RNA-Guided Cas9-Induced Mutagenesis in Tobacco Followed by Efficient Genetic Fixation in Doubled Haploid Plants.

Sindy Schedel,Andrea Müller,Stefanie Pencs,Jochen Kumlehn,Götz Hensel,Twan Rutten

doi:10.3389/fpls.2016.01995

Sindy Schedel, Andrea Müller + Show 4 more

Open Access

https://doi.org/10.3389/fpls.2016.01995

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Abstract

Customizable endonucleases are providing an effective tool for genome engineering. The resulting primary transgenic individuals (T0) are typically heterozygous and/or chimeric with respect to any mutations induced. To generate genetically fixed mutants, they are conventionally allowed to self-pollinate, a procedure which segregates individuals into mutant heterozygotes/homozygotes and wild types. The chances of recovering homozygous mutants among the progeny depend not only on meiotic segregation but also on the frequency of mutated germline cells in the chimeric mother plant. In Nicotiana species, the heritability of Cas9-induced mutations has not been demonstrated yet. RNA-guided Cas9 endonuclease-mediated mutagenesis was targeted to the green fluorescent protein (GFP) gene harbored by a transgenic tobacco line. Upon retransformation using a GFP-specific guide RNA/Cas9 construct, the T0 plants were allowed to either self-pollinate, or were propagated via regeneration from in vitro cultured embryogenic pollen which give rise to haploid/doubled haploid plants or from leaf explants that form plants vegetatively. Single or multiple mutations were detected in 80% of the T0 plants. About half of these mutations proved heritable via selfing. Regeneration from in vitro cultured embryogenic pollen allowed for homozygous mutants to be produced more efficiently than via sexual reproduction. Consequently, embryogenic pollen culture provides a convenient method to rapidly generate a variety of genetically fixed mutants following site-directed mutagenesis. The recovery of a mutation not found among sexually produced and analyzed progeny was shown to be achievable through vegetative plant propagation in vitro, which eventually resulted in heritability when the somatic clones were selfed. In addition, some in-frame mutations were associated with functional attenuation of the target gene rather than its full knock-out. The generation of mutants with compromised rather than abolished gene functionality holds promise for future approaches to the conclusive functional validation of genes which are indispensible for the plant.

Highlights

Site-specific modifications to genomic DNA sequence, induced by either customizable zinc finger nucleases (ZFNs, Kim et al, 1996), transcription activator-like effector nucleases (TALENs, Christian et al, 2010) or the more recently established RNAor DNA-guided endonucleases (RGENs, Jinek et al, 2012; Shan et al, 2013; Zetsche et al, 2015; NgAgo, Gao et al, 2016), represents the new frontier in genetic engineering
Selections are validated in the T2 generation. guide RNA (gRNA)/Cas9-mediated mutagenesis in the genus Nicotiana was first demonstrated at the cellular level in Nicotiana benthamiana (Li et al, 2013; Nekrasov et al, 2013), since when its effectiveness has been established in Nicotiana tabacum plants (Gao et al, 2014)
Introducing a green fluorescent protein (GFP)-specific gRNA/Cas9 construct into tobacco resulted in a high proportion (80%) of the T0 plants experiencing one or more mutations to the target locus

Summary

Introduction

Site-specific modifications to genomic DNA sequence, induced by either customizable zinc finger nucleases (ZFNs, Kim et al, 1996), transcription activator-like effector nucleases (TALENs, Christian et al, 2010) or the more recently established RNAor DNA-guided endonucleases (RGENs, Jinek et al, 2012; Shan et al, 2013; Zetsche et al, 2015; NgAgo, Gao et al, 2016), represents the new frontier in genetic engineering. All of these platforms involve a customizable DNA-binding module (proteinaceous in the case of ZFN and TALEN, and complementary nucleic acid molecules in the case of RGEN and NgAgo) along with a generic enzymatic DNA-cleavage module (FokI for ZFNs and TALENs, Cas or Cpf for RGENs and Argonaute in case of the NgAgo platform). Selections are validated in the T2 generation. gRNA/Cas9-mediated mutagenesis in the genus Nicotiana was first demonstrated at the cellular level in Nicotiana benthamiana (Li et al, 2013; Nekrasov et al, 2013), since when its effectiveness has been established in Nicotiana tabacum plants (Gao et al, 2014)

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