4.7 Article

A simple, flexible and high-throughput cloning system for plant genome editing via CRISPR-Cas system

Journal

JOURNAL OF INTEGRATIVE PLANT BIOLOGY
Volume 58, Issue 8, Pages 705-712

Publisher

WILEY
DOI: 10.1111/jipb.12474

Keywords

AarI-mediated sgRNA cloning; CRISPR-Cas9 T-DNA binary vector; Exchangeable U6; U3 promoter; Gateway compatible Cas9 cloning

Funding

  1. Institute for Basic Science [IBS-R021-D1]
  2. Ministry of Science, ICT & Future Planning, Republic of Korea [IBS-R021-D1-2016-A00] Funding Source: Korea Institute of Science & Technology Information (KISTI), National Science & Technology Information Service (NTIS)

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CRISPR-Cas9 system is now widely used to edit a target genome in animals and plants. Cas9 protein derived from Streptococcus pyogenes (SpCas9) cleaves double-stranded DNA targeted by a chimeric single-guide RNA (sgRNA). For plant genome editing, Agrobacterium-mediated T-DNA transformation has been broadly used to express Cas9 proteins and sgRNAs under the control of CaMV 35S and U6/U3 promoter, respectively. We here developed a simple and high-throughput binary vector system to clone a 19-20 bp of sgRNA, which binds to the reverse complement of a target locus, in a large T-DNA binary vector containing an SpCas9 expressing cassette. Two-step cloning procedures: (1) annealing two target-specific oligonucleotides with overhangs specific to the AarI restriction enzyme site of the binary vector; and (2) ligating the annealed oligonucleotides into the two AarI sites of the vector, facilitate the high-throughput production of the positive clones. In addition, Cas9-coding sequence and U6/U3 promoter can be easily exchanged via the Gateway(TM) system and unique EcoRI/XhoI sites on the vector, respectively. We examined the mutation ratio and patterns when we transformed these constructs into Arabidopsis thaliana and a wild tobacco, Nicotiana attenuata. Our vector system will be useful to generate targeted large-scale knock-out lines of model as well as non-model plant.

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