

Affiliations

¹ Institute of Laboratory Medicine, Clinical Chemistry and Molecular Diagnostics, University Hospital Leipzig, Germany; LIFE - Leipzig Research Center for Civilization Diseases, Universität Leipzig, Germany. Electronic address: christin.helmschrodt@medizin.uni-leipzig.de.
² Institute of Laboratory Medicine, Clinical Chemistry and Molecular Diagnostics, University Hospital Leipzig, Germany; LIFE - Leipzig Research Center for Civilization Diseases, Universität Leipzig, Germany.

PMID: 24370823
DOI: 10.1016/j.bbrc.2013.12.087

Abstract

The analysis of the oxysterols 7-keto-, 7-α/β-hydroxy-, 5α,6α-epoxy-, 5β,6β-epoxycholesterol and cholestane-3β,5α,6β-triol derived from reactive oxygen species (ROS) is of interest as biomarkers in the field of atherosclerosis. Preanalytical validation is a crucial point to minimize the susceptibility of oxysterols to in vitro autoxidation. The aim of this study was to standardize a preanalytical protocol for ROS-derived oxysterol analysis by liquid chromatography-tandem mass spectrometry in human plasma. Sample matrices were compared and stability of free oxysterols in whole blood and EDTA-plasma was investigated with regard to short-term storage until sample preparation, freeze-thaw cycles, addition of butylated hydroxytoluene and long-term storage up to 1 year at different temperatures (-20 °C, -80 °C and -130 °C) as well as different storage containers (safe-lock tubes, cryo tubes and straws). Sample preparation prior LC-MS/MS analysis was reduced to a simple concentration and protein precipitation step. Storing EDTA-whole blood for 30 min at room temperature resulted in <25% concentration changes, within acceptable change limits (ACL). In freshly prepared plasma samples, free oxysterols were stable for 90 min stored at 4 °C with concentration changes <23.5% (within ACL). Up to nine freeze-thaw cycles did not affect analyte concentrations (concentration change -8.5% to +5.0%). 7-Ketocholesterol was stable for 2 years stored <-80 °C; concentration changes below 20.5% (within ACL). The remaining oxysterols were stored for a maximum of 2-4 weeks without exceeding ACL. The addition of BHT did not reveal improvement in analyte stability for storage at -80 or -130 °C. We developed a standardized preanalytical protocol for oxysterol analysis based on LC-MS/MS, compared cryobanking conditions for each oxysterol and present data for long-term storage up to 2 years.

Keywords: Biobanking condition; Butylated hydroxytoluene; Free oxysterol; Long-term storage; Preanalytical protocol; Reactive oxygen species.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Blood Specimen Collection / methods
Cholesterol / analogs & derivatives
Cholesterol / blood
Chromatography, Liquid / methods*
Chromatography, Liquid / standards
Cryopreservation / methods
Edetic Acid / chemistry
Humans
Hydroxycholesterols / blood*
Oxidation-Reduction
Plasma / chemistry
Reactive Oxygen Species / analysis
Reactive Oxygen Species / chemistry*
Reproducibility of Results
Sitosterols / chemistry
Tandem Mass Spectrometry / methods*
Tandem Mass Spectrometry / standards
Temperature
Time Factors

Substances

5,6-epoxycholesterol
7-ketositosterol
Hydroxycholesterols
Reactive Oxygen Species
Sitosterols
cholest-5-en-3 beta,7 alpha-diol
Cholesterol
Edetic Acid