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Detection of Botulinum Neurotoxin A in a Spiked Milk Sample with Subtype Identification through Toxin Proteomics

机译:通过毒素蛋白质组学鉴定亚型鉴定牛奶样品中肉毒杆菌神经毒素A

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Botulinum neurotoxin (BoNT) causes the disease botulism, which can be lethal if untreated. Rapid determination of exposure to BoNT is an important public health goal. Previous work in our laboratory focused on the development of Endopep-MS, a mass spectrometry-based endopeptidase method for detecting and differentiating BoNT in buffer. This method can rapidly determine the presence of BoNT in a sample and differentiate the toxin type of BoNT present but does not yield additional information about the subtype. We now describe here the application of Endopep-MS to detect BoNT A in a spiked milk sample. This work also describes subtype identification achieved through mass spectrometric analysis of the protein toxin itself and does not require the presence of DNA from the toxin-producing bacteria. Tryptic digests of A1 and A2 subtypes of BoNT were analyzed by mass spectrometry, and peptides unique to either the A1 or A2 subtype were subjected to tandem mass spectrometry analysis to confirm their identities. Finally, subtype identification through mass spectrometric analysis was performed on BoNT A isolated from spiked milk. In its entirety, this method would allow for analysis of BoNT with toxin type identification in a few hours and subtype identification within 24 h.
机译:肉毒杆菌神经毒素(BoNT)会导致疾病肉毒中毒,如果不加以治疗可能会致命。快速确定接触BoNT的暴露是一项重要的公共卫生目标。我们实验室以前的工作重点是开发Endopep-MS,这是一种基于质谱的内肽酶方法,用于检测和区分缓冲​​液中的BoNT。此方法可以快速确定样品中BoNT的存在,并区分BoNT的毒素类型,但不会产生有关该亚型的其他信息。现在,我们在这里描述Endopep-MS在加标牛奶样品中检测BoNT A的应用。这项工作还描述了通过蛋白质毒素本身的质谱分析实现的亚型鉴定,并且不需要存在来自毒素产生细菌的DNA。通过质谱分析BoNT的A1和A2亚型的胰蛋白酶消化物,并对A1或A2亚型独特的肽进行串联质谱分析,以确认其身份。最后,通过质谱分析对加标牛奶中分离的BoNT A进行亚型鉴定。总体而言,该方法可在数小时内通过毒素类型鉴定分析BoNT,并在24小时内进行亚型鉴定。

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