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开发一种用于检测食品中B型肉毒梭菌神经毒素的体外生物测定法,该方法比小鼠生物测定法更灵敏。

Development of an in vitro bioassay for Clostridium botulinum type B neurotoxin in foods that is more sensitive than the mouse bioassay.

作者信息

Wictome M, Newton K, Jameson K, Hallis B, Dunnigan P, Mackay E, Clarke S, Taylor R, Gaze J, Foster K, Shone C

机构信息

Centre for Applied Microbiology and Research, Porton Down, Salisbury, Wiltshire, SP4 OJG, United Kingdom.

出版信息

Appl Environ Microbiol. 1999 Sep;65(9):3787-92. doi: 10.1128/AEM.65.9.3787-3792.1999.

Abstract

A novel, in vitro bioassay for detection of the botulinum type B neurotoxin in a range of media was developed. The assay is amplified by the enzymic activity of the neurotoxin's light chain and includes the following three stages: first, a small, monoclonal antibody-based immunoaffinity column captures the toxin; second, a peptide substrate is cleaved by using the endopeptidase activity of the type B neurotoxin; and finally, a modified enzyme-linked immunoassay system detects the peptide cleavage products. The assay is highly specific for type B neurotoxin and is capable of detecting type B toxin at a concentration of 5 pg ml(-1) (0.5 mouse 50% lethal dose ml(-1)) in approximately 5 h. The format of the test was found to be suitable for detecting botulinum type B toxin in a range of foodstuffs with a sensitivity that exceeds the sensitivity of the mouse assay. Using highly specific monoclonal antibodies as the capture phase, we found that the endopeptidase assay was capable of differentiating between the type B neurotoxins produced by proteolytic and nonproteolytic strains of Clostridium botulinum type B.

摘要

开发了一种用于在一系列培养基中检测B型肉毒杆菌神经毒素的新型体外生物测定法。该测定法通过神经毒素轻链的酶活性进行放大,包括以下三个阶段:第一,一个基于单克隆抗体的小型免疫亲和柱捕获毒素;第二,利用B型神经毒素的内肽酶活性切割肽底物;最后,一个改良的酶联免疫测定系统检测肽切割产物。该测定法对B型神经毒素具有高度特异性,能够在约5小时内检测到浓度为5 pg ml(-1)(0.5小鼠50%致死剂量ml(-1))的B型毒素。发现该测试形式适用于检测一系列食品中的B型肉毒杆菌毒素,其灵敏度超过小鼠测定法的灵敏度。使用高度特异性的单克隆抗体作为捕获阶段,我们发现内肽酶测定法能够区分由B型肉毒杆菌的蛋白水解和非蛋白水解菌株产生的B型神经毒素。

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