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Development of a rapid and accurate PCR-based detection method for commercially valuable green algal species

机译:开发一种基于PCR的快速准确的商业价值绿藻检测方法

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We developed a rapid and accurate PCR-based inspection technique for individual detection of five commercially important green algal species, Ulva linza, U. prolifera, U. intestinalis, U. compressa and Monostroma nitidum, all of which are controlled as import quota items in Japan. This analytical method has solved the general problem of PCR-based detection methods of being defenseless against false-negatives by application of a duplex PCR technique with an internal control band generated by a set of universal primers for green algal species. Due to the detection of small-sized PCR products of < 250 bp lengths, the analytical method would be useful for deeply processed products and completes its quick PCR amplification within 45 min. The validity of the developed analytical method was proved by a pre-test using a total of 129 samples (12 imported products and 31 Japanese commercial products). This analytical method is a powerful tool for screening of commercial green algal products to discover the five controlled algal species and will allow inspection authorities, including the Customs Service, to improve their examination systems in terms of simplification, rapidity and cost-effectiveness
机译:我们开发了一种基于PCR的快速准确的检测技术,用于单独检测五种具有重要商业价值的绿藻物种,即石莼、增殖藻、肠藻、压缩藻和单菌,所有这些藻类在日本都作为进口配额项目进行管制。该分析方法解决了基于PCR的检测方法的一般问题,即通过应用双链PCR技术,该技术具有由一组绿藻物种的通用引物生成的内部对照带,从而无法防御假阴性。由于可检测<250 bp长度的小尺寸PCR产物,该分析方法可用于深度加工产物,并在45 min内完成快速PCR扩增。使用总共129个样品(12个进口产品和31个日本商业产品)进行预测试,证明了所开发的分析方法的有效性。这种分析方法是筛选商业绿藻产品以发现五种受控藻类的有力工具,并使包括海关在内的检查机构能够在简化、快速和成本效益方面改进其检查系统

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