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2. Preanalytic aspects in postmortem toxicology.

Author

Skopp, G.

Subjects
Autopsy -- Analysis -- Research, Forensic toxicology -- Research -- Analysis, Biodegradation -- Research -- Analysis, Postmortem changes -- Analysis -- Research, Blood collection and preservation -- Research -- Analysis
Abstract

Abstract The preanalytic phase has been recognized to have a substantial role for the quality and reliability of analytical results, which very much depend on the type and quality of [...]

Published
2004

3. A criterion for establishing life limits

Author

Skopp, G. H and Porter, A. A

Subjects
Quality Assurance And Reliability
Abstract

The development of a rigorous statistical method that would utilize hardware-demonstrated reliability to evaluate hardware capability and provide ground rules for safe flight margin is discussed. A statistical-based method using the Weibull/Weibayes cumulative distribution function is described. Its advantages and inadequacies are pointed out. Another, more advanced procedure, Single Flight Reliability (SFR), determines a life limit which ensures that the reliability of any single flight is never less than a stipulated value at a stipulated confidence level. Application of the SFR method is illustrated.

Published
1990

4. Erratum to: Use of Fentanyl in Adolescents with Clinically Severe Obesity Undergoing Bariatric Surgery: A Pilot Study

Author

Vaughns, J.D. (Janelle D.), Ziesenitz, V.C. (Victoria), Williams, E.F. (Elaine F.), Mushtaq, A. (Alvina), Bachmann, R. (Ricarda), Skopp, G. (Gisela), Weiss, J. (Johanna), Mikus, G. (Gerd), Anker, J.N. (John) van den, Vaughns, J.D. (Janelle D.), Ziesenitz, V.C. (Victoria), Williams, E.F. (Elaine F.), Mushtaq, A. (Alvina), Bachmann, R. (Ricarda), Skopp, G. (Gisela), Weiss, J. (Johanna), Mikus, G. (Gerd), and Anker, J.N. (John) van den

Abstract

An Online First version of this article was made available online at _http://link.springer.com/journal/40272/onlineFirst/page/1_ on 25 February 2017. An omission was subsequently identified in the article, and the following correction should be noted: In Page 6, Acknowledgem

Published
2017
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6. Bestimmung der blut/serum-verhältnisse verschiedener forensisch relevanter analyten in authentischen proben [Determination of blood/serum ratios of different forensically relevant analytes in authentic samples]

Author

Jantos, R., Schuhmacher, M., Veldstra, J.L., Bosker, W.M., Klöpping-Ketelaars, I., Touliou, K., Sardi, G.M., Brookhuis, K.A., Ramaekers, J.G., Mattern, R., and Skopp, G.

Subjects
Life, Blood/serum-ratio, Authentic samples, Central nervous agents, EELS - Earth, Environmental and Life Sciences, PHS - Pharmacokinetics & Human Studies, Plasma protein binding, Nutrition
Abstract

For forensic toxicological investigations only whole blood, but no serum is often available. Pharmacokinetic data are helpful for interpreting the results, but most of these studies indicate serum or plasma concentrations. In order to obtain reliable conversion factors which also take intersubject variability into account, the blood/serum ratios (B/S) of oxycodone, morphine, fentanyl, hydromorphone, zopiclone, MDMA, dexamphetamine, alprazolam, risperidone and 9-hydroxyrisperidone were determined by LC-MS/MS using authentic samples. Blood and corresponding serum samples were obtained from driving studies performed with controlled or known dosages of the above drugs. The analytes were analysed in blood and serum and the following mean B/S ratios (relative standard deviations) were determined: oxycodone 1.48 (8.19 %); morphine 1.03 (3.59 %); fentanyl 0.87 (13.9 %); hydromorphone 1.04 (8.11 %); zopiclone 0.89 (16.1 %); MDMA 1.19 (8.04 %); dexamphetamine 0.89 (10.9 %); alprazolam 0.81 (5.84 %); risperidone 0.65 (7.52 %); 9-hydroxyrisperidone 0.73 (12.3%). These mean values are largely in line with those reported in the literature. The B/S ratios did not appear to depend on partition coefficients, whereas there was strong evidence that B/S ratios decreased with increasing plasma protein binding.

