Your search keyword '"Plakas SM"' showing total 2 results

1. Biomarkers of brevetoxin exposure and composite toxin levels in hard clam (Mercenaria sp.) exposed to Karenia brevis blooms.

Author

Abraham A, El Said KR, Wang Y, Jester EL, Plakas SM, Flewelling LJ, Henry MS, and Pierce RH

Subjects

Animals, Biological Assay, Bivalvia drug effects, Chromatography, Liquid, Enzyme-Linked Immunosorbent Assay, Florida, Marine Toxins analysis, Mass Spectrometry, Mice, Molecular Structure, Oxocins analysis, Time Factors, Biomarkers metabolism, Bivalvia metabolism, Dinoflagellida chemistry, Environmental Exposure, Harmful Algal Bloom, Marine Toxins toxicity, Oxocins toxicity

Abstract

Brevetoxins in clams (Mercenaria sp.) exposed to recurring blooms of Karenia brevis in Sarasota Bay, FL, were studied over a three-year period. Brevetoxin profiles in toxic clams were generated by ELISA and LC-MS. Several brevetoxin metabolites, as identified by LC-MS, were major contributors to the composite brevetoxin response of ELISA. These were S-desoxyBTX-B2 (m/z 1018), BTX-B2 (m/z 1034), BTX-B5 (m/z 911), open A-ring BTX-B5 (m/z 929), and BTX-B1 (m/z 1018). Summed values of these metabolites were highly correlated (R(2) = 0.9) with composite B-type brevetoxin measurements by ELISA. S-desoxyBTX-B2, BTX-B2, and BTX-B1 were the most persistent and detectable in shellfish for several months after dissipation of blooms. These metabolites were selected as LC-MS biomarkers of brevetoxin exposure and reflective of composite B-type brevetoxins in hard clam. ELISA and LC-MS values were moderately correlated with toxicity of the shellfish by mouse bioassay. ELISA and LC-MS methods offer rapid screening and confirmatory determination of brevetoxins, respectively, as well as toxicity assessment in clams exposed to K. brevis blooms., (Published by Elsevier Ltd.)

Published

2015

2. LC/MS analysis of brevetoxin metabolites in the Eastern oyster (Crassostrea virginica).

Author

Wang Z, Plakas SM, El Said KR, Jester EL, Granade HR, and Dickey RW

Subjects

Animals, Biological Assay, Chromatography, Liquid, Cytotoxicity Tests, Immunologic, Dinoflagellida, Florida, Hydrolysis, Mass Spectrometry, Oxidation-Reduction, Texas, Amino Acids metabolism, Fatty Acids metabolism, Marine Toxins chemistry, Marine Toxins metabolism, Ostreidae metabolism, Oxocins chemistry, Oxocins metabolism

Abstract

Brevetoxin (PbTx) metabolism was examined in the Eastern oyster (Crassostrea virginica) following exposure to a Karenia brevis red tide, by using LC/MS(/MS) and cytotoxicity assay. Metabolites observed in field-exposed oysters were confirmed in oysters exposed to K. brevis cultures in the laboratory. Previously, we identified a cysteine conjugate and its sulfoxide (MH(+): m/z 1018 and 1034) as metabolites of the brevetoxin congener PbTx-2. In the present study, we found a cysteine conjugate and its sulfoxide with A-type brevetoxin backbone structure (MH(+): m/z 990 and 1006), as probable derivatives of PbTx-1. We also found glycine-cysteine-PbTx (m/z 1047 and 1075), gamma-glutamyl-cysteine-PbTx (m/z 1147), and glutathione-PbTx (m/z 1176 and 1204) conjugates with A- and B-type backbone structures. Amino acid-PbTx conjugates react with fatty acids through amide linkage to form a series of fatty acid-amino acid-PbTx conjugates. These fatty acid conjugates are major contributors to the composite cytototoxic responses obtained in extracts of brevetoxin-contaminated oysters. Other brevetoxin derivatives found in oysters are consistent with hydrolytic ring-opening and oxidation/reduction reactions.

Published

2004