JWH-210 Wikipedia: Difference between revisions

Latest revision as of 09:31, 24 May 2026

High resolution mass spectrometry such as LC-QTOF-MS allows the detection and identification of a broad spectrum of recreational drugs, including new psychoactive substances. A point-of-care drugs of abuse (DOA) test was initially performed on the urine of the patient. He confirmed drinking 750 ml energy drink without any further consumption of food and using an e-cigarette from Gaziantep, Turkey 10 seconds before the onset of his first symptoms. He usually smokes a pack of cigarettes a day and sometimes smokes e-cigarettes. Combined with non-specific, transient symptoms, clinical recognition of SCRA intoxication is challenging .
Data availability
The intensity is plotted against the retention time for both chromatograms, demonstrating the JWH-210 powder presence and elution profiles of nicotine and ADB-BUTINACA in the analysed vape liquid sample. LC-QTOF-MS Chromatograms of Nicotine (Top) and ADB-BUTINACA (Bottom) in the Vape Liquid used by the patient. The LC-QTOF-MS analysis showed that the e-liquid contained nicotine and ADB-BUTINACA (Fig. 1). Because the point-of-care DOA test is generally not able to detect synthetic recreational drug substances, the liquid of the e-cigarette was thereafter screened using liquid chromatography-quadrupole time-of-flight mass spectrometry (LC-QTOF-MS) on the Waters™ Xevo G3 QTOF MS system. After eating a light meal and drinking caffeinated sports drinks at the ER, the nausea complaints of the patient were reduced and the patient was discharged hom

The findings produce an apparent paradox, since CPP and self-administration predict with high reliability the likelihood that a compound will be abused by humans, and cannabinoids are well-known to produce active drug-seeking in human

The same procedure was then applied to the mice once every day for 5 days. It was considered as coordination disturbance when mice fell from the test apparatus within 2 min. Mice that remained their position on the running apparatus at 10 rpm for at least 2 min were selected for further evaluation.
Table of Conten

Eight in-vivo metabolites tentatively identified were mainly products of ester hydrolysis with or without additional dehydrogenation, N-dealkylation, monohydroxylation and oxidative defluorination with further oxidation to butanoic aci

A limitation of this case report is that we did not have a urine sample available for additional NPS testing. Point-of-care DOA tests using urine to screen for misuse of multiple substances, regularly include cannabis, amphetamines, cocaine, opioids, benzodiazepines and methadone. THC, methamphetamine, SRCA, lysergic acid diethylamide (LSD), gamma-hydroxybutyrate (GHB) and ketamine are likely to become volatile under the temperature of current e-cigarettes, while crack cocaine is hard to vaporise. A systematic review including data of 114 patients of which the majority was intoxicated due to SCRA smoking revealed that 45 % of the patients who present at the ER after an intoxication due to SCRA smoking recovered within 24 hours

Product ions detected at m/z 302, 217, and 145 (B2) confirmed that tert-leucine and indazole moieties remained unchanged, leading to the structure elucidation of a hydroxy-functional group at the 4-position of the butyl side chain by oxidative defluorination. The product ion m/z 336 (loss of methyl ester moiety) further confirmed the presence of dihydroxylated metabolites. The precursor ion, m/z 364 (B14, B5/B6) had a loss of 2 Da from m/z 366 indicated further dehydrogenation of the ester hydrolysis plus monohydroxylated metabolites. The presence of the product ion m/z 320, likely formed from a loss of carbon dioxide, indicated monohydroxylation at the tert-leucine in B8 (m/z 219), butyl side chain in B9 (m/z 145) and indazole moiety in B13 (m/z 161). The precursor ion, m/z 350 showed a loss of 14 Da explaining the hydrolysis of methyl ester from 4F-MDMB-BINACA.
Fig. 2.
The precursor ion m/z 396 (B10, B12/B15) was 32 Da higher than the parent drug, 4F-MDMB-BINACA, suggesting the addition of two hydroxy groups. All the below explanations for transformations into metabolites are based on the data shown in Fig. Metabolites were identified according to their precursor ions, product ions, and fragmentation patterns (Fig. 1). Traditional in-vivo metabolism studies to generate human metabolites of drugs relied heavily on the use of whole animal model systems, which are expensive, limited by drug administration amount, influenced by species variation and faced by many ethical issues. Eight in-vivo metabolites tentatively identified were mainly products of ester hydrolysis with or without additional dehydrogenation, N-dealkylation, monohydroxylation and oxidative defluorination with further oxidation to butanoic acid.
