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Metabolic patterns of JWH‐210, RCS‐4, and THC in pig urine elucidated using LC‐HR‐MS/MS: Do they reflect patterns in humans?
Drug testing and analysis, 2017-04, Vol.9 (4), p.613-625
Schaefer, Nadine
Helfer, Andreas G.
Kettner, Mattias
Laschke, Matthias W.
Schlote, Julia
Ewald, Andreas H.
Meyer, Markus R.
Menger, Michael D.
Maurer, Hans H.
Schmidt, Peter H.
2017
Volltextzugriff (PDF)
Details
Autor(en) / Beteiligte
Schaefer, Nadine
Helfer, Andreas G.
Kettner, Mattias
Laschke, Matthias W.
Schlote, Julia
Ewald, Andreas H.
Meyer, Markus R.
Menger, Michael D.
Maurer, Hans H.
Schmidt, Peter H.
Titel
Metabolic patterns of JWH‐210, RCS‐4, and THC in pig urine elucidated using LC‐HR‐MS/MS: Do they reflect patterns in humans?
Ist Teil von
Drug testing and analysis, 2017-04, Vol.9 (4), p.613-625
Ort / Verlag
England: Wiley Subscription Services, Inc
Erscheinungsjahr
2017
Quelle
Wiley-Blackwell Journals
Beschreibungen/Notizen
The knowledge of pharmacokinetic (PK) properties of synthetic cannabinoids (SCs) is important for interpretation of analytical results found for example in intoxicated individuals. In the absence of human data from controlled studies, animal models elucidating SC PK have to be established. Pigs providing large biofluid sample volumes were tested for prediction of human PK data. In this context, the metabolic fate of two model SCs, namely 4‐ethylnaphthalen‐1‐yl‐(1‐pentylindol‐3‐yl)methanone (JWH‐210) and 2‐(4‐methoxyphenyl)‐1‐(1‐pentyl‐indol‐3‐yl)methanone (RCS‐4), was elucidated in addition to Δ9‐tetrahydrocannabinol (THC). After intravenous administration of the compounds, hourly collected pig urine was analyzed by liquid chromatography‐high resolution mass spectrometry. The following pathways were observed: for JWH‐210, hydroxylation at the ethyl side chain or pentyl chain and combinations of them followed by glucuronidation; for RCS‐4, hydroxylation at the methoxyphenyl moiety or pentyl chain followed by glucuronidation as well as O‐demethylation followed by glucuronidation or sulfation; for THC, THC glucuronidation, 11‐hydroxylation, followed by carboxylation and glucuronidation. For both SCs, parent compounds could not be detected in urine in contrast to THC. These results were consistent with those obtained from human hepatocyte and/or human case studies. Urinary markers for the consumption of JWH‐210 were the glucuronide of the N‐hydroxypentyl metabolite (detectable for 3–4 h) and of RCS‐4 the glucuronides of the N‐hydroxypentyl, hydroxy‐methoxyphenyl (detectable for at least 6 h), and the O‐demethyl‐hydroxy metabolites (detectable for 4 h). Copyright © 2016 John Wiley & Sons, Ltd. Observed metabolic pathways in pig urine were mono‐ and dihydroxylation followed by glucuronidation for JWH‐210; monohydroxylation followed by glucuronidation as well as O‐demethylation followed by glucuronidation or sulfation for RCS‐4; and for THC, THC glucuronidation, 11‐hydroxylation, followed by carboxylation and glucuronidation. The results found in pig urine are in accordance to those obtained from human hepatocyte and/or human case studies.
Sprache
Englisch
Identifikatoren
ISSN: 1942-7603
eISSN: 1942-7611
DOI: 10.1002/dta.1995
Titel-ID: cdi_proquest_journals_1886231565
Format
–
Schlagworte
Animals
,
Cannabinoids - metabolism
,
Cannabinoids - urine
,
Chromatography, Liquid - methods
,
Dronabinol - metabolism
,
Dronabinol - urine
,
Humans
,
Indoles - metabolism
,
Indoles - urine
,
LC‐HR‐MS/MS
,
Naphthalenes - metabolism
,
Naphthalenes - urine
,
pigs
,
Psychotropic Drugs - metabolism
,
Psychotropic Drugs - urine
,
Street Drugs - metabolism
,
Street Drugs - urine
,
Substance Abuse Detection - methods
,
Swine - metabolism
,
Swine - urine
,
synthetic cannabinoids
,
Tandem Mass Spectrometry - methods
,
tetrahydrocannabinol
,
urinary metabolic patterns
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