Qualitative and quantitative PCR methods for event-specific detection of genetically modified cotton Mon1445 and Mon531

文献类型: 外文期刊

第一作者: Yang, LT

作者: Yang, LT;Pan, AH;Zhang, KW;Yin, CS;Qian, BJ;Chen, JX;Huang, C;Zhang, DB

作者机构:

关键词: genetically modified cotton;Mon1445;Mon531;multiplex PCR;reference molecule;TaqMan real-time PCR

期刊名称:TRANSGENIC RESEARCH ( 影响因子:2.788; 五年影响因子:2.377 )

ISSN: 0962-8819

年卷期: 2005 年 14 卷 6 期

页码:

收录情况: SCI

摘要: Based on the DNA sequences of the junctions between recombinant and cotton genomic DNA of the two genetically modified (GM) cotton varieties, herbicide-tolerance Mon1445 and insect-resistant Mon531, event-specific primers and probes for qualitative and quantitative PCR detection for both GM cotton varieties were designed, and corresponding detection methods were developed. In qualitative PCR detection, the simplex and multiplex PCR detection systems were established and employed to identify Mon1445 and Mon531 from other GM cottons and crops. The limits of detection (LODs) of the simplex PCR were 0.05% for both Mon1445 and Mon531 using 100 ng DNA templates in one reaction, and the LOD of multiplex PCR analysis was 0.1%. For further quantitative detection using TaqMan real-time PCR systems for Mon1445 and Mon531, one plasmid pMD-ECS, used as reference molecule was constructed, which contained the quantitative amplified fragments of Mon1445, Mon531, and cotton endogenous reference gene. The limits of quantification (LOQs) of Mon1445 and Mon531 event-specific PCR systems using plasmid pMD-ECS as reference molecule were 10 copies, and the quantification range was from 0.03 to 100% in 100 ng of the DNA template for one reaction. Thereafter, five mixed cotton samples containing 0, 0.5, 0.9, 3 and 5% Mon1445 or Mon531 were quantified using established real-time PCR systems to evaluate the accuracy and precision of the developed real-time PCR detection systems. The accuracy expressed as bias varied from 1.33 to 8.89% for tested Mon1445 cotton samples, and from 2.67 to 6.80% for Mon531. The precision expressed as relative standard deviations (RSD) were different from 1.13 to 30.00% for Mon1445 cotton, and from 1.27 to 24.68% for Mon531. The range of RSD was similar to other laboratory results (25%). Concluded from above results, we believed that the established event-specific qualitative and quantitative PCR systems for Mon1445 and Mon531 in this study are acceptable and suitable for GM cotton identification and quantification.

分类号:

  • 相关文献

[1]Integrated structure and event-specific real-time detection of transgenic cry1Ac/SCK rice Kefeng 6. Su, Changqing,Xie, Jiajian,Wang, Xifeng,Peng, Yufa,Su, Changqing. 2011

[2]Fitness of Bt-resistant cabbage loopers on Bt cotton plants. Tetreau, Guillaume,Wang, Ran,Wang, Ping,Wang, Ran,Tetreau, Guillaume,Wang, Ran. 2017

[3]Application and development of a TaqMan real-time PCR for detecting infectious spleen and kidney necrosis virus in Siniperca chuatsi. Lin, Qiang,Fu, Xiaozhe,Liu, Lihui,Liang, Hongru,Guo, Huizhi,Yin, Shuwen,Huang, Zhibin,Li, Ningqiu,Kumaresan, Venkatesh.

[4]Estimating the copy number of transgenes in transformed rice by real-time quantitative PCR. Yang, LT,Ding, JY,Zhang, CM,Jia, JW,Weng, HB,Liu, WX,Zhang, DB. 2005

[5]A specific qualitative and real-time PCR detection of MON863 maize based on the 5 '-transgene integration sequence. Zhu, Hong,Jia, Junwei,Sun, Jianping,Zhao, Kai,Zhao, Xiao. 2008

[6]Pre-infestation of Tomato Plants by Aphids Modulates Transmission-Acquisition Relationship among Whiteflies, Tomato Yellow Leaf Curl Virus (TYLCV) and Plants. Ge, Feng,Tan, Xiao L.,Chen, Ju L.,Tan, Xiao L.,Liu, Tong X.,Tan, Xiao L.,Liu, Tong X.,Benelli, Giovanni,Desneux, Nicolas,Yang, Xue Q.. 2017