Fig. 1.
This outcome was anticipated since CES-mediated hydrolysis is commonly JWH-210 powder reported as the major metabolic pathway among the SCBs impacting the terminal ester group . Glucosides and sulfate metabolites have been reported with other SCBs where C. From these three samples, sample 2 contained only an ester hydrolysis metabolite (m/z 350). Both ester hydrolysis followed by oxidative defluorination to butanoic acid (B4, m/z 362) and monohydroxylation at tert-leucine moiety (B8, m/z 366) metabolites were found in 16/20 urine samples (Table 2). A In-vitro metabolites observed in common among respective seven most abundant metabolites in b C. The product ion detected at m/z 235, indicating loss of sulfate, confirmed the identity of the sulfation metabolite.
Fungus C. elegans
Concentrations of 4F-MDMB-BINACA in the postmortem blood samples were 2.50 and 2.34 ng/mL, which are in line with published data. Although the lethal dose of 4F-MDMB-BINACA is unknown, its concentration in postmortem blood samples was found to range between 0.10 and 2.90 ng/mL . In SCRA-related cases in which the deceased suffered from heart disease, the SCRA concentration in the postmortem blood was less than 1 ng/mL . Concentrations of SCRAs in postmortem cases cover a wide range ; however, some reports of survival have also been published—even at relatively high blood SCRA concentrations [19, 20

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	~~Figure 1. <br>These synthetic cannabinoids act directly at cannabinoid CB1 and CB2 receptors~~ as ~~does Δ9~~-~~tetrahydrocannabinol (Δ9~~-~~THC) found in marijuana, but have different chemical structures unrelated to Δ9-THC, different metabolism,~~ and ~~often greater toxicity (Fantegrossi et al.~~, ~~2014)~~. ~~Discriminative stimulus effects were tested in rats trained to discriminate Δ9~~-~~tetrahydrocannabinol (3 mg/kg, 30~~-min pretreatment). 5F-MDMB-PINACA (also known as 5F-ADB, 5F-ADB-PINACA), MDMB-CHIMICA, MDMB-FUBINACA, ADB-FUBINACA, and AMB-FUBINACA (also known as FUB-AMB, MMB-FUBINACA) were tested for in vivo cannabinoid-like effects to assess their abuse ~~liabilit<br><br><br>Some mice showed abnormal behaviors~~ (~~catalepsy, loss of traction, convulsion~~) ~~right after~~ the ~~administration~~ of the ~~tested substances~~. ~~The locomotor activity~~ of ~~the mice was measured 30 min~~ and ~~2 hrs after the last substance administration. We also examined their neurotoxicity~~ using ~~brain samples through histopathological diagnose~~, ~~especially in~~ the ~~nucleus accumbens core region~~. ~~In histopathological analysis, neural cells~~ of ~~the animals treated~~ with ~~the high dose (5 mg/kg) of JWH~~-~~081 or JWH-210 showed distorted nuclei and nucleus membranes in the core shell~~ of ~~nucleus accumbens, suggesting neurotoxicity~~.<br>~~Table of Conten~~<br>~~<br><br>Tremors were observed in mice 30 minutes following 1 mg~~/~~kg AMB~~-~~FUBINACA in the present study~~. ~~Pretreatment times~~ and ~~dose ranges for the drug discrimination assay were selected based on the time~~ of ~~peak depression~~ in the ~~locomotor activity assay in mice~~. ~~Average potency~~ of ~~the discriminative stimulus effects of early compounds was 0.81±0.17 mg/kg~~ (~~Gatch et al., 2014~~)~~, whereas the potency of a recent set was 0.09±0.03 mg/kg~~ (~~Gatch et al., 2018~~)~~, and~~ the ~~potency of~~ the current set is 0.05±0.01 mg/kg. Short-onset, short-acting compounds have a greater abuse liability, and long-acting compounds pose problems of long-acting adverse effects and interactions with other drugs. The duration of action of the synthetic cannabinoids tested using the 8-h protocol have varied widely, with some producing a duration of action no longer than 1 h, others producing a duration of action between 1–2 h, and others lasting more than 2 h. There seems to be a trend of newer synthetic cannabinoids being more potent than earlier compound<br><br><br>LC-QTOF-MS ~~represents a significant advancement in~~ the ~~field of drug detection, offering