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Efficient gene targeting in soybean using Ochrobactrum haywardense-mediated delivery of a marker-free donor template
Author(s) -
Sandeep Kumar,
Zhan-Bin Liu,
Nathalie Sanyour-Doyel,
Brian Lenderts,
Andrew Worden,
Ajith Anand,
HyeonJe Cho,
Joy Bolar,
C. Jake Harris,
Lingxia Huang,
Aiqiu Xing,
Alexandra Richardson
Publication year - 2022
Publication title -
plant physiology
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 3.554
H-Index - 312
eISSN - 1532-2548
pISSN - 0032-0889
DOI - 10.1093/plphys/kiac075
Subject(s) - selectable marker , biology , plasmid , genetics , crispr , gene , transformation (genetics) , locus (genetics) , computational biology , genomic dna , genome editing , microbiology and biotechnology
Gene targeting (GT) for precise gene insertion or swap into pre-defined genomic location has been a bottleneck for expedited soybean precision breeding. We report a robust selectable marker-free GT system in soybean, one of the most economically important crops. An efficient Oh H1-8 (Ochrobactrum haywardense H1-8)-mediated embryonic axis transformation method was used for the delivery of CRISPR-Cas9 components and donor template to regenerate T0 plants 6–8 weeks after transformation. This approach generated up to 3.4% targeted insertion of the donor sequence into the target locus in T0 plants, with ∼ 90% mutation rate observed at the genomic target site. The GT was demonstrated in two genomic sites using two different donor DNA templates without the need for a selectable marker within the template. High-resolution Southern-by-Sequencing analysis identified T1 plants with precise targeted insertion and without unintended plasmid DNA. Unlike previous low-frequency GT reports in soybean that involved particle bombardment–mediated delivery and extensive selection, the method described here is fast, efficient, reproducible, does not require a selectable marker within the donor DNA, and generates nonchimeric plants with heritable GT.

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