In Vitro and In Vivo Human Metabolism of Synthetic Cannabinoids FDU-PB-22 and FUB-PB-22

In 2014, FDU-PB-22 and FUB-PB-22, two novel synthetic cannabinoids, were detected in herbal blends in Japan, Russia, and Germany and were quickly added to their scheduled drugs list. Unfortunately, no human metabolism data are currently available, making it challenging to confirm their intake. The p...

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Bibliographic Details
Published inThe AAPS journal Vol. 18; no. 2; pp. 455 - 464
Main Authors Diao, Xingxing, Scheidweiler, Karl B., Wohlfarth, Ariane, Pang, Shaokun, Kronstrand, Robert, Huestis, Marilyn A.
Format Journal Article
LanguageEnglish
Published New York Springer US 01.03.2016
Subjects
Biochemistry
Biomedical and Life Sciences
Biomedicine
Biotechnology
Cannabinoids - chemistry
Cannabinoids - pharmacology
Cannabinoids - urine
Hepatocytes - drug effects
Hepatocytes - metabolism
Humans
Microsomes, Liver - drug effects
Microsomes, Liver - metabolism
Pharmacology/Toxicology
Pharmacy
Plant Preparations - chemistry
Plant Preparations - pharmacology
Plant Preparations - urine
Research Article
high-resolution mass spectrometry
synthetic cannabinoid
FUB-PB-22
FDU-PB-22
hepatocyte metabolism
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Summary:In 2014, FDU-PB-22 and FUB-PB-22, two novel synthetic cannabinoids, were detected in herbal blends in Japan, Russia, and Germany and were quickly added to their scheduled drugs list. Unfortunately, no human metabolism data are currently available, making it challenging to confirm their intake. The present study aims to identify appropriate analytical markers by investigating FDU-PB-22 and FUB-PB-22 metabolism in human hepatocytes and confirm the results in authentic urine specimens. For metabolic stability, 1 μM FDU-PB-22 and FUB-PB-22 was incubated with human liver microsomes for up to 1 h; for metabolite profiling, 10 μM was incubated with human hepatocytes for 3 h. Two authentic urine specimens from FDU-PB-22 and FUB-PB-22 positive cases were analyzed after β-glucuronidase hydrolysis. Metabolite identification in hepatocyte samples and urine specimens was accomplished by high-resolution mass spectrometry using information-dependent acquisition. Both FDU-PB-22 and FUB-PB-22 were rapidly metabolized in HLM with half-lives of 12.4 and 11.5 min, respectively. In human hepatocyte samples, we identified seven metabolites for both compounds, generated by ester hydrolysis and further hydroxylation and/or glucuronidation. After ester hydrolysis, FDU-PB-22 and FUB-PB-22 yielded the same metabolite M7, fluorobenzylindole-3-carboxylic acid (FBI-COOH). M7 and M6 (hydroxylated FBI-COOH) were the major metabolites. In authentic urine specimens after β-glucuronidase hydrolysis, M6 and M7 also were the predominant metabolites. Based on our study, we recommend M6 (hydroxylated FBI-COOH) and M7 (FBI-COOH) as suitable urinary markers for documenting FDU-PB-22 and/or FUB-PB-22 intake.
ISSN:1550-7416
1550-7416
DOI:10.1208/s12248-016-9867-4