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竞争性酶联免疫吸附测定法:一种监测环境和生物样品中短裸甲藻毒素的准确、快速且有效的工具。

Competitive ELISA: An Accurate, Quick and Effective Tool to Monitor Brevetoxins in Environmental and Biological Sample.

作者信息

Naar Jerome, Weidner Allison, Baden Daniel G

出版信息

Harmful Algae 2002 (2002). 2004;10:291-293.

Abstract

A competitive Enzyme-Linked Immuno-Sorbent Assay (competitive ELISA) has been developed for analyzing brevetoxins (PbTxs). Antibodies to brevetoxins were used in combination with a multi-step signal amplification procedure for the detection of toxins. This procedure minimizes non-specific signals and background noise often observed in complex matrices. Therefore, analysis can be performed with various samples (seawater, air filter, mammalian body fluids, shellfish, etc.) without the need for extensive extraction and/or purification steps. Brevetoxin analysis in liquid samples like seawater, urine and serum can be performed without pretreatment, dilution or purification. The limit of quantification of PbTxs is 2 ng mL in any of the liquid sample matrices tested. For shellfish monitoring, analyses are performed after homogenization of shellfish meat (5 g) with brevetoxin-ELISA buffer (200 mL) and can be performed on tissue from a single mollusk as well as on a pool of shellfish meat. Comparative quantification of PbTxs achieved in buffer, seawater, mammalian body fluid and shellfish homogenate spiked with equal amounts of toxin (10 ng mL sample) varied by no more than 5%. These data suggest that the matrix composition of the sample does not affect the performance of the assay. Because this assay is not affected by matrix composition and can be performed in shellfish homogenate, this procedure can be used to prevent or diagnose human exposure to PbTxs and has the potential to replace the currently used mouse bioassay for monitoring PbTxs in shellfish.

摘要

已开发出一种竞争性酶联免疫吸附测定法(竞争性ELISA)用于分析短裸甲藻毒素(PbTxs)。短裸甲藻毒素抗体与多步信号放大程序结合使用以检测毒素。该程序可将复杂基质中常见的非特异性信号和背景噪声降至最低。因此,无需大量提取和/或纯化步骤即可对各种样品(海水、空气过滤器、哺乳动物体液、贝类等)进行分析。像海水、尿液和血清等液体样品中的短裸甲藻毒素分析无需预处理、稀释或纯化即可进行。在所测试的任何液体样品基质中,PbTxs的定量限为2 ng/mL。对于贝类监测,将贝类肉(5 g)与短裸甲藻毒素ELISA缓冲液(200 mL)匀浆后进行分析,可对单个软体动物的组织以及贝类肉池进行分析。在添加等量毒素(10 ng/mL样品)的缓冲液、海水、哺乳动物体液和贝类匀浆中实现的PbTxs比较定量差异不超过5%。这些数据表明样品的基质组成不会影响该测定法的性能。由于该测定法不受基质组成的影响且可在贝类匀浆中进行,因此该程序可用于预防或诊断人类接触PbTxs,并有潜力取代目前用于监测贝类中PbTxs的小鼠生物测定法。

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