Untargeted profiling of secondary metabolites and phytotoxins associated with stemphylium blight of lentil

Stanley Adobor; Sabine Banniza; Albert Vandenberg; Randy W Purves

doi:10.1007/s00425-023-04105-3

Untargeted profiling of secondary metabolites and phytotoxins associated with stemphylium blight of lentil

Planta. 2023 Mar 2;257(4):73. doi: 10.1007/s00425-023-04105-3.

Authors

Stanley Adobor¹, Sabine Banniza², Albert Vandenberg², Randy W Purves^{3

4}

Affiliations

¹ Pulse Crop Breeding and Genetics, Department of Plant Sciences, Crop Development Centre, University of Saskatchewan, Saskatoon, SK, Canada. stanley.adobor@usask.ca.
² Pulse Crop Breeding and Genetics, Department of Plant Sciences, Crop Development Centre, University of Saskatchewan, Saskatoon, SK, Canada.
³ College of Pharmacy and Nutrition, University of Saskatchewan, Saskatoon, SK, Canada. randy.purves@usask.ca.
⁴ Centre for Veterinary Drug Residues, Canadian Food Inspection Agency, Saskatoon, SK, Canada. randy.purves@usask.ca.

PMID: 36864322
DOI: 10.1007/s00425-023-04105-3

Abstract

Stemphylium botryosum alters lentil secondary metabolism and differentially affects resistant and susceptible genotypes. Untargeted metabolomics identifies metabolites and their potential biosynthetic pathways that play a crucial role in resistance to S. botryosum. The molecular and metabolic processes that mediate resistance to stemphylium blight caused by Stemphylium botryosum Wallr. in lentil are largely unknown. Identifying metabolites and pathways associated with Stemphylium infection may provide valuable insights and novel targets to breed for enhanced resistance. The metabolic changes following infection of four lentil genotypes by S. botryosum were investigated by comprehensive untargeted metabolic profiling employing reversed-phase or hydrophilic interaction liquid chromatography (HILIC) coupled to a Q-Exactive mass spectrometer. At the pre-flowering stage, plants were inoculated with S. botryosum isolate SB19 spore suspension and leaf samples were collected at 24, 96 and 144 h post-inoculation (hpi). Mock-inoculated plants were used as negative controls. After analyte separation, high-resolution mass spectrometry data was acquired in positive and negative ionization modes. Multivariate modeling revealed significant treatment, genotype and hpi effects on metabolic profile changes that reflect lentil response to Stemphylium infection. In addition, univariate analyses highlighted numerous differentially accumulated metabolites. By contrasting the metabolic profiles of SB19-inoculated and mock-inoculated plants and among lentil genotypes, 840 pathogenesis-related metabolites were detected including seven S. botryosum phytotoxins. These metabolites included amino acids, sugars, fatty acids and flavonoids in primary and secondary metabolism. Metabolic pathway analysis revealed 11 significant pathways including flavonoid and phenylpropanoid biosynthesis, which were affected upon S. botryosum infection. This research contributes to ongoing efforts toward a comprehensive understanding of the regulation and reprogramming of lentil metabolism under biotic stress, which will provide targets for potential applications in breeding for enhanced disease resistance.

Keywords: HILIC; Mass spectrometry; Metabolomics; Plant-pathogen interaction; RPLC; Stemphylium botryosum.

MeSH terms

Alkaloids*
Lens Plant*
Metabolomics
Plant Breeding
Secondary Metabolism

Substances

Alkaloids

Supplementary concepts

Stemphylium botryosum