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Multiallelic, Targeted Mutagenesis of Magnesium Chelatase With CRISPR/Cas9 Provides a Rapidly Scorable Phenotype in Highly Polyploid Sugarcane

Front Genome Ed. 2021-04; 
Ayman Eid, Chakravarthi Mohan, Sara Sanchez, Duoduo Wang, Fredy Altpeter
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DNA Sequencing … sgRNA vectors containing Oryza sativa U6 promoter were designed and custom synthesized in the pUC57 backbone (Genscript, NJ, USA) to generate pUCMg12. The Mg-chelatase target guide sequences were simultaneously cloned into the vector using annealed primer-… Get A Quote

摘要

Genome editing with sequence-specific nucleases, such as clustered regularly interspaced short palindromic repeats (CRISPR)/CRISPR-associated protein 9 (Cas9), is revolutionizing crop improvement. Developing efficient genome-editing protocols for highly polyploid crops, including sugarcane ( = 10-13), remains challenging due to the high level of genetic redundancy in these plants. Here, we report the efficient multiallelic editing of magnesium chelatase subunit I () in sugarcane. Magnesium chelatase is a key enzyme for chlorophyll biosynthesis. CRISPR/Cas9-mediated targeted co-mutagenesis of 49 copies/alleles of magnesium chelatase was confirmed via Sanger sequencing of cloned PCR amplicons. This resulted in se... More

关键词

CRISPR/Cas9, biolistic gene transfer, genome editing, heat treatment, magnesium chelatase, polyploid, sugarcane