[7]Comparison of white spot syndrome virus quantification of fleshy shrimp Fenneropenaeus chinensis in outdoor ponds between different growing seasons by TaqMan real-time polymerase chain reaction. Meng, Xian-Hong,Jang, In Kwon,Kim, Jong-Sheek,Kim, Bong-Rae,Meng, Xian-Hong. 2011

[8]Real-time PCR quantification of Bemisia tabaci (Homoptera : Aleyrodidae) B-biotype remains in predator guts. Zhang, Gui-Fen,Lue, Zhi-Chuang,Wan, Fang-Hao,Loevei, Gabor L.. 2007

[9]A TaqMan real-time PCR assay for survey of white spot syndrome virus (WSSV) infections in Litopenaeus vannamei postlarvae and shrimp of farms in different grow-out seasons. Meng, Xian-Hong,Jang, In Kwon,Seo, Hyung-Chul,Cho, Yeong-Rok,Meng, Xian-Hong.

[10]Development of an allele-specific marker for Glu-B3 alleles in common wheat and establishment of a multiplex PCR assay. Sui, Xinxia,Wang, Linhai,Xia, Xianchun,He, Zhonghu,Sui, Xinxia,Wang, Zhenlin,He, Zhonghu. 2010

[11]Response surface methodology to design a selective co-enrichment broth of Escherichia coli, Salmonella spp. and Staphylococcus aureus for simultaneous detection by multiplex PCR. Zhang, Qiao Yan,Zhou, Yu,Wang, Xiao Fu,Xu, Jun Feng,Zhou, Wen Wu. 2012

[12]Establishment of a Multiplex PCR and an Investigation of Co-Infection Rate of WSSV and IHHNV in Penaeid vannamei in Northern of Jiangsu. Chen, Yi-Bing,Gao, Song,Zhou, Jun-Fang,Wan, Xi-He. 2012

[13]Identification and Quantification of Three Genetically Modified Insect Resistant Cotton Lines Using Conventional and TaqMan Real-Time Polymerase Chain Reaction Methods. Yang, LT,Pan, AH,Zhang, KW,Guo, JC,Yin, CS,Chen, JX,Huang, C,Zhang, DB.

[14]Rapid diagnosis of goose viral infections by multiplex PCR. Chen, Zongyan,Li, Chuanfeng,Li, Guoxin,Yu, Hai,Jiang, Yifeng,Yan, Liping,Meng, Chunchun,Zhou, Yanjun,Tong, Guangzhi,Liu, Guangqing.

[15]Development of a multiplex PCR assay for detection and discrimination of Theileria annulata and Theileria sergenti in cattle. Junlong, Liu,Li, Youquan,Liu, Aihong,Guan, Guiquan,Xie, Junren,Yin, Hong,Luo, Jianxun,Junlong, Liu,Li, Youquan,Liu, Aihong,Guan, Guiquan,Xie, Junren,Yin, Hong,Luo, Jianxun.

[16]Development of one-tube multiplex polymerase chain reaction (PCR) for detecting Mycobacterium bovis. Quan, Zhang,Haiming, Tan,Xiaoya, Cai,Weifeng, Yuan,Hong, Jia,Hongfei, Zhu.

[17]A multiplex reverse transcription-PCR assay for the detection of influenza A virus and differentiation of the H1, H3, H5 and H9 subtypes. Wu, Ling,Ding, Longfei,Pei, Zenglin,Pan, Zishu,Huo, Xixiang,Wen, Guoyuan.

[18]Development and characterization of four moderate multiplex microsatellite panels in crucian carp (Carassius auratus). Cheng, Lei,Lu, Cui-Yun,Li, Chao,Sun, Xiao-Wen,Zhang, Yan. 2013

[19]Rapid identification of deer products by multiplex PCR assay. Zha, Dai-Ming,Xing, Xiu-Mei,Yang, Fu-He,Zha, Dai-Ming,Zha, Dai-Ming,Xing, Xiu-Mei,Yang, Fu-He,Zha, Dai-Ming,Xing, Xiu-Mei,Yang, Fu-He.

[20]A PCR method targeting internal transcribed spacers: the simultaneous detection of Babesia bigemina and Babesia bovis in cattle. Liu, Junlong,Guan, Guiquan,Liu, Aihong,Li, Youquan,Yin, Hong,Luo, Jianxun.

作者其他论文 更多>>

微信小程序