Single transcript unit CRISPR 2.0 systems for robust Cas9 and Cas12a mediated plant genome editing

Plant Biotechnology Journal

2019

141

Summary Recently, CRISPR‐Cas12a (Cpf1) from Prevotella and Francisella was engineered to modify plant genomes. In this report, we employed CRISPR‐LbCas12a (LbCpf1), which is derived from Lachnospiraceae bacterium ND2006, to edit a citrus genome for the first time. First, LbCas12a was used to modify the CsPDS gene successfully in Duncan grapefruit via Xcc‐facilitated agroinfiltration. Next, LbCas12a driven by either the 35S or Yao promoter was used to edit the PthA4 effector binding elements in the promoter (EBEPthA4‐CsLOBP) of CsLOB1. A single crRNA was selected to target a conserved region of both Type I and Type II CsLOBPs, since the protospacer adjacent motif of LbCas12a (TTTV) allows crRNA to act on the conserved region of these two types of CsLOBP. CsLOB1 is the canker susceptibility gene, and it is induced by the corresponding pathogenicity factor PthA4 in Xanthomonas citri by binding to EBEPthA4‐CsLOBP. A total of seven 35S‐LbCas12a‐transformed Duncan plants were generated, and they were designated as #D35s1 to #D35s7, and ten Yao‐LbCas12a‐transformed Duncan plants were created and designated as #Dyao1 to #Dyao10. LbCas12a‐directed EBEPthA4‐CsLOBP modifications were observed in three 35S‐LbCas12a‐transformed Duncan plants (#D35s1, #D35s4 and #D35s7). However, no LbCas12a‐mediated indels were observed in the Yao‐LbCas12a‐transformed plants. Notably, transgenic line #D35s4, which contains the highest mutation rate, alleviates XccΔpthA4:dCsLOB1.4 infection. Finally, no potential off‐targets were observed. Therefore, CRISPR‐LbCas12a can readily be used as a powerful tool for citrus genome editing.

Section: Discussionmentioning

confidence: 99%

CRISPR‐LbCas12a‐mediated modification of citrus

Jia

Orbović

Plant Biotechnology Journal

2019

141

“…Primers were designed and synthesized for PCR analysis ( Supplementary Table S1). Amplified products were cloned into each target site, amplified by PCR, excised by restriction digestion with the corresponding enzymes, and positive clones were selected for Sanger sequencing [53,54]. All resistant callus material used to detect mutations was also used for off-target analysis.…”

Section: Targeted Mutagenesis Of Osnac006mentioning

confidence: 99%

Knockout of the OsNAC006 Transcription Factor Causes Drought and Heat Sensitivity in Rice

Zhong

et al. 2020

IJMS

Self Cite

Rice (Oryza sativa) responds to various abiotic stresses during growth. Plant-specific NAM, ATAF1/2, and CUC2 (NAC) transcription factors (TFs) play an important role in controlling numerous vital growth and developmental processes. To date, 170 NAC TFs have been reported in rice, but their roles remain largely unknown. Herein, we discovered that the TF OsNAC006 is constitutively expressed in rice, and regulated by H2O2, cold, heat, abscisic acid (ABA), indole-3-acetic acid (IAA), gibberellin (GA), NaCl, and polyethylene glycol (PEG) 6000 treatments. Furthermore, knockout of OsNAC006 using the CRISPR-Cas9 system resulted in drought and heat sensitivity. RNA sequencing (RNA-seq) transcriptome analysis revealed that OsNAC006 regulates the expression of genes mainly involved in response to stimuli, oxidoreductase activity, cofactor binding, and membrane-related pathways. Our findings elucidate the important role of OsNAC006 in drought responses, and provide valuable information for genetic manipulation to enhance stress tolerance in future plant breeding programs.

“…Because the tRNA sequence contains A and B boxes acting as promoter/enhancer, it increased gRNA expression in rice by one order of magnitude (Xie et al 2015). This gRNA processing strategy was later demonstrated in various plant, animal and microbial systems with consistently high efficiencies of multiplex genome editing (Dong et al 2017;Port and Bullock 2016;Shiraki and Kawakami 2018;Tang et al 2019). In addition to the tRNA-gRNA strategy, tandem repeats of gRNA-shRNA (short hairpin RNA) transcripts were also engineered for multiplex genome editing through excision of shRNAs by endogenous ribonuclease DROSHA in mammalian cells (Yan et al 2016).…”

Section: Diverse Strategies For Expressing Multiple Grnasmentioning

confidence: 98%

“…HDV gene), and may provide sequence variability, which reduces gene silencing and instability. The PTG transcript can be expressed by both Pol II and Pol III promoters, and was first reported in rice by achieving indel mutation frequencies up to 100% under a single U3 promoter (Dong et al 2017;Port and Bullock 2016;Shiraki and Kawakami 2018;Tang et al 2019;Xie et al 2015). Because the tRNA sequence contains A and B boxes acting as promoter/enhancer, it increased gRNA expression in rice by one order of magnitude (Xie et al 2015).…”

Section: Diverse Strategies For Expressing Multiple Grnasmentioning

confidence: 99%

“…1B). This system was shown to allow successful multiplex genome editing in animals and plants, in which a single RNA Pol II promoter is used to express Cas nuclease, gRNAs and other gRNA processing elements (e.g., ribozyme or tRNA elements) (Ding et al 2018;Tang et al 2016Tang et al , 2019Xu et al 2018;Yoshioka et al 2015). The STU system is first studied in mammalian cells, where HH-gRNA-HDV cassette is linked with Cas9 by an internal ribosome entry site (IRES) (Yoshioka et al 2015).…”

Section: Expression Of Cas Nuclease and Grnas From A Single Transcriptmentioning

confidence: 99%

See 1 more Smart Citation

Efficient expression of multiple guide RNAs for CRISPR/Cas genome editing

Hsieh‐Feng

Yang

2020

aBIOTECH

The Clustered Regularly Interspaced Short Palindromic Repeats/CRISPR-associated protein system (CRISPR/Cas) has recently become the most powerful tool available for genome engineering in various organisms. With efficient and proper expression of multiple guide RNAs (gRNAs), the CRISPR/Cas system is particularly suitable for multiplex genome editing. During the past several years, different CRISPR/Cas expression strategies, such as two-component transcriptional unit, single transcriptional unit, and bidirectional promoter systems, have been developed to efficiently express gRNAs as well as Cas nucleases. Significant progress has been made to optimize gRNA production using different types of promoters and RNA processing strategies such as ribozymes, endogenous RNases, and exogenous endoribonuclease (Csy4). Besides being constitutively and ubiquitously expressed, inducible and spatiotemporal regulations of gRNA expression have been demonstrated using inducible, tissue-specific, and/or synthetic promoters for specific research purposes. Most recently, the emergence of CRISPR/Cas ribonucleoprotein delivery methods, such as engineered nanoparticles, further revolutionized transgene-free and multiplex genome editing. In this review, we discuss current strategies and future perspectives for efficient expression and engineering of gRNAs with a goal to facilitate CRISPR/Cas-based multiplex genome editing.