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Novel Disease Resistance Gene Paralogs Created by CRISPR/Cas9 in Soy.

Nagy Ervin D.,Stevens Julia L.,Yu Neil, Hubmeier Chris S., LaFaver Nona, Gillespie Megan,Gardunia Brian, Cheng Qianshun,Johnson Steven, Vaughn Audrey L.,Vega-Sanchez Miguel E., Deng Mingqui,Rymarquis Linda,Lawrence Richard J.,Garvey Graeme S.,Gaeta Robert T.

Plant Cell Reports(2021)

Bayer Crop Science

Cited 18|Views19
Abstract
Novel disease resistance gene paralogues are generated by targeted chromosome cleavage of tandem duplicated NBS-LRR gene complexes and subsequent DNA repair in soybean. This study demonstrates accelerated diversification of innate immunity of plants using CRISPR. Nucleotide-binding-site-leucine-rich-repeat (NBS-LRR) gene families are key components of effector-triggered immunity. They are often arranged in tandem duplicated arrays in the genome, a configuration that is conducive to recombinations that will lead to new, chimeric genes. These rearrangements have been recognized as major sources of novel disease resistance phenotypes. Targeted chromosome cleavage by CRISPR/Cas9 can conceivably induce rearrangements and thus emergence of new resistance gene paralogues. Two NBS-LRR families of soy have been selected to demonstrate this concept: a four-copy family in the Rpp1 region (Rpp1L) and a large, complex locus, Rps1 with 22 copies. Copy-number variations suggesting large-scale, CRISPR/Cas9-mediated chromosome rearrangements in the Rpp1L and Rps1 complexes were detected in up to 58.8% of progenies of primary transformants using droplet-digital PCR. Sequencing confirmed development of novel, chimeric paralogs with intact open reading frames. These novel paralogs may confer new disease resistance specificities. This method to diversify innate immunity of plants by genome editing is readily applicable to other disease resistance genes or other repetitive loci.
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CRISPR,Cas9,Soy,NBS-LRR,Disease resistance
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