High performance liquid chromatographic quantitation of aflatoxin metabolites in animal tissues.

A previously reported reverse phase high performance liquid chromatographic (HPLC) procedure was modified to permit the determination of the parent aflatoxins and various free and conjugated metabolites in animal tissues. The modified procedure was based on HPLC analysis of duplicate portions of a sample extract which had been prepared with and without treatment with trifluoroacetic acid (TFA). TFA catalyzes the conversion of aflatoxins G1, B1, M1, and Q1 to the fluorescent derivatives G2a, B2a, M2a, and Q2a. Aflatoxicol, which exhibited a sharp fluorescent peak in its native state, eluted as a tailing peak with weaker fluorescence following TFA treatment. Acid hydrolysis of the aqueous phase of tissue samples permitted the analysis of water-soluble conjugated forms of the various aflatoxins. Analysis of fluorescence spectra of manually collected HPLC fractions qualitatively supported the accuracy of the method. Representative data on the distribution of aflatoxins in turkey liver following ingestion of an experimentally contaminated ration are presented.