Outlook for coeliac disease patients: towards bread wheat with hypoimmunogenic gluten by gene editing of α- and γ-gliadin gene families

Aurélie Jouanin; Jan G Schaart; Lesley A Boyd; James Cockram; Fiona J Leigh; Ruth Bates; Emma J Wallington; Richard G F Visser; Marinus J M Smulders

doi:10.1186/s12870-019-1889-5

Outlook for coeliac disease patients: towards bread wheat with hypoimmunogenic gluten by gene editing of α- and γ-gliadin gene families

BMC Plant Biol. 2019 Aug 1;19(1):333. doi: 10.1186/s12870-019-1889-5.

Authors

Aurélie Jouanin^{1

2}, Jan G Schaart³, Lesley A Boyd⁴, James Cockram⁴, Fiona J Leigh⁴, Ruth Bates⁴, Emma J Wallington⁴, Richard G F Visser³, Marinus J M Smulders⁵

Affiliations

¹ Wageningen University and Research, Plant Breeding, Wageningen, The Netherlands. aurelie.jouanin@gmail.com.
² The John Bingham Laboratory, NIAB, Huntingdon Road, Cambridge, UK. aurelie.jouanin@gmail.com.
³ Wageningen University and Research, Plant Breeding, Wageningen, The Netherlands.
⁴ The John Bingham Laboratory, NIAB, Huntingdon Road, Cambridge, UK.
⁵ Wageningen University and Research, Plant Breeding, Wageningen, The Netherlands. rene.smulders@wur.nl.

Abstract

Background: Wheat grains contain gluten proteins, which harbour immunogenic epitopes that trigger Coeliac disease in 1-2% of the human population. Wheat varieties or accessions containing only safe gluten have not been identified and conventional breeding alone struggles to achieve such a goal, as the epitopes occur in gluten proteins encoded by five multigene families, these genes are partly located in tandem arrays, and bread wheat is allohexaploid. Gluten immunogenicity can be reduced by modification or deletion of epitopes. Mutagenesis technologies, including CRISPR/Cas9, provide a route to obtain bread wheat containing gluten proteins with fewer immunogenic epitopes.

Results: In this study, we analysed the genetic diversity of over 600 α- and γ-gliadin gene sequences to design six sgRNA sequences on relatively conserved domains that we identified near coeliac disease epitopes. They were combined in four CRISPR/Cas9 constructs to target the α- or γ-gliadins, or both simultaneously, in the hexaploid bread wheat cultivar Fielder. We compared the results with those obtained with random mutagenesis in cultivar Paragon by γ-irradiation. For this, Acid-PAGE was used to identify T1 grains with altered gliadin protein profiles compared to the wild-type endosperm. We first optimised the interpretation of Acid-PAGE gels using Chinese Spring deletion lines. We then analysed the changes generated in 360 Paragon γ-irradiated lines and in 117 Fielder CRISPR/Cas9 lines. Similar gliadin profile alterations, with missing protein bands, could be observed in grains produced by both methods.

Conclusions: The results demonstrate the feasibility and efficacy of using CRISPR/Cas9 to simultaneously edit multiple genes in the large α- and γ-gliadin gene families in polyploid bread wheat. Additional methods, generating genomics and proteomics data, will be necessary to determine the exact nature of the mutations generated with both methods.

Keywords: CRISPR/Cas9; Coeliac disease; Gene editing; Gluten; Mutation breeding; Polyploid; Wheat; α-Gliadin; γ-Gliadin; γ-Irradiation.

MeSH terms

CRISPR-Associated Protein 9
CRISPR-Cas Systems
Electrophoresis, Polyacrylamide Gel
Gene Editing / methods*
Genes, Plant / genetics*
Gliadin / genetics*
Glutens / genetics*
Glutens / immunology
Plant Breeding / methods
Plants, Genetically Modified
Sequence Alignment
Triticum / genetics*

Substances

Glutens
Gliadin
CRISPR-Associated Protein 9

Grants and funding

FP7-PEOPLE-2013_ITN-607178/FP7 People: Marie-Curie Actions