A prolific and robust whole-genome genotyping method using PCR amplification via primer-template mismatched annealingOO

Whole-genome genotyping methods are important for breeding. However, it has been challenging to develop a robust method for simultaneous fore-ground and background genotyping that can easily be adapted to different genes and species. In our study, we accidently discovered that in adapter ligation-me...

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Veröffentlicht in:植物学报(英文版) 2023, Vol.65 (3), p.633-645
Hauptverfasser: Sheng Zhao, Cuicui Zhang, Liqun Wang, Minxuan Luo, Peng Zhang, Yue Wang, Waqar Afzal Malik, Peng Chen, Xianjin Qiu, Chongrong Wang, Hong Lu, Yong Xiang, Yuwen Liu, Jue Ruan, Qian Qian, Haijian Zhi, Yuxiao Chang
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Sprache:eng
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Zusammenfassung:Whole-genome genotyping methods are important for breeding. However, it has been challenging to develop a robust method for simultaneous fore-ground and background genotyping that can easily be adapted to different genes and species. In our study, we accidently discovered that in adapter ligation-mediated PCR, the amplification by primer-template mismatched annealing (PTMA) along the genome could generate thousands of stable PCR products. Based on this observation, we con-sequently developed a novel method for simulta-neous foreground and background integrated geno-typing by sequencing (FBI-seq) using one specific primer, in which foreground genotyping is performed by primer-template perfect annealing (PTPA), while background genotyping employs PTMA. Unlike DNA arrays, multiple PCR, or genome target enrichments, FBI-seq requires little preliminary work for primer design and synthesis, and it is easily adaptable to different foreground genes and species. FBI-seq therefore provides a prolific, robust, and accurate method for simultaneous foreground and back-ground genotyping to facilitate breeding in the post-genomics era.
ISSN:1672-9072