4.7 Article

Determination of Urinary Mycotoxin Biomarkers Using a Sensitive Online Solid Phase Extraction-UHPLC-MS/MS Method

Journal

TOXINS
Volume 13, Issue 6, Pages -

Publisher

MDPI
DOI: 10.3390/toxins13060418

Keywords

mycotoxin; biomonitoring; urine; online solid phase extraction; metabolite; HPLC-MS; MS

Funding

  1. Bill & Melinda Gates Foundation [OPP1021542, OPP1066264]
  2. United Kingdom Department for International Development (DFID/UKAID)
  3. Wellcome Trust [093768/Z/10/Z, 108065/Z/15/Z, 203905/Z/16/Z]
  4. Swiss Agency for Development and Cooperation
  5. US National Institutes of Health [2R01HD060338-06]
  6. UNICEF [PCA-2017-0002]

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Biomarker-based approaches are important tools in assessing human exposure to mycotoxins, and the online solid phase extraction-ultra high-performance liquid chromatography-tandem mass spectrometry method provides sensitive, robust, and rapid analysis of relevant mycotoxins and metabolites in human urine.
In the course of assessing the human exposure to mycotoxins, biomarker-based approaches have proven to be important tools. Low concentration levels, complex matrix compositions, structurally diverse analytes, and the large size of sample cohorts are the main challenges of analytical procedures. For that reason, an online solid phase extraction-ultra high-performance liquid chromatography-tandem mass spectrometry (online SPE-UHPLC-MS/MS) method was developed, allowing for the sensitive, robust, and rapid analysis of 11 relevant mycotoxins and mycotoxin metabolites in human urine. The included spectrum of analytes comprises aflatoxin M-1 (AFM(1)), altenuene (ALT), alternariol monomethyl ether (AME), alternariol (AOH), citrinin (CIT) and its metabolite dihydrocitrinone (DH-CIT), fumonisin B-1 (FB1), ochratoxin A (OTA), and zearalenone (ZEN) as well as alpha- and beta-zearalenol (alpha- and beta-ZEL). Reliable quantitation was achieved by means of stable isotope dilution, except for ALT, AME and AOH using matrix calibrations. The evaluation of method performance displayed low limits of detection in the range of pg/mL urine, satisfactory apparent recovery rates as well as high accuracy and precision during intra- and interday repeatability. Within the analysis of Zimbabwean urine samples (n = 50), the applicability of the newly developed method was shown. In addition to FB1 being quantifiable in all analyzed samples, six other mycotoxin biomarkers were detected. Compared to the occurrence rates obtained after analyzing the same sample set using an established dilute and shoot (DaS) approach, a considerably higher number of positive samples was observed when applying the online SPE method. Owing to the increased sensitivity, less need of sample handling, and low time effort, the herein presented online SPE approach provides a valuable contribution to human biomonitoring of mycotoxin exposure.

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