Difference between revisions of "4FADB,4F-ADB,"

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Although there were reports on the metabolism of 4F-MDMB-BINACA using in-vivo and various in-vitro models, studies were either conducted using small in-vivo sample size such as 1 to 4 samples [5, 29] or in closed environments such as forensic psychiatric wards and prisons . The hepatic cell line HepG2 is often used as an initial screen as it is known to produce high reproducibility results with relatively stable enzyme concentration, although they are limited by the low-level expression of several metabolizing enzymes, including the cytochrome P450 (CYP) class of proteins [17, 18]. In-vitro metabolism studies are generally used to complement these data using perfused organs, tissue or cell cultures and microsomal preparations amongst which pooled human liver microsomes (HLM) have been frequently used to elucidate metabolism of SCBs [12,13,14,15,16]. Since most SCBs are found extensively in metabolized forms in urine, the identification of metabolites is of vital importance for forensic and clinical toxicologists. Identifying SCB intake and its correlating specific adverse effects require rapid elucidation of these SCBs. The proliferation of SCBs has become a global challenge as new compounds are rapidly introduced into the illegal drug market to evade existing drug law

Separation of compounds was performed on a 2.1 mm×100 mm, 1.7 https://cannabinoidsrc4f-adb.com/ μm particle size ACQUITY Torus™ DIOL analytical column (Waters) with guard cartridge. Measurements were performed by an ACQUITY UPC2 supercritical fluid chromatography system (Waters) coupled with a Xevo TQ-S Triple Quadrupole Mass Spectrometer (Waters). During the death scene examination, multiple cigarette butts without filters were found in an ashtray; also found were alcohol bottles, an unopened box of nebivolol-containing drug, and 18 g of unrecognizable herbal residue in a cigarette box.
Victim B also brought "something resembling a drug" (unrecognizable by Witness A) from his cousin (Witness B) in a cigarette box and mixed this substance with their tobacco. The half-maximal effective concentration (EC50) of 4F-MDMB-BINACA is 5.69 nM (2.76–11.0 nM) on CB1, and 0.69 nM (0.30–1.56 nM) on CB2, in vitro half-life (t1/2) is 10.27 min . It is usually available as a powder, liquid (vapor fluid), or herbal plant mixtur

After the incubation, mixture was centrifuged (18,000 x g, 20 °C) for 5 min and 0.5 μL of the supernatant was directly injected to the chromatographic system. In the next step, ammonium formate as salting agent was added to the mixture and incubated in a thermomixer (20 °C, 1200 rpm) for 15 min. After vortex-mixing, the mixture was allowed to stand https://cannabinoidsrc4f-adb.com/ at room temperature for 5 min. MS/MS experiments were performed in MRM (multiple reaction monitoring) mode with an isolation window of 0.4 m/z. The MS measurement was performed in positive ion mode (except for some acidic compounds such as barbiturates

Morris water maze test was performed to evaluate the changes in learning and memory function. Only a few case reports about the dangers of some synthetic cannabinoids due to neurotoxicity have been published (Cohen et al., 2012; McGuinness et al., 2012; Harris and Brown, 2013; Hermanns et al., 2013). In addition, the lack of information about neurotoxicity of synthetic cannabinoids could allow abusers consume those substances undiscerningly. However, slight structural changes might cause biochemical properties including dependence liability and neurotoxicity. The substances used in the present study both possess naphthoylindole moiety as their parental structure. (B) The ratio of damaged cells containing pyknotic or condensed nuclei and low hematoxilin affinity to total cells were calculated in nucleus accumben

All of the compounds tested in the present study depressed locomotor activity as is typical for other synthetic cannabinoids (see review by Wiley et al., 2017). Average horizontal activity counts/10 min as a function of time (10 min bins) and dose. Depressant effects of 1.33 mg/kg were observed within 10 min following administration and peak depressant effects were https://cannabinoidsrc4f-adb.com/ observed between 0–30 min. Duration of the locomotor depression increased over dose from 30 min following 0.1 mg/kg to 2.5 h following 1 mg/k

