A Fluorescent Microplate Assay for Diarrheic Shellfish Toxins

A fluorescent enzyme inhibition assay for okadaic acid using 4-methylumbelliferyl phosphate and fluorescein diphosphate as substrates for the enzyme phosphatase 2A was developed. In the inhibition assay, performed in a microtiter plate, the PP2A was inhibited by adding okadaic acid and the resulting...

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Published inAnalytical biochemistry Vol. 248; no. 2; pp. 258 - 264
Main Authors Vieytes, M.R., Fontal, O.I., Leira, F., de Sousa, J.M.V.Baptista, Botana, L.M.
Format Journal Article
LanguageEnglish
Published United States Elsevier Inc 01.06.1997
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Abstract A fluorescent enzyme inhibition assay for okadaic acid using 4-methylumbelliferyl phosphate and fluorescein diphosphate as substrates for the enzyme phosphatase 2A was developed. In the inhibition assay, performed in a microtiter plate, the PP2A was inhibited by adding okadaic acid and the resulting fluorescence enhancement derived from enzymatic hydrolysis of the substrate was quantified in a fluorescence plate reader. The measurable range of okadaic acid was 3.2 to 3200 pg/ml with an IC50= 0.1 nm. The detection limit of okadaic acid was 2.56 pg/well in buffer solutions and 12.8 ng/g hepatopancreas in shellfish extracts. The coefficient of variation (CV,n= 22) for each point ranged from 18.80 to 37.90% (mean 28.35%). The proposed method is very convenient, rapid, and sensitive by using the enzyme inhibition assay system and fluorescent reaction as a detection system. This work demonstrates that the fluorescent assay can be used to quantify the amount of okadaic acid in shellfish samples and also is valid for very dilute samples, such as phytoplankton samples.
AbstractList A fluorescent enzyme inhibition assay for okadaic acid using 4-methylumbelliferyl phosphate and fluorescein diphosphate as substrates for the enzyme phosphatase 2A was developed. In the inhibition assay, performed in a microtiter plate, the PP2A was inhibited by adding okadaic acid and the resulting fluorescence enhancement derived from enzymatic hydrolysis of the substrate was quantified in a fluorescence plate reader. The measurable range of okadaic acid was 3.2 to 3200 pg/ml with an IC50 = 0.1 nM. The detection limit of okadaic acid was 2.56 pg/well in buffer solutions and 12.8 ng/g hepatopancreas in shellfish extracts. The coefficient of variation (CV, n = 22) for each point ranged from 18.80 to 37.90% (mean 28.35%). The proposed method is very convenient, rapid, and sensitive by using the enzyme inhibition assay system and fluorescent reaction as a detection system. This work demonstrates that the fluorescent assay can be used to quantify the amount of okadaic acid in shellfish samples and also is valid for very dilute samples, such as phytoplankton samples.
Author Botana, L.M.
Leira, F.
de Sousa, J.M.V.Baptista
Vieytes, M.R.
Fontal, O.I.
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Snippet A fluorescent enzyme inhibition assay for okadaic acid using 4-methylumbelliferyl phosphate and fluorescein diphosphate as substrates for the enzyme...
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StartPage 258
SubjectTerms Animals
Diarrhea - etiology
Fluoresceins
Fluorescent Dyes
Fluorometry - methods
Fluorometry - statistics & numerical data
Humans
Hymecromone - analogs & derivatives
Marine Toxins - analysis
Okadaic Acid - analysis
Organophosphorus Compounds
Phosphoprotein Phosphatases - antagonists & inhibitors
Protein Phosphatase 2
Reproducibility of Results
Sensitivity and Specificity
Shellfish - analysis
Shellfish Poisoning
Substrate Specificity
Title A Fluorescent Microplate Assay for Diarrheic Shellfish Toxins
URI https://dx.doi.org/10.1006/abio.1997.2127
https://www.ncbi.nlm.nih.gov/pubmed/9177752
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