Harnessing the Power of an Extensive EMS‐Induced Sorghum Population for Rapid Crop Improvement

Author:

Mason Patrick John12ORCID,Blaakmeer Anko3,Furtado Agnelo1,Stuart Peter Norman4,Nomula Rajesh1,Bjarnholt Nanna56,Sørensen Mette5,Koleva Donka Teneva5,Pedas Pai Rosager3,Knudsen Søren3,Møller Birger Lindberg52,Skadhauge Birgitte3,Henry Robert James12ORCID

Affiliation:

1. Queensland Alliance of Agriculture and Food Innovation, The University of Queensland St Lucia QLD Australia

2. ARC Centre of Excellence for Plant Success in Nature and Agriculture, The University of Queensland St Lucia QLD Australia

3. Carlsberg Research Laboratory Copenhagen V Denmark

4. Seedtek Pty Ltd Toowoomba QLD Australia

5. Plant Biochemistry Laboratory, Department of Plant and Environmental Sciences, University of Copenhagen Frederiksberg Denmark

6. Copenhagen Plant Science Centre, Department of Plant and Environmental Sciences, University of Copenhagen Frederiksberg Denmark

Abstract

AbstractPlant breeders leverage mutagenesis using chemical, biological, and physical mutagens to create novel trait variations. Many widely used sorghum genotypes have a narrow genetic base, which hinders improvements using classical breeding. Enhancing the diversity of the sorghum genome thus remains a key priority for sorghum breeders. To accelerate the genetic enhancement of sorghum, an extensive library comprised of seeds from 150,000 individual mutant plants of the Sorghum bicolor inbred line BTx623 was established using ethyl methanesulphonate (EMS) as a mutagen. The sorghum mutant library was bulked into 1498 pools (~100 seed heads per pool). In each pool, DNA was extracted from a subset of the seed and screened using the FIND‐IT technology based on droplet digital PCR. All 43 nucleotide substitutions that were screened using FIND‐IT were identified, demonstrating the potential to identify any EMS‐derived mutation in an elite line of sorghum within days. This diverse library represents the largest collection of sorghum mutants ever conceived, estimated to cover 240% of all possible EMS‐induced mutation points within the Sorghum genome. Using FIND‐IT, the speed at which a specific desired EMS‐derived mutation can be identified is a major upgrade to conventional reverse genetic techniques. Additionally, the ease at which valuable variants can be integrated into elite commercial lines is a far simpler and less expensive process compared to genome editing. Genomic variations in the library will have direct utility as a breeding resource for commercial sorghum applications, allowing enhanced adaptation to climate change and enhanced yield potential in marginal environments.

Publisher

Wiley

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