Published
2011

7. Effects of alcohol (BAC 0.5‰) and ecstasy (MDMA 100 mg) on simulated driving performance and traffic safety

Author

Veldstra, J.L. (author), Brookhuis, K.A. (author), De Waard, D. (author), Molmans, B.H.W. (author), Verstraete, A.G. (author), Skopp, G. (author), Janstos, R. (author), Veldstra, J.L. (author), Brookhuis, K.A. (author), De Waard, D. (author), Molmans, B.H.W. (author), Verstraete, A.G. (author), Skopp, G. (author), and Janstos, R. (author)

Abstract

Rational An increasing number of fatal road-accidents have been reported in which ecstasy was found in the blood of drivers. Although, ecstasy is frequently found to have been used in combination with alcohol, studies on the acute effects of ecstasy co-administered with alcohol on driving performance are relatively rare. Objective The present study was designed to establish the extent of driver impairment as a consequence of ecstasy or combined ecstasy and alcohol use as compared to driving under the influence of 0.3‰, 0.5‰ and 0.8‰ alcohol. Furthermore, subjective performance was also assessed. Results Alcohol and ecstasy mainly influenced automated driving performance such as lateral and speed control. However, small to no effects of the substances were found on more complex driving behaviour. Overall, variance within the different driving measures was high especially when participants were treated with 3.4-methylenedioxy-methamphetamine (MDMA) and alcohol. Furthermore, equivalence testing showed that combined use may lead to impaired driving for some, but not all, drivers. Participants rated their own performance to be slightly worse than normal in both studies. Since driving was actually seriously deteriorated, this was a falsely positive assessment of their condition. Conclusions The dissociation between subjective perceptions and objective performance decrements are important notions for traffic safety since this may affect a driver’s judgement of whether or not it is safe to drive. For example, an intoxicated individual might decide to drive because the feelings of alertness caused by MDMA cloud the impairing effects of other drugs such as alcohol, thereby creating a potentially serious risk for traffic safety., Infrastructures, Systems and Services, Technology, Policy and Management

Published
2012
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9. Determination of Morphine and 6-Acetylmorphine in Blood With Use of Dried Blood Spots

Author

Garcia Boy, R., Henseler, J., Mattern, R., Skopp, G., Garcia Boy, R., Henseler, J., Mattern, R., and Skopp, G.

Abstract

Contains fulltext : 160871.pdf (publisher's version ) (Closed access), The use of dried blood spots (DBS) which has successfully been introduced in neonatal metabolic screening is an appropriate method to reduce virus infection risk to a minimum, facilitating regular mailing and handling of samples in the laboratory. Injection diacetylmorphine use is notably associated with a prevalence of infection and a risk of transmission of blood-borne viruses. The aim of the present study was to establish a method to determine morphine and 6-acetylmorphine (6-AM) as accurately and sensitively from DBS as from whole blood. Analysis by liquid chromatography/tandem mass spectrometry was checked for carryover, ion suppression/enhancement, linearity of response, lower limits of detection and quantification, and the within-run and between-run assay imprecision for both whole blood and DBS after liquid/liquid extraction. DBS drying time and elution were optimized, and extraction efficiency from DBS was compared with that of blood and of a solution of the pure compounds. Short-term stability of morphine and 6-AM was determined at -20°C, 4°C, and 40°C up to 7 days from both whole blood and DBS. Furthermore, it was tested whether analysis of DBS may be as reliable as that of whole blood investigating 50 authentic samples. The lower limit of detection was 0.4 ng of morphine per spot and 0.8 ng of 6-AM per spot using a DBS blood volume of 100 µL and was 0.3 and 0.7 ng/100 µL whole blood for morphine and 6-AM, respectively. Recovery rates of the analytes from DBS did not differ from those from whole blood and were >=55% for 6-AM and >=25% for morphine, and the within- and between-run coefficients of variation were always <=9%. 6-AM degraded rapidly at both 4°C and 40°C in whole blood; however, it seemed to be much more stable in DBS. Significant correlations between real whole-blood samples and DBS were obtained. The DBS assay has potential as a precise and inexpensive option for the determination of morphine and 6-AM in small blood samples. Further, the DBS

Published
2008

26. Certification of Death: External Postmortem Examination

Author

Madea, B, ARGO, Antonina, Madea, B, Amberg, R, Ampanozi, G, Argo, A, Bajanowski, T, Balikova, M, Bauer, J, Beh, P, Bello, S, Benedix, KP, Berghaus, G, Beyer, J, Blumenthal, R, Buschmann, CT, Cattaneo, C, Drasch, G, Drummer, OH, Felthous, AR, Fineschi, V, Flanagan, RJ, Gerostamoulos, D, Gibelli, D, Grellner, W, Henn, V, Hougen, HP, Hunsaker, JC, Jones, AW, Jones, GR, Jung, W, Karger, B, Keil, W, Kernbach-Wighton, G, Knudsen, PT, Kondo, T, Krämer, T, Kuypers, KPC, Lessig, R, Leth, PM, Lignitz, E, Luna, LA, Lunetta, P, Magalhães, T, Maurer, HH, Meissner, C, Meyer, MR, Minns, RA, Musshoff, F, Oehmichen, M, Ojanperä, I, Pilgrim, JL, Pollak, S, Pragst, F, Prinz, M, Procaccianti, P, Quester, W, Ramaekers, JG, Reibe, S, Rothschild, MA, Ruspa, M, Rutty, G, Schänzer, W, Schmeling, A, Schnabel, E, Schwaninger, AE, Skopp, G, Tag, B, Teixeira, H, Thali, MJ, Theunissen, EL, Thevis, M, Thierauf, A, Thomsen, JL, Tsokos, M, Turillazzi, E, Vann, R, Vennemann, M, Vermeeren, A, Vieira, DN, Vivell, P, Vuori, E, Vuurman, EF, Wehner, HD, Wiegand, P, and Worm-Leonhard, M

