Abstract

Key messageDiscriminatory co-expression of maizeBBMandWUStranscriptional factor genes promoted somatic embryogenesis and efficientAgrobacterium-mediated transformation of recalcitrant maize inbred B73 and sorghum P898012 genotypes without use of a selectable marker gene.The use of morphogenic regulators to overcome barriers in plant transformation is a revolutionary breakthrough for basic plant science and crop applications. Current standard plant transformation systems are bottlenecks for genetic, genomic, and crop improvement studies. We investigated the differential use of co-expression of maize transcription factors BABY BOOM and WUSCHEL2 coupled with a desiccation inducible CRE/lox excision system to enable regeneration of stable transgenic recalcitrant maize inbred B73 and sorghum P898012 without a chemical selectable marker. The PHP78891 expression cassette contains CRE driven by the drought inducible maize RAB17M promoter with lox P sites which bracket the CRE, WUS, and BBM genes. A constitutive maize UBIM promoter directs a ZsGreen GFP expression cassette as a reporter outside of the excision sites and provides transient, transgenic, and developmental analysis. This was coupled with evidence for molecular integration and analysis of stable integration and desiccation inducible CRE-mediated excision. Agrobacterium-mediated transgenic introduction of this vector showed transient expression of GFP and induced somatic embryogenesis in maize B73 and sorghum P898012 explants. Subjection to desiccation stress in tissue culture enabled the excision of CRE, WUS, and BBM, leaving the UBIM::GFP cassette and allowing subsequent plant regeneration and GFP expression analysis. Stable GFP expression was observed in the early and late somatic embryos, young shoots, vegetative plant organs, and pollen. Transgene integration and expression of GFP positive T0 plants were also analyzed using PCR and Southern blots. Progeny segregation analysis of primary events confirmed correlation between functional GFP expression and presence of the GFP transgene in T1 plants generated from self pollinations, indicating good transgene inheritance. This study confirms and extends the use of morphogenic regulators to overcome transformation barriers.

Highlights

  • Cereal crops arguably feed the world and are grown in greater quantities on more land across more diverse ecosystems than any other crop (Borlaug 2002; FAOSTAT 2012)

  • We investigated the differential use of co-expression of maize transcription factors BABY BOOM and WUSCHEL2 coupled with a desiccation inducible CRE/lox excision system to enable regeneration of stable transgenic recalcitrant maize inbred B73 and sorghum P898012 without a chemical selectable marker

  • Plant Cell Rep (2017) 36:1477–1491 accomplish heritable genetic transformation of plants has been essential to basic science in plant biology and to myriad crop applications essential to worldwide agriculture and world food supply

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Summary

Introduction

Cereal crops arguably feed the world and are grown in greater quantities on more land across more diverse ecosystems than any other crop (Borlaug 2002; FAOSTAT 2012). To become more broadly significant, a pan-application systems approach to plant biology and genomics is being actuated (Altpeter et al 2016) These efforts have been stymied by technological limitations because of inherent features of standard plant transgenics. Plant transformation has been encumbered by several bottlenecks (Altpeter et al 2016) including genotype and varietal dependence, explant sources and specific cell culture dependence, as well as laborious, expensive, and time-consuming technologies. This is especially true for the cereal crops. The need to overcome these obstacles is apparent (Altpeter et al 2016)

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