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Detection method of genetically modified papaya using duplex PCR

机译:双链PCR检测转基因木瓜的方法

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摘要

A simple and rapid method for the identification of genetically modified (GM) papaya, derived from Line 55-1, was developed by modifying the Japanese official PCR method. Genomic DNA was directly extracted from the fresh fruit without the lyophilization step, using a commercial silica-based kit. To develop a duplex PCR method which simultaneously detects the GM papaya-specific gene and the intrinsic papain gene, the papain 2-5'/3' (amplicon size; 184 bp) primer pair for the detection of the papain gene was newly designed within the region of the products (211 bp) amplified using the papain 1-5'/-3' primer pair adopted in the Japanese official PCR method. To detect the GM papaya-specific gene, the primer pair Nos C-5'/CaM N-3' described in the Japanese official method was used. The DNA sequences of the GM papaya gene and the intrinsic papain gene were co-amplified using the PCR method in a single tube. The developed duplex PCR method allows the simultaneous detection of the products by means of agarose gel electrophoresis or microchip electrophoresis. The proposed method for GM papaya identification is simple and rapid.
机译:通过修改日本官方PCR方法,开发了一种简单快速的鉴定来自55-1品系的转基因(GM)木瓜的方法。使用商业的基于二氧化硅的试剂盒,无需冷冻干燥步骤即可直接从新鲜水果中提取基因组DNA。为了开发一种可同时检测GM木瓜特异性基因和内在木瓜基因的双链PCR方法,新设计了用于检测木瓜基因的木瓜2-5'/ 3'(扩增子大小; 184 bp)引物对。使用日本官方PCR方法中采用的木瓜蛋白酶1-5'/-3'引物对扩增的产物区域(211 bp)。为了检测转基因木瓜特异性基因,使用了日本官方方法中所述的引物对C-5'/ CaM N-3'。使用PCR方法在单个管中共同扩增了GM木瓜基因和固有木瓜蛋白基因的DNA序列。发达的双链PCR方法允许通过琼脂糖凝胶电泳或微芯片电泳同时检测产物。提出的转基因木瓜鉴定方法简便,快速。

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