Profiling of pyrrolizidine alkaloids using a retronecine-based untargeted metabolomics approach coupled to the quantitation of the retronecine-core in medicinal plants using UHPLC-QTOF

Evangelia Tsiokanos; Nikolaos Tsafantakis; Hélène Obé; Till Beuerle; Mathieu Leti; Nikolas Fokialakis; Antonio Grondin

doi:10.1016/j.jpba.2022.115171

Profiling of pyrrolizidine alkaloids using a retronecine-based untargeted metabolomics approach coupled to the quantitation of the retronecine-core in medicinal plants using UHPLC-QTOF

J Pharm Biomed Anal. 2023 Feb 5:224:115171. doi: 10.1016/j.jpba.2022.115171. Epub 2022 Nov 21.

Authors

Evangelia Tsiokanos¹, Nikolaos Tsafantakis², Hélène Obé³, Till Beuerle⁴, Mathieu Leti⁵, Nikolas Fokialakis⁶, Antonio Grondin⁷

Affiliations

¹ Department of Pharmacognosy and Natural Products Chemistry, Faculty of Pharmacy, National and Kapodistrian University of Athens, 15771 Athens, Greece. Electronic address: evatsiokanos@pharm.uoa.gr.
² Department of Pharmacognosy and Natural Products Chemistry, Faculty of Pharmacy, National and Kapodistrian University of Athens, 15771 Athens, Greece. Electronic address: ntsafantakis@pharm.uoa.gr.
³ Pierre Fabre Research Institute, Green Mission Department, Herbal Products Laboratory, 3, Avenue Hubert Curien, BP 13562, 31035 Toulouse, France. Electronic address: helene.vercauteren@pierre-fabre.com.
⁴ Department of Pharmaceutical Biology, Technical University of Braunschweig, Mendelssohnstr. 1, 38106 Braunschweig, Germany. Electronic address: t.beuerle@tu-braunschweig.de.
⁵ Pierre Fabre Research Institute, Green Mission Department, Herbal Products Laboratory, 3, Avenue Hubert Curien, BP 13562, 31035 Toulouse, France. Electronic address: mathieu.leti@pierre-fabre.com.
⁶ Department of Pharmacognosy and Natural Products Chemistry, Faculty of Pharmacy, National and Kapodistrian University of Athens, 15771 Athens, Greece. Electronic address: fokialakis@pharm.uoa.gr.
⁷ Pierre Fabre Research Institute, Green Mission Department, Herbal Products Laboratory, 3, Avenue Hubert Curien, BP 13562, 31035 Toulouse, France. Electronic address: antonio.grondin@pierre-fabre.com.

PMID: 36459765
DOI: 10.1016/j.jpba.2022.115171

Abstract

Pyrrolizidine alkaloids (PA) are secondary metabolites of high toxicological relevance. Several PA quantitative methodologies were developed based on a limited number of certified standards, including time consuming solid phase extraction (SPE) purification steps. Herein, we shed light on the variability of PA in herbal extracts and propose a quantification methodology based on ultra-high-performance liquid chromatography high-resolution mass spectrometry (UHPLC-HRMS) for the evaluation of the total PA content as retronecine-equivalents (RE) directly from crude matrices. Particularly in the focus of the investigation were Alkanna spp. (Boraginaceae), which possess a wide range of pharmaceutical properties. In addition, a comparative PA screening of crude and SPE enriched extracts was performed and PA-containing plants from Fabaceae and Compositae families were included to demonstrate universal applicability. In total, 105 PA were identified using HRMS^e experiments, specific MS/MS fragmentation PA patterns, a customized in-house library and literature data. Among them, 18 glycosidic PA derivatives were reported for the first time in literature. Using a hierarchical clustering approach, PA distribution in herbal extracts was shown to be family-dependent and significantly different among species. This was further supported by the results of the total PA concentrations, obtained using a retronecine/heliotridine/internal standard-based targeted UHPLC-HRMS quantification method, which varied from 8.64 ± 0.08-3096.28 ± 273.72 μg RE/g extract dry weight in shoots extracts of Alkanna spp. and leaves extracts of Crotalaria retusa L. respectively. Worth mentioning is that the procedure allowed to quantify PA in Alkanna spp. If the procedure based on 35 specific PA recommended by European regulations had been used, results would have been equal to zero for the four species since none were observed in Alkanna spp. Finally, by combining the RE results with the corresponding dereplication results, a customized correction factor for each extract (ranging from 2.12 to 2.48) was assessed leading to a more accurate estimate of the PA content regardless of the molecular weight of each PA. The present methodology will facilitate PA quantification directly from crude extracts and avoid the underestimation the real PA content due to limited availabilty of authentic reference compounds in botanical extracts used in phytomedicines or food supplements/cosmetics.

Keywords: Alkanna; Metabolomics; Profiling; Pyrrolizidine alkaloids; Retronecine; UHPLC-HRMS quantification.

MeSH terms

Chromatography, High Pressure Liquid / methods
Humans
Plants, Medicinal*
Pyrrolizidine Alkaloids* / analysis
Tandem Mass Spectrometry / methods

Substances

retronecine
Pyrrolizidine Alkaloids