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A competitive ELISA to detect brevetoxins from Karenia brevis (formerly Gymnodinium breve) in seawater, shellfish, and mammalian body fluid.

We developed a competitive enzyme-linked immunosorbent assay (ELISA) to analyze brevetoxins, using goat anti-brevetoxin antibodies obtained after immunization with keyhole limpet hemocyanin-brevetoxin conjugates, in combination with a three-step signal amplification process. The procedure, which use...

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Autores principales: Naar, Jerome, Bourdelais, Andrea, Tomas, Carmelo, Kubanek, Julia, Whitney, Philip L, Flewelling, Leanne, Steidinger, Karen, Lancaster, Johnny, Baden, Daniel G
Formato: Texto
Lenguaje:English
Publicado: 2002
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC1240733/
https://www.ncbi.nlm.nih.gov/pubmed/11836147
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author Naar, Jerome
Bourdelais, Andrea
Tomas, Carmelo
Kubanek, Julia
Whitney, Philip L
Flewelling, Leanne
Steidinger, Karen
Lancaster, Johnny
Baden, Daniel G
author_facet Naar, Jerome
Bourdelais, Andrea
Tomas, Carmelo
Kubanek, Julia
Whitney, Philip L
Flewelling, Leanne
Steidinger, Karen
Lancaster, Johnny
Baden, Daniel G
author_sort Naar, Jerome
collection PubMed
description We developed a competitive enzyme-linked immunosorbent assay (ELISA) to analyze brevetoxins, using goat anti-brevetoxin antibodies obtained after immunization with keyhole limpet hemocyanin-brevetoxin conjugates, in combination with a three-step signal amplification process. The procedure, which used secondary biotinylated antibodies, streptavidine-horseradish peroxidase conjugate, and chromogenic enzyme substrate, was useful in reducing nonspecific background signals commonly observed with complex matrices. This competitive ELISA detected brevetoxins in seawater, shellfish extract and homogenate, and mammalian body fluid such as urine and serum without pretreatment, dilution, or purification. We investigated the application of this technique for shellfish monitoring by spiking shellfish meat with brevetoxins and by analyzing oysters from two commercial shellfish beds in Florida that were exposed to a bloom of Karenia brevis (formerly Gymnodinium breve). We performed brevetoxin analysis of shellfish extracts and homogenates by ELISA and compared it with the mouse bioassay and receptor binding assay. The detection limit for brevetoxins in spiked oysters was 2.5 microg/100 g shellfish meat. This assay appears to be a useful tool for neurotoxic shellfish poisoning monitoring in shellfish and seawater, and for mammalian exposure diagnostics, and significantly reduces the time required for analyses.
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spelling pubmed-12407332005-11-08 A competitive ELISA to detect brevetoxins from Karenia brevis (formerly Gymnodinium breve) in seawater, shellfish, and mammalian body fluid. Naar, Jerome Bourdelais, Andrea Tomas, Carmelo Kubanek, Julia Whitney, Philip L Flewelling, Leanne Steidinger, Karen Lancaster, Johnny Baden, Daniel G Environ Health Perspect Research Article We developed a competitive enzyme-linked immunosorbent assay (ELISA) to analyze brevetoxins, using goat anti-brevetoxin antibodies obtained after immunization with keyhole limpet hemocyanin-brevetoxin conjugates, in combination with a three-step signal amplification process. The procedure, which used secondary biotinylated antibodies, streptavidine-horseradish peroxidase conjugate, and chromogenic enzyme substrate, was useful in reducing nonspecific background signals commonly observed with complex matrices. This competitive ELISA detected brevetoxins in seawater, shellfish extract and homogenate, and mammalian body fluid such as urine and serum without pretreatment, dilution, or purification. We investigated the application of this technique for shellfish monitoring by spiking shellfish meat with brevetoxins and by analyzing oysters from two commercial shellfish beds in Florida that were exposed to a bloom of Karenia brevis (formerly Gymnodinium breve). We performed brevetoxin analysis of shellfish extracts and homogenates by ELISA and compared it with the mouse bioassay and receptor binding assay. The detection limit for brevetoxins in spiked oysters was 2.5 microg/100 g shellfish meat. This assay appears to be a useful tool for neurotoxic shellfish poisoning monitoring in shellfish and seawater, and for mammalian exposure diagnostics, and significantly reduces the time required for analyses. 2002-02 /pmc/articles/PMC1240733/ /pubmed/11836147 Text en
spellingShingle Research Article
Naar, Jerome
Bourdelais, Andrea
Tomas, Carmelo
Kubanek, Julia
Whitney, Philip L
Flewelling, Leanne
Steidinger, Karen
Lancaster, Johnny
Baden, Daniel G
A competitive ELISA to detect brevetoxins from Karenia brevis (formerly Gymnodinium breve) in seawater, shellfish, and mammalian body fluid.
title A competitive ELISA to detect brevetoxins from Karenia brevis (formerly Gymnodinium breve) in seawater, shellfish, and mammalian body fluid.
title_full A competitive ELISA to detect brevetoxins from Karenia brevis (formerly Gymnodinium breve) in seawater, shellfish, and mammalian body fluid.
title_fullStr A competitive ELISA to detect brevetoxins from Karenia brevis (formerly Gymnodinium breve) in seawater, shellfish, and mammalian body fluid.
title_full_unstemmed A competitive ELISA to detect brevetoxins from Karenia brevis (formerly Gymnodinium breve) in seawater, shellfish, and mammalian body fluid.
title_short A competitive ELISA to detect brevetoxins from Karenia brevis (formerly Gymnodinium breve) in seawater, shellfish, and mammalian body fluid.
title_sort competitive elisa to detect brevetoxins from karenia brevis (formerly gymnodinium breve) in seawater, shellfish, and mammalian body fluid.
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC1240733/
https://www.ncbi.nlm.nih.gov/pubmed/11836147
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