A fast and simple LC-MS-based characterization of the flavonoid biosynthesis pathway for few seed(ling)s

Benjamin Jaegle; Miran Kalle Uroic; Xu Holtkotte; Christina Lucas; Andreas Ole Termath; Hans-Günther Schmalz; Marcel Bucher; Ute Hoecker; Martin Hülskamp; Andrea Schrader

doi:10.1186/s12870-016-0880-7

A fast and simple LC-MS-based characterization of the flavonoid biosynthesis pathway for few seed(ling)s

BMC Plant Biol. 2016 Sep 1;16(1):190. doi: 10.1186/s12870-016-0880-7.

Affiliations

¹ Botanical Institute and Cluster of Excellence on Plant Sciences (CEPLAS), University of Cologne, Cologne Biocenter, Zülpicher Str. 47b, 50674, Cologne, Germany.
² Department of Chemistry, University of Cologne, Greinstr. 4, 50939, Cologne, Germany.
³ Botanical Institute and Cluster of Excellence on Plant Sciences (CEPLAS), University of Cologne, Cologne Biocenter, Zülpicher Str. 47b, 50674, Cologne, Germany. martin.huelskamp@uni-koeln.de.
⁴ Botanical Institute and Cluster of Excellence on Plant Sciences (CEPLAS), University of Cologne, Cologne Biocenter, Zülpicher Str. 47b, 50674, Cologne, Germany. andrea.schrader@uni-koeln.de.

Abstract

Background: (Pro)anthocyanidins are synthesized by the flavonoid biosynthesis pathway with multi-layered regulatory control. Methods for the analysis of the flavonoid composition in plants are well established for different purposes. However, they typically compromise either on speed or on depth of analysis.

Results: In this work we combined and optimized different protocols to enable the analysis of the flavonoid biosynthesis pathway with as little as possible biological material. We chose core substances of this metabolic pathway that serve as a fingerprint to recognize alterations in the main branches of the pathway. We used a simplified sample preparation, two deuterated internal standards, a short and efficient LC separation, highly sensitive detection with tandem MS in multiple reaction monitoring (MRM) mode and hydrolytic release of the core substances to reduce complexity. The method was optimized for Arabidopsis thaliana seeds and seedlings. We demonstrate that one Col-0 seed/seedling is sufficient to obtain a fingerprint of the core substances of the flavonoid biosynthesis pathway. For comparative analysis of different genotypes, we suggest the use of 10 seed(lings). The analysis of Arabidopsis thaliana mutants affecting steps in the pathway revealed foreseen and unexpected alterations of the pathway. For example, HY5 was found to differentially regulate kaempferol in seeds vs. seedlings. Furthermore, our results suggest that COP1 is a master regulator of flavonoid biosynthesis in seedlings but not of flavonoid deposition in seeds.

Conclusions: When sample numbers are high and the plant material is limited, this method effectively facilitates metabolic fingerprinting with one seed(ling), revealing shifts and differences in the pathway. Moreover the combination of extracted non-hydrolysed, extracted hydrolysed and non-extracted hydrolysed samples proved useful to deduce the class of derivative from which the individual flavonoids have been released.

Keywords: Anthocyanidin; Arabidopsis thaliana; Deuterated internal standard; Flavonoids; Hydrolysis; LC-MS; Proanthocyanidin; Seed; Seedling.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Anthocyanins / metabolism
Arabidopsis / genetics
Arabidopsis / metabolism
Arabidopsis Proteins / genetics
Arabidopsis Proteins / metabolism
Chromatography, Liquid / methods*
Flavonoids / biosynthesis*
Gene Expression Regulation, Plant / genetics
Gene Expression Regulation, Plant / physiology
Mass Spectrometry / methods*
Seedlings / genetics
Seedlings / metabolism*

Substances

Anthocyanins
Arabidopsis Proteins
Flavonoids