Scientia Agricultura Sinica ›› 2017, Vol. 50 ›› Issue (7): 1294-1301.doi: 10.3864/j.issn.0578-1752.2017.07.012

• HORTICULTURE • Previous Articles     Next Articles

Establishment of an Efficient CRISPR/Cas9-Mediated Gene Editing System in Banana

HU ChunHua, DENG GuiMing, SUN XiaoXuan, ZUO CunWu, LI ChunYu, KUANG RuiBin, YANG QiaoSong, YI GanJun   

  1. Fruit Tree Research Institute, Guangdong Academy of Agricultural Science/Key Laboratory of Biology and Genetic Resource Utilization of Fruit Trees in South Subtropics, the Ministry of Agriculture, Guangzhou 510640
  • Received:2016-11-08 Online:2017-04-01 Published:2017-04-01

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Abstract: Objective The objective of this study is to establish a CRISPR/Cas9-mediated gene editing system in order to find a new way for revealing gene function and breeding of banana. Method According to the Musa genomic (A genome) sequence of phytoene desaturase gene 8 (MaPDS), online tools ZiFiT Targeter Version 4.2 was used to determine the appropriate designing of CRISPR/Cas9 target sites, one of the output target sites was selected for designing the sgRNA. The sgRNA and U6a promoter sequences were linked by overlapping PCR to produce U6a-sgRNA expression cassette, then the fragment was cloned into the binary pYLCRISPR/Cas9 multiplex genome targeting vector system based on Golden Gate Cloning, a pYLCRISPR/Cas9 vector carrying sgRNA cassette named pYLCRISPR/Cas9-sgRNA was generated. The plant expression binary vector, containing a Cas9 (Cas9p) expression cassette, driven by the maize ubiquitin promoter (Pubi), and the sgRNA with target sequence of MaPDS was transcribed under the control of the U6a promoter from rice. The constructed plasmid was then transformed into EHA105 strain of Agrobacterium tumefaciens, which was subsequently used to infect embryogenic cell suspensions (ECS) of banana to obtain resistant plantlets. PCR amplifications were carried out using primer pairs flanking the designed target site. The PCR products were sequenced for detection of mutation.ResultMaPDS was selected as the target of Cas9 endonuclease, and a sgRNA was designed as the target site for CRIPSR/Cas9. The sgRNA with target sequence was firstly inserted into the sgRNA expression cassette by using overlapping PCR, then the cassette was combined with the pYLCRISPR/Cas9 in a single plant binary vector. The results of identification by enzyme digestion and sequencing showed that the pYLCRISPR/Cas9-sgRNA vector aiming at MaPDSa Cas9 expression cassette driven by Pu was successfully constructed, and the vector harbors bi, and a sgRNA expression cassette under the U6a promoter. Using this system and Agrobacterium-mediated transformation,129 independently transformed lines with visible albino, chimerism mutant phenotypes and normal phenotypes were regenerated from ECS after transformation, resistance screening, resistant embryo induction, germination and rooting process. The ratio of albino and chimerism phenotype occurred in transgenic banana was more than 55% (71 out of 129).Albino phenotype in these transgenic plants indicates the loss of PtoPDS function. To further verify whether the loss of green in the transgenic banana was caused by generation of mutations in the MaPDS by the CRISPR/Cas9 system, 33mutant phenotypes and 14 normal phenotypes from 129 independent transgenic plants were randomly selected for sequencing. The results confirmed that all of these transgenic plants with albino phenotype contained mutants in the MaPDS, insertion (a Aor T) and displacement were found in the target sites of MaPDS in the mutants. And it was also found the displacement in downstream of the target sites of MaPDS in the experiments, no mutation was detected in the normal phenotypes of transgenic and control plants.Conclusion The CRISPR/Cas9 system was successfully applied to knock out the endogenous phytoene dehydrogenase (PDS) gene in banana. The results demonstrate that the Cas9/sgRNA system can be exploited to targeted mutagenesis and effectively create knockout mutations in banana.

Key words: banana, CRISPR/Cas9, MaPDS, gene editing

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