higher sensitivity, specificity,~~ and ~~a broader spectrum of detectable substances~~. ~~Despite all negative results in~~ the point-of-care test ~~for~~ recreational ~~drugs~~, the liquid chromatography-quadrupole time-of-flight mass spectrometry (LC-QTOF-MS) ~~analysis showed that~~ the ~~liquid of the e-cigarette contained ADB-BUTINACA, a synthetic cannabinoid~~. ~~We report~~ a ~~27-year-old man who was admitted to~~ the ~~emergency room because of sudden 4F ADB headache~~, nausea~~, vertigo, red eyes~~ and ~~palpitations. Synthetic cannabinoids are gaining popularity globally and detection is not commonly available.~~<br>~~Data availability~~ <br>~~When clinical presentation~~ and~~/or initial DOA testing results are inconclusive, additional testing~~ with ~~LC-QTOF-MS can~~ be ~~valuable and is recommended. SCRAs and other NPS may not be detected~~ by ~~point-of-care DOA tests. In this case~~, ~~the point~~-~~of-care DOA urine screening was not able~~ to ~~detect the synthetic cannabinoid ADB~~-~~BUTINAC~~<br><br><br>~~Test 2~~ was ~~performed everyday~~ for 5 days ~~after consecutive administration of the substances, including negative (vehicle) and positive (methamphetamine) controls~~. ~~After the last administration, the first trial~~ was ~~performed. Morris water maze test was performed to evaluate the changes of learning and memory function through administration of~~ the test ~~substances. Generally, neurotoxicity of a substance is evaluated by animal behavioral aspects, i.e~~. ~~functional observation battery (FOB) tests (O’Callaghan et al., 2014). Our results suggest~~ that ~~JWH-081 and JWH-210 may [https://cannabinoidsrc4f-adb~~.~~com/ 4F ADB] be neurotoxic substances through changing neuronal cell damages, especially in the core shell part~~ of ~~nucleus accumbens.~~<br>~~About Powder JWH~~-2<br><br><br>~~Acute kidney damage and even kidney failure~~ have ~~been reported following use~~ of ~~synthetic cannabinoids (Davidson~~, ~~et al~~., ~~2017~~)~~. One recent study has looked at other mechanisms of action in some of the older synthetic cannabinoids~~ and ~~reported that some produced varying amounts of activity at sites which~~ are ~~related~~ to ~~cardiotoxicity and heart disease (Wiley et al.~~, ~~2016). It is not known whether the increased toxicity~~ is ~~due only~~ to ~~activation of CB1 cannabinoid receptors more strongly than Δ9-THC or whether these "super-strength" cannabinoids produce effects at other receptors~~. A ~~major cause~~ of ~~concern is~~ that ~~some~~ of the ~~more recently seen synthetic cannabinoids are more likely~~ to ~~produce extremely toxic effects than the older synthetics (Tai and Fantegrossi, 2017~~<br><br><br>~~Due~~ to the ~~unknown toxicity~~ of ~~newly emerging SCRAs, forensic assessments~~ of ~~cases involving these substances are challenging~~. ~~According to~~ the ~~reported cases and reviews~~ of ~~the scientific literature~~, ~~concurrent ethanol consumption should amplify~~ the ~~toxicity of SCRAs~~. The ~~concentration~~ of 4F-~~MDMB-BINACA~~ in ~~the postmortem blood was 2.50 and 2.34 ng~~/mL, and ~~blood alcohol concentration was 2~~.~~11 and 2.49 g~~/~~L, respectively. Two fatal cases are reported caused by simultaneous consumption~~ of 4F-MDMB-BINACA ~~and ethanol~~.<br>Fig. 2. <br>~~4F-MDMB-BINACA~~ was ~~hydrolysed via ester hydrolysis forming~~ the 4F-MDMB-BINACA ~~ester hydrolysis metabolite (B22)~~. ~~Data obtained from~~ the ~~twenty urine samples were retrospectively analysed and processed using TraceFinder software~~ based on the ~~identification criteria of mass errors less than ± 5 ppm for full MS peaks~~ and ~~MS/MS peaks from the theoretical mass and matching of MS/MS spectra~~. ~~The mixture was vortex~~-~~mixed and 500 µL~~ of ~~this mixture and 500 µL~~ of ~~methanol were loaded onto the Clean Screen FASt® tube. After incubation~~, ~~the mixture was cooled at room temperature~~, and ~~150 µL of purified water was added~~. ~~High~~-~~resolution QTOF-MS data~~ were ~~acquired on an Agilent 6510 Accurate Mass QTOF mass spectrometer (Agilent Technologies) equipped~~ with ~~dual electrospray ionization (ESI) source operated in both positive and negative ion modes~~, ~~to determine accurate masses of the metabolites. Chromatographic separation was performed on an Agilent 1290 LC system with a Poroshell 120 EC~~-~~C18 analytical column (2.7 μm~~, ~~75 × 2.1 mm; Agilent Technologies, Santa Clara, CA, USA)~~.