Detection and quantification of transgenes in grains by multiplex and real-time PCR

被引:94
作者
Permingeat, HR [1 ]
Reggiardo, MI [1 ]
Vallejos, RH [1 ]
机构
[1] Univ Nacl Rosario, CEFOBI, CONICET, Fdn M Lillo, RA-2000 Rosario, Santa Fe, Argentina
关键词
GMOs; real-time PCR; maize; soybean; CrylA(b); PAT;
D O I
10.1021/jf020081d
中图分类号
S [农业科学];
学科分类号
09 ;
摘要
Multiplex PCR reactions.,were developed for detecting simultaneously the CrylA(b) and pat genes from events 176, MON810, BT11, and T25 of transgenic maize, using only two pairs of primers, one for the CrylA(b) gene and the other for the pat gene. The Roundup Ready soybean can be precisely detected by a multiplex PCR reaction using known primers, amplifying fragments of the NOS and the epsps sequences simultaneously. Transgenic events such as Roundup Ready soybean and GA21 maize, among others, can be quantified b real-time PCR using a pair of primers and a probe specifically designed for annealing to the NOS ending region. As an alternative to amplifying an endogenous gene, the addition of a foreign gene in a percentage equal to the required level of detection, in a parallel reaction, is proposed. The use of hexane to homogenize large flour samples is suggested.
引用
收藏
页码:4431 / 4436
页数:6
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