A Carbamoylase-Based Bioassay for the Detection of Paralytic Shellfish Poisoning Toxins

被引:9
|
作者
Raposo, Mariana [1 ,2 ]
Botelho, Maria Joao [3 ,4 ]
Costa, Sara T. [3 ]
Gomes, Maria Teresa S. R. [1 ,2 ]
Rudnitskaya, Alisa [1 ,2 ]
机构
[1] Univ Aveiro, CESAM, P-3810193 Aveiro, Portugal
[2] Univ Aveiro, Dept Chem, P-3810193 Aveiro, Portugal
[3] Portuguese Inst Sea & Atmosphere, IPMA, P-1449006 Lisbon, Portugal
[4] Univ Porto, CIIMAR, Interdisciplinary Ctr Marine & Environm Res, P-4050123 Porto, Portugal
关键词
carbamoylase; paralytic shellfish toxins; potentiometric sensor; gonyautoxin; 5; decarbamoylsaxitoxin; enzymatic assay; RECEPTOR-BINDING ASSAY; MARINE TOXINS; GYMNODINIUM-CATENATUM; TRANSFORMING ENZYME; BIOSENSOR; SAXITOXIN; ALGAL; PURIFICATION; BIOTOXINS; PROFILES;
D O I
10.3390/s20020507
中图分类号
O65 [分析化学];
学科分类号
070302 ; 081704 ;
摘要
Out of control proliferation of toxic phytoplankton, called harmful algal blooms (HABs), have a significant economic impact on bivalve aquaculture and harvesting in coastal waters. Some phytotoxins, such as paralytic shellfish toxins (PSTs), are of concern due to the life-threatening symptoms they can cause. Development of rapid and low-cost screening tools would be a welcome addition to the laboratory methodologies employed in routine monitoring programs. However, most of the assays and biosensors for the screening of PSTs, are restricted to a single target, saxitoxin (STX), which is the most potent PST. The present study aimed at developing an assay for the detection of N-sulfocarbamoyl PST-GTX5, which is one of the most abundant toxins in bivalves during G. catenatum blooms as found on the Portuguese coast. Enzymatic assay employing PSTs' transforming enzyme-carbamoylase-was proposed. Carbamoylase was extracted and purified from the surf clam S. solida. Carbamoylase displayed similar specificity to both carbamate (STX) and N-sulfocarbamate toxins (GTX5 and C1+2) converting them into decarbamoyl saxitoxin (dcSTX) and decarbamoyl gonyautoxins 2+3 (dcGTX2+3), respectively. The enzymatic assay involved hydrolysis of GTX5 by carbamoylase and quantification of the product of enzymatic reaction, dcSTX, using a potentiometric chemical sensor. A potentiometric sensor with plasticized PVC membrane that displayed sensitivity to dcSTX and selectivity in the presence of GTX5 was employed. Enzymatic assay allowed determination of GTX5 in the concentration range from 0.43 to 3.30 mu molL(-1), which encompasses levels of GTX5 in contaminated bivalve extracts with toxicities above PSTs regulatory limits. The feasibility of the carbamoylase-based potentiometric assay for detection of GTX5 was demonstrated.
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页数:14
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