Detection and characterization of twenty‐eight isomers of fumonisin B1 (FB1) mycotoxin in a solid rice culture infected with Fusarium verticillioides by reversed‐phase high‐performance liquid chromatography/electrospray ionization time‐of‐flight and ion trap mass spectrometry

Fumonisin mycotoxins which are hazardous to humans and animals were produced in a Fusarium verticillioides‐infected solid rice culture. To decrease the possibility of the formation of artifacts, the fumonisins were analysed by reversed‐phase high‐performance liquid chromatography/electrospray ionization time‐of‐flight (RP‐HPLC/ESI‐TOFMS) and ion trap mass spectrometry (RP‐HPLC/ESI‐ITMS) immediately after the extraction of the culture material, without any further sample clean‐up. The fumonisin isomers were separated by using a flat gradient on a special, high‐coverage C₁₈, narrow‐bore HPLC column (YMC‐Pack J'sphere ODS H80) suggested for the separation of structural isomers by the manufacturer. Exact mass measurements (TOFMS) of the protonated molecules and extraction of the ion chromatogram corresponding to the empirical formula (C₃₄H₅₉NO₁₅) of FB₁ toxins led to the identification of 29 peaks and shoulders, including those of FB₁. The FB₁ toxin and 28 of its isomers were also detected by ITMS after separation with RP‐HPLC. The characteristic m/z values of the product ions, including the backbones obtained by ITMS², undoubtedly indicated the structures of the FB₁ isomers for 28 peaks and shoulders. In the MS² spectra of the protonated molecules of the FB₁ isomers, with some exceptions, 15 characteristic product ions including the hydrocarbon backbone at m/z 299 were observed. The abundance ratio of the cation at m/z 299 ranged up to 5.8%. The relative quantities of the isomers found in the sample extract were expressed as percentages of the FB₁ content (0.001–0.579%). The total amount of the 28 FB₁ isomers was 2.803% of the quantity of FB₁ that is important from the aspect of food and feed safety. Copyright © 2009 John Wiley & Sons, Ltd.