Genome-wide identification and characterization of the GDP-L-galactose phosphorylase gene family in bread wheat

Ronan C Broad; Julien P Bonneau; Jesse T Beasley; Sally Roden; Joshua G Philips; Ute Baumann; Roger P Hellens; Alexander A T Johnson

doi:10.1186/s12870-019-2123-1

Genome-wide identification and characterization of the GDP-L-galactose phosphorylase gene family in bread wheat

BMC Plant Biol. 2019 Nov 26;19(1):515. doi: 10.1186/s12870-019-2123-1.

Authors

Ronan C Broad¹, Julien P Bonneau¹, Jesse T Beasley¹, Sally Roden², Joshua G Philips², Ute Baumann³, Roger P Hellens², Alexander A T Johnson⁴

Affiliations

¹ School of BioSciences, The University of Melbourne, Melbourne, Victoria, 3010, Australia.
² Centre for Tropical Crops and Biocommodities, Institute for Future Environments, Queensland University of Technology, Brisbane, Queensland, 4001, Australia.
³ School of Agriculture, The University of Adelaide, Adelaide, South Australia, 5064, Australia.
⁴ School of BioSciences, The University of Melbourne, Melbourne, Victoria, 3010, Australia. johnsa@unimelb.edu.au.

Abstract

Background: Ascorbate is a powerful antioxidant in plants and an essential micronutrient for humans. The GDP-L-galactose phosphorylase (GGP) gene encodes the rate-limiting enzyme of the L-galactose pathway-the dominant ascorbate biosynthetic pathway in plants-and is a promising gene candidate for increasing ascorbate in crops. In addition to transcriptional regulation, GGP production is regulated at the translational level through an upstream open reading frame (uORF) in the long 5'-untranslated region (5'UTR). The GGP genes have yet to be identified in bread wheat (Triticum aestivum L.), one of the most important food grain sources for humans.

Results: Bread wheat chromosomal groups 4 and 5 were found to each contain three homoeologous TaGGP genes on the A, B, and D subgenomes (TaGGP2-A/B/D and TaGGP1-A/B/D, respectively) and a highly conserved uORF was present in the long 5'UTR of all six genes. Phylogenetic analyses demonstrated that the TaGGP genes separate into two distinct groups and identified a duplication event of the GGP gene in the ancestor of the Brachypodium/Triticeae lineage. A microsynteny analysis revealed that the TaGGP1 and TaGGP2 subchromosomal regions have no shared synteny suggesting that TaGGP2 may have been duplicated via a transposable element. The two groups of TaGGP genes have distinct expression patterns with the TaGGP1 homoeologs broadly expressed across different tissues and developmental stages and the TaGGP2 homoeologs highly expressed in anthers. Transient transformation of the TaGGP coding sequences in Nicotiana benthamiana leaf tissue increased ascorbate concentrations more than five-fold, confirming their functional role in ascorbate biosynthesis in planta.

Conclusions: We have identified six TaGGP genes in the bread wheat genome, each with a highly conserved uORF. Phylogenetic and microsynteny analyses highlight that a transposable element may have been responsible for the duplication and specialized expression of GGP2 in anthers in the Brachypodium/Triticeae lineage. Transient transformation of the TaGGP coding sequences in N. benthamiana demonstrated their activity in planta. The six TaGGP genes and uORFs identified in this study provide a valuable genetic resource for increasing ascorbate concentrations in bread wheat.

Keywords: Ascorbic acid; Gene expression; Phylogeny; Synteny; Transient expression; Upstream open reading frame; Vitamin C.

MeSH terms

Ascorbic Acid / metabolism
Bread
Genes, Plant
Phosphoric Monoester Hydrolases / genetics*
Plant Proteins / genetics*
Triticum / enzymology
Triticum / genetics*

Substances

Plant Proteins
Phosphoric Monoester Hydrolases
Ascorbic Acid