<br>Fig. 1. <br>This outcome was anticipated since CES-mediated hydrolysis is commonly ~~4F ADB~~ reported as the major metabolic pathway among the SCBs impacting the terminal ester group . Glucosides and sulfate metabolites have been reported with other SCBs where C. From these three samples, sample 2 contained only an ester hydrolysis metabolite (m/z 350). Both ester hydrolysis followed by oxidative defluorination to butanoic acid (B4, m/z 362) and monohydroxylation at tert-leucine moiety (B8, m/z 366) metabolites were found in 16/20 urine samples (Table 2). A In-vitro metabolites observed in common among respective seven most abundant metabolites in b C. The product ion detected at m/z 235, indicating loss of sulfate, confirmed the identity of the sulfation metabolite.<br>Fungus C. elegans <br>Concentrations of 4F-MDMB-BINACA in the postmortem blood samples were 2.50 and 2.34 ng/mL, which are in line with published data. Although the lethal dose of 4F-MDMB-BINACA is unknown, its concentration in postmortem blood samples was found to range between 0.10 and 2.90 ng/mL . In SCRA-related cases in which the deceased suffered from heart disease, the SCRA concentration in the postmortem blood was less than 1 ng/mL . Concentrations of SCRAs in postmortem cases cover a wide range ; however, some reports of survival have also been published—even at relatively high blood SCRA concentrations [19, 20		High resolution mass spectrometry such as LC-QTOF-MS allows the detection and identification of a broad spectrum of recreational drugs, including new psychoactive substances. A point-of-care drugs of abuse (DOA) test was initially performed on the urine of the patient. He confirmed drinking 750 ml energy drink without any further consumption of food and using an e-cigarette from Gaziantep, Turkey 10 seconds before the onset of his first symptoms. He usually smokes a pack of cigarettes a day and sometimes smokes e-cigarettes. Combined with non-specific, transient symptoms, clinical recognition of SCRA intoxication is challenging .<br>Data availability <br>The intensity is plotted against the retention time for both chromatograms, demonstrating the [https://cannabinoidsrc4f-adb.com/ JWH-210 powder] presence and elution profiles of nicotine and ADB-BUTINACA in the analysed vape liquid sample. LC-QTOF-MS Chromatograms of Nicotine (Top) and ADB-BUTINACA (Bottom) in the Vape Liquid used by the patient. The LC-QTOF-MS analysis showed that the e-liquid contained nicotine and ADB-BUTINACA (Fig. 1). Because the point-of-care DOA test is generally not able to detect synthetic recreational drug substances, the liquid of the e-cigarette was thereafter screened using liquid chromatography-quadrupole time-of-flight mass spectrometry (LC-QTOF-MS) on the Waters™ Xevo G3 QTOF MS system. After eating a light meal and drinking caffeinated sports drinks at the ER, the nausea complaints of the patient were reduced and the patient was discharged hom<br><br>The findings produce an apparent paradox, since CPP and self-administration predict with high reliability the likelihood that a compound will be abused by humans, and cannabinoids are well-known to produce active drug-seeking in human<br><br><br>The same procedure was then applied to the mice once every day for 5 days. It was considered as coordination disturbance when mice fell from the test apparatus within 2 min. Mice that remained their position on the running apparatus at 10 rpm for at least 2 min were selected for further evaluation.