Identification and functional characterisation of a locus for target site integration in Fusarium graminearum

Martin Darino; Martin Urban; Navneet Kaur; Ana Machado Wood; Mike Grimwade-Mann; Dan Smith; Andrew Beacham; Kim Hammond-Kosack

doi:10.1186/s40694-024-00171-8

Identification and functional characterisation of a locus for target site integration in Fusarium graminearum

Fungal Biol Biotechnol. 2024 Feb 26;11(1):2. doi: 10.1186/s40694-024-00171-8.

Authors

Martin Darino¹, Martin Urban^#², Navneet Kaur^#², Ana Machado Wood³, Mike Grimwade-Mann⁴, Dan Smith⁵, Andrew Beacham⁶, Kim Hammond-Kosack⁷

Affiliations

¹ Protecting Crops and the Environment, Rothamsted Research, Harpenden, Hertfordshire, AL5 2JQ, UK. martin.darino@rothamsted.ac.uk.
² Protecting Crops and the Environment, Rothamsted Research, Harpenden, Hertfordshire, AL5 2JQ, UK.
³ Jealott's Hill International Research Centre, Syngenta, Warfield, Bracknell, RG42 6EY, UK.
⁴ Human Milk Foundation, Daniel Hall Building, Harpenden, Hertfordshire, AL5 2JQ, UK.
⁵ Intelligent Data Ecosystems, Harpenden, Hertfordshire, AL5 2JQ, UK.
⁶ Centre for Crop and Environment Sciences, Harper Adams University, Shropshire, TF10 8NB, UK.
⁷ Protecting Crops and the Environment, Rothamsted Research, Harpenden, Hertfordshire, AL5 2JQ, UK. kim.hammond-kosack@rothamsted.ac.uk.

^# Contributed equally.

Abstract

Background: Fusarium Head Blight (FHB) is a destructive floral disease of different cereal crops. The Ascomycete fungus Fusarium graminearum (Fg) is one of the main causal agents of FHB in wheat and barley. The role(s) in virulence of Fg genes include genetic studies that involve the transformation of the fungus with different expression cassettes. We have observed in several studies where Fg genes functions were characterised that integration of expression cassettes occurred randomly. Random insertion of a cassette may disrupt gene expression and/or protein functions and hence the overall conclusion of the study. Target site integration (TSI) is an approach that consists of identifying a chromosomal region where the cassette can be inserted. The identification of a suitable locus for TSI in Fg would avert the potential risks of ectopic integration.

Results: Here, we identified a highly conserved intergenic region on chromosome 1 suitable for TSI. We named this intergenic region TSI locus 1. We developed an efficient cloning vector system based on the Golden Gate method to clone different expression cassettes for use in combination with TSI locus 1. We present evidence that integrations in the TSI locus 1 affects neither fungal virulence nor fungal growth under different stress conditions. Integrations at the TSI locus 1 resulted in the expression of different gene fusions. In addition, the activities of Fg native promoters were not altered by integration into the TSI locus 1. We have developed a bespoke bioinformatic pipeline to analyse the existence of ectopic integrations, cassette truncations and tandem insertions of the cassette that may occurred during the transformation process. Finally, we established a protocol to study protein secretion in wheat coleoptiles using confocal microscopy and the TSI locus 1.

Conclusion: The TSI locus 1 can be used in Fg and potentially other cereal infecting Fusarium species for diverse studies including promoter activity analysis, protein secretion, protein localisation studies and gene complementation. The bespoke bioinformatic pipeline developed in this work together with PCR amplification of the insert could be an alternative to Southern blotting, the gold standard technique used to identify ectopic integrations, cassette truncations and tandem insertions in fungal transformation.

Keywords: Coleoptiles; Complementation; Confocal microscopy; Fungal transformation; Fusarium Head Blight; Fusarium graminearum; Genome sequence; Secretion; Target site integration; Wheat.

Abstract

Grants and funding