Testosterone Measurement by Isotope-Dilution Liquid Chromatography–Tandem Mass Spectrometry: Validation of a Method for Routine Clinical Practice

Author:

Cawood Marion L1,Field Helen P1,Ford Clive G1,Gillingwater Scott2,Kicman Andrew3,Cowan David3,Barth Julian H1

Affiliation:

1. SAS Centre for Steroid Hormones (Leeds), Department of Clinical Biochemistry & Immunology, Leeds General Infirmary, Leeds, United Kingdom

2. Waters Corporation, Manchester, United Kingdom

3. Drug Control Centre, King’s College, London, United Kingdom

Abstract

Abstract Background: Immunoassay is unsatisfactory for measuring the testosterone concentrations typically found in women. Bench-top tandem mass spectrometers are a viable alternative technology for measurements in the clinical laboratory. Methods: We used stable-isotope dilution liquid chromatography–tandem mass spectrometry (ID/LC-MS/MS) to measure testosterone in plasma and serum. The sample volume was 50 μL in duplicate; preparation and analysis were carried out in a single tube, and a batch of 192 tubes was analyzed in 17.5 h. Results: Intra- and interassay imprecision was <15% in the range 0.3–49 nmol/L. Recovery of testosterone added to samples at concentrations of 0.625–20 nmol/L was 96% (CV = 12%; n = 26). Six samples were serially diluted with double charcoal-stripped serum to demonstrate linearity. Correlation (r2) with isotope-dilution gas chromatography–mass spectrometry for 20 pools of clinical samples (range, 0.5–38.5 nmol/L) was 0.99. Correlations with our extraction RIA were 0.97 for clinical samples from men (range, 8–46.3 nmol/L) and 0.66 for samples from women (range, 0.7–3.0 nmol/L), but were 0.35 for male samples containing <3 nmol/L testosterone and 0.77 for female samples containing >8 nmol/L. Various steroids added to double charcoal-stripped serum showed no interference at the retention time of the testosterone peak. Conclusions: The ID/LC-MS/MS method has improved accuracy compared with immunoassay. The low sample volume and simplicity, rapidity, and robustness of the method make it suitable for use as a high-throughput assay in routine clinical biochemistry laboratories.

Publisher

Oxford University Press (OUP)

Subject

Biochemistry, medical,Clinical Biochemistry

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