Published October 15, 2021 | Version v1
Journal article Open

CRISPR-Cas12a Genome Editing at the Whole-Plant Level Using Two Compatible RNA Virus Vectors

Description

The use of viral vectors that can replicate and move systemically through the host plant to deliver bacterialCRISPR components enables genome editing at the whole-plant level and avoids the requirement for labor-intensive stable transformation. However, this approach usually relies on previously transformed plants thatstably express a CRISPR-Cas nuclease. Here, we describe successful DNA-free genome editing ofNicotiana ben-thamianausing two compatible RNA virus vectors derived from tobacco etch virus (TEV; genusPotyvirus) andpotato virus X (PVX; genusPotexvirus), which replicate in the same cells. The TEV and PVX vectors respectivelyexpress a Cas12a nuclease and the corresponding guide RNA. This novel two-virus vector system improvesthe toolbox for transformation-free virus-induced genome editing in plants and will advance efforts to breedmore nutritious, resistant, and productive crops.

Notes

This research was supported by grants BIO2017-83184-Rand PID2019-108203RB-I00 from the Ministerio deCiencia e Innovacio ́n (Spain) through the Agencia Estatalde Investigacio ́n (co-financed by the European RegionalDevelopment Fund) and H2020-760331 Newcotiana fromthe European Commission. M.U. and M.V.-V. are the recip-ients of fellowships FPU17/05503 from the Ministerio deCiencia e Innovacio ́n (Spain) and APOSTD/2020/096from the Generalitat Valenciana (Spain), respectively.

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crispr.2021.0049.pdf

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Additional details

Funding

Newcotiana – Developing Multipurpose Nicotiana Crops for Molecular Farming using New Plant Breeding Techniques 760331
European Commission