Highly efficient generation of bacterial leaf blight-resistant and transgene-free rice using a genome editing and multiplexed selection system

Kun Yu; Zhiqiang Liu; Huaping Gui; Lizhao Geng; Juan Wei; Dawei Liang; Jian Lv; Jianping Xu; Xi Chen

doi:10.1186/s12870-021-02979-7

Highly efficient generation of bacterial leaf blight-resistant and transgene-free rice using a genome editing and multiplexed selection system

BMC Plant Biol. 2021 Apr 24;21(1):197. doi: 10.1186/s12870-021-02979-7.

Authors

Kun Yu¹, Zhiqiang Liu¹, Huaping Gui¹, Lizhao Geng¹, Juan Wei¹, Dawei Liang¹, Jian Lv¹, Jianping Xu¹, Xi Chen²

Affiliations

¹ Syngenta Biotechnology (China) Co., Ltd, No.25, Life Science Park Road, Beijing, 102206, China.
² Syngenta Biotechnology (China) Co., Ltd, No.25, Life Science Park Road, Beijing, 102206, China. [email protected].

Abstract

Background: Rice leaf blight, which is a devastating disease worldwide, is caused by the bacterium Xanthomonas oryzae pv. oryzae (Xoo). The upregulated by transcription activator-like 1 (UPT) effector box in the promoter region of the rice Xa13 gene plays a key role in Xoo pathogenicity. Mutation of a key bacterial protein-binding site in the UPT box of Xa13 to abolish PXO99-induced Xa13 expression is a way to improve rice resistance to bacteria. Highly efficient generation and selection of transgene-free edited plants are helpful to shorten and simplify the gene editing-based breeding process. Selective elimination of transgenic pollen of T0 plants can enrich the proportion of T1 transgene-free offspring, and expression of a color marker gene in seeds makes the selection of T2 plants very convenient and efficient. In this study, a genome editing and multiplexed selection system was used to generate bacterial leaf blight-resistant and transgene-free rice plants.

Results: We introduced site-specific mutations into the UPT box using CRISPR/Cas12a technology to hamper with transcription-activator-like effector (TAL) protein binding and gene activation and generated genome-edited rice with improved bacterial blight resistance. Transgenic pollen of T0 plants was eliminated by pollen-specific expression of the α-amylase gene Zmaa1, and the proportion of transgene-free plants increased from 25 to 50% among single T-DNA insertion events in the T1 generation. Transgenic seeds were visually identified and discarded by specific aleuronic expression of DsRed, which reduced the cost by 50% and led to up to 98.64% accuracy for the selection of transgene-free edited plants.

Conclusion: We demonstrated that core nucleotide deletion in the UPT box of the Xa13 promoter conferred resistance to rice blight, and selection of transgene-free plants was boosted by introducing multiplexed selection. The combination of genome editing and transgene-free selection is an efficient strategy to accelerate functional genomic research and plant breeding.

Keywords: Bacterial blight; Disease; Genome editing; Transgene-free.

MeSH terms

Disease Resistance*
Gene Editing / methods*
Genome, Plant*
Oryza / genetics*
Oryza / microbiology
Plant Breeding
Plant Diseases / genetics*
Plant Diseases / microbiology
Transgenes
Xanthomonas / physiology*

Supplementary concepts

Xanthomonas oryzae