数字聚合酶链反应技术对堆叠性状转基因大豆MON87708×MON89788的绝对定量检测

Q3 Agricultural and Biological Sciences

Oil Crop Science Pub Date : 2022-10-01 DOI:10.1016/j.ocsci.2022.11.001

Junyi Xu , Xin Li , Jinglian Bai , Ying Liu , Shaojie Wang , Yueting Liu , Chunguang Yang

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引用次数: 0

摘要

数字PCR (dPCR)的主要优点是便于对目标物进行绝对定量，而无需参考标准/校准曲线。结晶液滴dPCR具有三色染色检测功能，可实现多重PCR反应。本研究利用该技术建立了堆叠性状转基因大豆MON87708 × MON89788的三重dPCR检测方法。对转基因大豆MON87708 × MON89788种子均质化提取的基因组DNA进行了特异性绝对定量检测。研究结果可为转基因作物堆叠事件的绝对定量检测提供参考。

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Absolute quantitative detection of genetically modified soybean MON87708×MON89788 with stacked traits by digital polymerase chain reaction

The main advantage of digital PCR (dPCR) is that it facilitates absolute quantification of the target without reference to the standard/calibration curve. Crystal droplet dPCR has a three-color staining detection function, which enables multiplex PCR reaction. In this study, this technique was used to establish triple dPCR detection for the genetically modified soybean MON87708 × MON89788 with stacked traits. Specific absolute quantitative detection was accomplished for the genomic DNA extracted from the homogenized seeds of GM stack MON87708 × MON89788 soybean. Our results can serve as a reference for the absolute quantitative detection of stacked events of genetically modified crops.

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来源期刊

Oil Crop Science Food Science, Plant Science, Agronomy and Crop Science

CiteScore

3.40

自引率

0.00%

发文量

审稿时长

74 days