Plant gene editing through de novo induction of meristems
Abstract
Plant gene editing is typically performed by delivering
reagents such as Cas9 and single guide RNAs to explants in culture. Edited
cells are then induced to differentiate into whole plants by exposure to
various hormones. The creation of edited plants through tissue culture is often
inefficient, time-consuming, works for only limited species and genotypes, and
causes unintended changes to the genome and epigenome.
Here we report two
methods to generate gene-edited dicotyledonous plants through de novo meristem
induction. Developmental regulators and gene-editing reagents are delivered to
somatic cells of whole plants. This induces meristems that produce shoots with
targeted DNA modifications, and gene edits are transmitted to the next
generation.
The de novo induction of gene-edited meristems sidesteps the need
for tissue culture and promises to overcome a bottleneck in plant gene editing.
Maher, M.F., Nasti, R.A., Vollbrecht, M. et al. Plant gene
editing through de novo induction of meristems. Nat Biotechnol (2019)
doi:10.1038/s41587-019-0337-2
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