Activity-based detection of synthetic cannabinoid receptor agonists in plant materials

Axelle Timmerman; Margot Balcaen; Vera Coopman; Maarten Degreef; Eline Pottie; Christophe P. Stove

doi:10.1186/s12954-024-01044-4

Harm Reduction Journal (Jul 2024)

Activity-based detection of synthetic cannabinoid receptor agonists in plant materials

Axelle Timmerman,
Margot Balcaen,
Vera Coopman,
Maarten Degreef,
Eline Pottie,
Christophe P. Stove

Affiliations

Axelle Timmerman: Laboratory of Toxicology, Department of Bioanalysis, Faculty of Pharmaceutical Sciences, Ghent University
Margot Balcaen: Belgian Early Warning System on Drugs
Vera Coopman: Eurofins Forensics Belgium
Maarten Degreef: Belgian Early Warning System on Drugs
Eline Pottie: Laboratory of Toxicology, Department of Bioanalysis, Faculty of Pharmaceutical Sciences, Ghent University
Christophe P. Stove: Laboratory of Toxicology, Department of Bioanalysis, Faculty of Pharmaceutical Sciences, Ghent University

DOI: https://doi.org/10.1186/s12954-024-01044-4
Journal volume & issue: Vol. 21, no. 1
pp. 1 – 11

Abstract

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Abstract Background Since late 2019, fortification of ‘regular’ cannabis plant material with synthetic cannabinoid receptor agonists (SCRAs) has become a notable phenomenon on the drug market. As many SCRAs pose a higher health risk than genuine cannabis, recognizing SCRA-adulterated cannabis is important from a harm reduction perspective. However, this is not always an easy task as adulterated cannabis may only be distinguished from genuine cannabis by dedicated, often expensive and time-consuming analytical techniques. In addition, the dynamic nature of the SCRA market renders identification of fortified samples a challenging task. Therefore, we established and applied an in vitro cannabinoid receptor 1 (CB1) activity-based procedure to screen plant material for the presence of SCRAs. Methods The assay principle relies on the functional complementation of a split-nanoluciferase following recruitment of β-arrestin 2 to activated CB1. A straightforward sample preparation, encompassing methanolic extraction and dilution, was optimized for plant matrices, including cannabis, spiked with 5 µg/mg of the SCRA CP55,940. Results The bioassay successfully detected all samples of a set (n = 24) of analytically confirmed authentic Spice products, additionally providing relevant information on the ‘strength’ of a preparation and whether different samples may have originated from separate batches or possibly the same production batch. Finally, the methodology was applied to assess the occurrence of SCRA adulteration in a large set (n = 252) of herbal materials collected at an international dance festival. This did not reveal any positives, i.e. there were no samples that yielded a relevant CB1 activation. Conclusion In summary, we established SCRA screening of herbal materials as a new application for the activity-based CB1 bioassay. The simplicity of the sample preparation, the rapid results and the universal character of the bioassay render it an effective and future-proof tool for evaluating herbal materials for the presence of SCRAs, which is relevant in the context of harm reduction.

Published in Harm Reduction Journal

ISSN: 1477-7517 (Online)
Publisher: BMC
Country of publisher: United Kingdom
LCC subjects: Medicine: Public aspects of medicine
Website: http://harmreductionjournal.biomedcentral.com

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