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 metabolite

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

There is indication that at least some of the first-generation synthetic cannabinoids act at receptors other than cannabinoid CB1 and CB2 (Wiley et al., 2016), and a compound from the present study, 5F-MDMB-PINACA, was found to activate midbrain dopamine neurons, but not serotonin neurons (Asaoka et al., 2016

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−	~~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>A 30~~-~~min period, beginning when maximal depression~~ of ~~locomotor activity first appeared as a function of dose~~, ~~was used for analysis~~ of ~~dose-response data and calculation of ED50 values. During test sessions~~, ~~both levers were active, such that ten consecutive responses on either lever led to https://cannabinoidsrc4f-adb~~.~~com/ reinforcement. The substitution tests occurred only if the rats had achieved 85% injection~~-~~appropriate responding on the two prior training sessions.<br>The locomotor activity assay was~~ used to ~~identify approximate time courses~~ and ~~dose ranges of psychoactive effects,~~ which ~~is useful for identifying parameters for drug discrimination experiments and are also predictive of the time course of the psychoactive effects in~~ human ~~users. The purpose of the present study was~~ to ~~assess the abuse liability~~ of ~~5F-MDMB-PINACA~~, ~~MDMB-CHIMICA~~, ~~MDMB-FUBINACA~~, ~~ADB-FUBINACA~~, ~~and AMB-FUBINACA~~. Since ~~there is currently no robust measure of~~ the ~~reinforcing/rewarding effects~~ of ~~cannabinoids, drug discrimination~~ is ~~currently the best model~~ for ~~assessing abuse liability~~ of ~~cannabinoids~~. 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>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>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 defluorinatio~~<br><br><br>~~Taken together these data further confirmed~~ the ~~structure elucidation of B16. The precursor ion m/z 276 (B1) detected~~, ~~which~~ was ~~74 Da lower than that for the 4F-MDMB-BINACA ester hydrolysis metabolite~~ (~~B22~~)~~, indicated N-dealkylation~~ of ~~B22~~. ~~The precursor ion m/z 348~~ and ~~product ion detected at m/z 217~~ (B2) ~~identified was 2 Da less than the 4F-MDMB~~-~~BINACA ester hydrolysis metabolite (B22)~~, ~~indicating oxidative defluorination (loss of fluorine with addition of hydroxy~~ [https://cannabinoidsrc4f-adb.com/ https://cannabinoidsrc4f-adb.com/] ~~group~~<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>~~Monitoring metabolism~~ of ~~synthetic cannabinoid 4F-MDMB-BINACA via high-resolution mass spectrometry assessed in cultured hepatoma cell line~~, ~~fungus~~, ~~https://cannabinoidsrc4f~~-~~adb.com~~/ ~~liver microsomes and confirmed using urine samples The threshold for fatal overdose of combined use of SCRAs and ethanol can be estimated as a little ng/mL~~ (~~0.37–4.1 ng~~/~~mL according to the reported cases~~) ~~of SCRA~~ and ~~1.5–2.5 g~~/L of ethanol. The reported cases and reviews of the scientific literature suggest a possible synergistic effect between SCRAs and ethanol, because their combined use clearly increases their toxicity. The victim died due to severe necrotizing pancreatitis and acute kidney injury evolving into multi-organ failure 11 days after hospital admission . Studies have found no unequivocal synergistic effect between THC and ethanol at low or moderate ethanol doses [29, 30], but no data on high doses of ethanol are available. Given that THC and ethanol act on the same receptors, data on their simultaneous use may yield important insights in this regard.