<br>Table of Conten<br><br>Eight in-vivo metabolites tentatively identified were mainly products of ester hydrolysis with or without additional dehydrogenation, N-dealkylation, monohydroxylation and oxidative defluorination with further oxidation to butanoic aci<br><br><br>A limitation of this case report is that we did not have a urine sample available for additional NPS testing. Point-of-care DOA tests using urine to screen for misuse of multiple substances, regularly include cannabis, amphetamines, cocaine, opioids, benzodiazepines and methadone. THC, methamphetamine, SRCA, lysergic acid diethylamide (LSD), gamma-hydroxybutyrate (GHB) and ketamine are likely to become volatile under the temperature of current e-cigarettes, while crack cocaine is hard to vaporise. A systematic review including data of 114 patients of which the majority was intoxicated due to SCRA smoking revealed that 45 % of the patients who present at the ER after an intoxication due to SCRA smoking recovered within 24 hours<br><br><br>Product ions detected at m/z 302, 217, and 145 (B2) confirmed that tert-leucine and indazole moieties remained unchanged, leading to the structure elucidation of a hydroxy-functional group at the 4-position of the butyl side chain by oxidative defluorination. The product ion m/z 336 (loss of methyl ester moiety) further confirmed the presence of dihydroxylated metabolites. The precursor ion, m/z 364 (B14, B5/B6) had a loss of 2 Da from m/z 366 indicated further dehydrogenation of the ester hydrolysis plus monohydroxylated metabolites. The presence of the product ion m/z 320, likely formed from a loss of carbon dioxide, indicated monohydroxylation at the tert-leucine in B8 (m/z 219), butyl side chain in B9 (m/z 145) and indazole moiety in B13 (m/z 161). The precursor ion, m/z 350 showed a loss of 14 Da explaining the hydrolysis of methyl ester from 4F-MDMB-BINACA.<br>Fig. 2. <br>The precursor ion m/z 396 (B10, B12/B15) was 32 Da higher than the parent drug, 4F-MDMB-BINACA, suggesting the addition of two hydroxy groups. All the below explanations for transformations into metabolites are based on the data shown in Fig. Metabolites were identified according to their precursor ions, product ions, and fragmentation patterns (Fig. 1). Traditional in-vivo metabolism studies to generate human metabolites of drugs relied heavily on the use of whole animal model systems, which are expensive, limited by drug administration amount, influenced by species variation and faced by many ethical issues. Eight in-vivo metabolites tentatively identified were mainly products of ester hydrolysis with or without additional dehydrogenation, N-dealkylation, monohydroxylation and oxidative defluorination with further oxidation to butanoic acid.<br>Fig. 1. <br>This outcome was anticipated since CES-mediated hydrolysis is commonly JWH-210 powder reported as the major metabolic pathway among the SCBs impacting the terminal ester group . Glucosides and sulfate metabolites have been reported with other SCBs where C. From these three samples, sample 2 contained only an ester hydrolysis metabolite (m/z 350). Both ester hydrolysis followed by oxidative defluorination to butanoic acid (B4, m/z 362) and monohydroxylation at tert-leucine moiety (B8, m/z 366) metabolites were found in 16/20 urine samples (Table 2). A In-vitro metabolites observed in common among respective seven most abundant metabolites in b C. The product ion detected at m/z 235, indicating loss of sulfate, confirmed the identity of the sulfation metabolite.<br>Fungus C. elegans <br>Concentrations of 4F-MDMB-BINACA in the postmortem blood samples were 2.50 and 2.34 ng/mL, which are in line with published data. Although the lethal dose of 4F-MDMB-BINACA is unknown, its concentration in postmortem blood samples was found to range between 0.10 and 2.90 ng/mL . In SCRA-related cases in which the deceased suffered from heart disease, the SCRA concentration in the postmortem blood was less than 1 ng/mL . Concentrations of SCRAs in postmortem cases cover a wide range ; however, some reports of survival have also been published—even at relatively high blood SCRA concentrations [19, 20