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The Development of DNA Based Methods for the Reliable and Efficient Identification of Nicotiana tabacum in Tobacco and Its Derived Products

机译:基于DNA的烟草及其衍生产物可靠高效鉴定方法的建立。

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摘要

Reliable methods are needed to detect the presence of tobacco components in tobacco products to effectively control smuggling and classify tariff and excise in tobacco industry to control illegal tobacco trade. In this study, two sensitive and specific DNA based methods, one quantitative real-time PCR (qPCR) assay and the other loop-mediated isothermal amplification (LAMP) assay, were developed for the reliable and efficient detection of the presence of tobacco (Nicotiana tabacum) in various tobacco samples and commodities. Both assays targeted the same sequence of the uridine 5′-monophosphate synthase (UMPS), and their specificities and sensitivities were determined with various plant materials. Both qPCR and LAMP methods were reliable and accurate in the rapid detection of tobacco components in various practical samples, including customs samples, reconstituted tobacco samples, and locally purchased cigarettes, showing high potential for their application in tobacco identification, particularly in the special cases where the morphology or chemical compositions of tobacco have been disrupted. Therefore, combining both methods would facilitate not only the detection of tobacco smuggling control, but also the detection of tariff classification and of excise.
机译:需要可靠的方法来检测烟草制品中烟草成分的存在,以有效控制走私,并对烟草业的关税和消费税进行分类,以控制非法烟草贸易。在这项研究中,开发了两种基于敏感DNA和特异性DNA的方法,一种是定量实时PCR(qPCR)测定法,另一种是环介导的等温扩增(LAMP)测定法,用于可靠,有效地检测烟草(Nicotiana)的存在。烟草)和各种烟草样品和商品中。两种测定法均靶向尿苷5'-单磷酸合酶(UMPS)的相同序列,并使用多种植物材料确定了它们的特异性和敏感性。 qPCR和LAMP方法在快速检测各种实际样品(包括海关样品,重构烟草样品和本地购买的卷烟)中的烟草成分方面均可靠且准确,显示出其在烟草鉴定中的应用潜力,尤其是在特殊情况下烟草的形态或化学成分已被破坏。因此,将这两种方法结合起来不仅将有助于检测烟草走私管制,而且还有助于检测关税分类和消费税。

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