Screening procedures for clenbuterol residue determination in bovine urine and liver matrices using enzyme-linked immunosorbent assay and liquid chromatography

The suitability of analytical protocols for simultaneous determination of clenbuterol (CL) by ELISA and liquid chromatography (LC) was investigated. Clenbuterol spiked bovine urine and liver samples were treated with aqueous and organic solutions followed by clean-up by solid phase extraction (SPE)....

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Bibliographic Details
Published in:Analytica chimica acta 2003-04, Vol.483 (1), p.61-67
Main Authors: Posyniak, Andrzej, Zmudzki, Jan, Niedzielska, Jolanta
Format: Article
Language:English
Subjects:
Analytical chemistry
Animal productions
Biological and medical sciences
Chemistry
Chromatographic methods and physical methods associated with chromatography
Clenbuterol
ELISA
Exact sciences and technology
Fundamental and applied biological sciences. Psychology
Liquid chromatography
Liver
Miscellaneous
Other chromatographic methods
Spectrometric and optical methods
Terrestrial animal productions
Urine
Vertebrates
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Summary:The suitability of analytical protocols for simultaneous determination of clenbuterol (CL) by ELISA and liquid chromatography (LC) was investigated. Clenbuterol spiked bovine urine and liver samples were treated with aqueous and organic solutions followed by clean-up by solid phase extraction (SPE). The determination of clenbuterol in prepared solutions was performed by a commercial ELISA test (R-Biofarm) and by LC with UV detection. The optimal conditions for liver were obtained when CL was isolated by a mixture of ethyl acetate–isopropanol (7:3 (v/v)) and purified by a mixed mode SPE column. However, additional purification with perchloric acid should be used to decrease the interference from matrices. For urine samples, the optimal conditions were obtained after dilution of the sample with borate buffer (pH 8.5), and clean-up by mixed mode SPE. The recoveries of CL were >80% from both matrices. The procedures were useful for clenbuterol screening by ELISA as well as by LC.
ISSN:0003-2670
1873-4324
DOI:10.1016/S0003-2670(02)01021-8