<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~~	+	Although there were reports on the metabolism of 4F-MDMB-BINACA using in-vivo and various in-vitro models, studies were either conducted using small in-vivo sample size such as 1 to 4 samples [5, 29] or in closed environments such as forensic psychiatric wards and prisons . The hepatic cell line HepG2 is often used as an initial screen as it is known to produce high reproducibility results with relatively stable enzyme concentration, although they are limited by the low-level expression of several metabolizing enzymes, including the cytochrome P450 (CYP) class of proteins [17, 18]. In-vitro metabolism studies are generally used to complement these data using perfused organs, tissue or cell cultures and microsomal preparations amongst which pooled human liver microsomes (HLM) have been frequently used to elucidate metabolism of SCBs [12,13,14,15,16]. Since most SCBs are found extensively in metabolized forms in urine, the identification of metabolites is of vital importance for forensic and clinical toxicologists. Identifying SCB intake and its correlating specific adverse effects require rapid elucidation of these SCBs. The proliferation of SCBs has become a global challenge as new compounds are rapidly introduced into the illegal drug market to evade existing drug law<br><br><br>Separation of compounds was performed on a 2.1 mm×100 mm, 1.7 https://cannabinoidsrc4f-adb.com/ μm particle size ACQUITY Torus™ DIOL analytical column (Waters) with guard cartridge. Measurements were performed by an ACQUITY UPC2 supercritical fluid chromatography system (Waters) coupled with a Xevo TQ-S Triple Quadrupole Mass Spectrometer (Waters). During the death scene examination, multiple cigarette butts without filters were found in an ashtray; also found were alcohol bottles, an unopened box of nebivolol-containing drug, and 18 g of unrecognizable herbal residue in a cigarette box.<br>Victim B also brought "something resembling a drug" (unrecognizable by Witness A) from his cousin (Witness B) in a cigarette box and mixed this substance with their tobacco. The half-maximal effective concentration (EC50) of 4F-MDMB-BINACA is 5.69 nM (2.76–11.0 nM) on CB1, and 0.69 nM (0.30–1.56 nM) on CB2, in vitro half-life (t1/2) is 10.27 min . It is usually available as a powder, liquid (vapor fluid), or herbal plant mixtur<br><br><br>After the incubation, mixture was centrifuged (18,000 x g, 20 °C) for 5 min and 0.5 μL of the supernatant was directly injected to the chromatographic system. In the next step, ammonium formate as salting agent was added to the mixture and incubated in a thermomixer (20 °C, 1200 rpm) for 15 min. After vortex-mixing, the mixture was allowed to stand [https://cannabinoidsrc4f-adb.com/ https://cannabinoidsrc4f-adb.com/] at room temperature for 5 min. MS/MS experiments were performed in MRM (multiple reaction monitoring) mode with an isolation window of 0.4 m/z. The MS measurement was performed in positive ion mode (except for some acidic compounds such as barbiturates<br><br><br>Morris water maze test was performed to evaluate the changes in learning and memory function. Only a few case reports about the dangers of some synthetic cannabinoids due to neurotoxicity have been published (Cohen et al., 2012; McGuinness et al., 2012; Harris and Brown, 2013; Hermanns et al., 2013). In addition, the lack of information about neurotoxicity of synthetic cannabinoids could allow abusers consume those substances undiscerningly. However, slight structural changes might cause biochemical properties including dependence liability and neurotoxicity. The substances used in the present study both possess naphthoylindole moiety as their parental structure. (B) The ratio of damaged cells containing pyknotic or condensed nuclei and low hematoxilin affinity to total cells were calculated in nucleus accumben<br><br><br>All of the compounds tested in the present study depressed locomotor activity as is typical for other synthetic cannabinoids (see review by Wiley et al., 2017). Average horizontal activity counts/10 min as a function of time (10 min bins) and dose. Depressant effects of 1.33 mg/kg were observed within 10 min following administration and peak depressant effects were https://cannabinoidsrc4f-adb.com/ observed between 0–30 min. Duration of the locomotor depression increased over dose from 30 min following 0.1 mg/kg to 2.5 h following 1 mg/k<br><br>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 metabolite<br><br>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<br><br>There is indication that at least some of the first-generation synthetic cannabinoids act at receptors other than cannabinoid CB1 and CB2 (Wiley et al., 2016), and a compound from the present study, 5F-MDMB-PINACA, was found to activate midbrain dopamine neurons, but not serotonin neurons (Asaoka et al., 2016