AI Article Synopsis

  • A new electrochemiluminescence-based immunoassay has been developed for detecting type-2 brevetoxins in oyster extracts, validated with known amounts of PbTx-3.
  • The assay can also analyze various sample types, including 100% acetone extracts and clinical samples like urine and serum, with minimal interference.
  • Key advantages include a short 2-hour analysis time, simplicity with only two additions and no wash steps, a low detection limit, and the use of a stable nonradioactive label, making it a promising tool for regulatory screening and pharmacokinetic studies.

Article Abstract

A new competitive electrochemiluminescence-based immunoassay for the type-2 brevetoxins in oyster extracts was developed. The assay was verified by spiking known amounts of PbTx-3 into 80% methanol extracts of Gulf Coast oysters. We also provide preliminary data demonstrating that 100% acetone extracts, aqueous homogenates, and the clinical matrixes urine and serum can also be analyzed without significant matrix interferences. The assay offers the advantages of speed ( 2 h analysis time); simplicity (only 2 additions, one incubation period, and no wash steps before analysis); low limit of quantitation (conservatively, 50 pg/mL = 1 ng/g tissue equivalents); and a stable, nonradioactive label. Due to the variety of brevetoxin metabolites present and the lack of certified reference standards for liquid chromatography-mass spectrometry confirmation, a true validation of brevetoxins in shellfish extracts is not possible at this time. However, our assay correlated well with another brevetoxin immunoassay currently in use in the United States. We believe this assay could be useful as a regulatory screening tool and could support pharmacokinetic studies in animals and clinical evaluation of neurotoxic shellfish poisoning victims.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC2844730PMC

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