Subjects
external postmortem examination, death certification, Settore MED/43 - Medicina Legale
Published
2014

27. Formation of phosphatidylethanol and ethylglucuronide after low to moderate alcohol consumption in volunteers with a previous three-week alcohol abstinence.

Author

Herzog J, Skopp G, Musshoff F, and Hartung B

Subjects
Humans, Alcohol Abstinence, Biomarkers, Ethanol, Glycerophospholipids, Volunteers, Blood Alcohol Content, Alcohol Drinking
Abstract

Aims: Phosphatidylethanol (PEth) is only formed when ethanol is present in blood. This direct alcohol marker has been widely discussed, including the minimum amount of ethanol being necessary to form as much PEth as to exceed the threshold of 20 ng/mL in previously PEth negative subjects. In order to corroborate hitherto existing results, a drinking study including 18 participants after a 3-week alcohol abstinence was performed., Methods: They consumed a pre-calculated amount of ethanol to reach a blood alcohol concentration (BAC) of at least 0.6 g/kg. Blood was drawn before and periodically seven times after alcohol administration on day 1. Blood and urine were also collected the next morning. Dried blood spots (DBS) were prepared immediately from collected venous blood. BAC was determined by head space gas chromatography and the concentrations of both PEth (16:0/18:1, 16:0/18:2 and five additional homologues) and ethyl glucuronide (EtG) were analysed using liquid chromatography-tandem mass spectrometry., Results: Out of 18, 5 participants had concentrations of PEth 16:0/18:1 above the threshold of 20 ng/mL, and 11 out of the 18 subjects had concentrations between 10 and 20 ng/mL. In addition, four persons had PEth 16:0/18:2 concentrations above 20 ng/mL the following morning. All test subjects tested positive for EtG in DBS (≥ 3 ng/mL) and urine (≥100 ng/mL) upon 20-21 h after alcohol administration., Conclusion: By combining both a lower cutoff of 10 ng/mL and the homologue PEth 16:0/18:2, the sensitivity to detect a single alcohol intake after a 3-week abstinence increases to 72.2%., (© The Author(s) 2023. Medical Council on Alcohol and Oxford University Press. All rights reserved. For permissions, please e-mail: journals.permissions@oup.com.)

Published
2023
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28. Development and Validation of Seven Phosphatidylethanol Homologues in Dried Blood Spots Including Preliminary Results after Excessive Use of an Ethanol-Based Hand Sanitizer.

Author

Herzog J, Skopp G, and Musshoff F

Subjects
Humans, Ethanol, Alcohol Drinking, Retrospective Studies, Biomarkers urine, Hand Sanitizers, COVID-19
Abstract

Phosphatidylethanol (PEth) has become a widespread marker offering an up to 4-week retrospective window to detect alcohol use. Due to the pandemic of coronavirus disease 2019, ethanol-based hand sanitizers are frequently used. The aim of this study was to develop and validate a method for the determination of up to seven different homologues of PEth from dried blood spots (DBSs) after use of an ethanol-based hand sanitizer. The objectives of its preliminary application were to prove whether a threshold of 20 ng/mL for PEth 16:0/18:1 is reached and whether other homologues are formed as well as if positive findings of urinary ethyl glucuronide (UEtG) can be observed with respect to assess monitoring of abstinence control programs. Ten volunteers (8 occasional and 2 regular drinkers) were recruited to excessively use an ethanol-based hand sanitizer on 5 successive days. DBSs and urine samples were collected daily. PEth and UEtG were determined by liquid chromatography--tandem mass spectrometry. In total, two volunteers with initial PEth 16:0/18:1 concentrations of 19.3 and 14.6 ng/mL exceeded the threshold of 20 ng/mL six times. Subjects drinking daily or almost daily had starting PEth 16:0/18:1 concentrations of 242 and 354 ng/mL, showing a decline of PEth concentrations in six out of the seven homologues over 5 days. In teetotalers, formation of PEth species could not be observed. Thus, not satisfying requirements in an alcohol monitoring program with initial PEth-negative blood cannot be explained by a frequent use of ethanol-based hand sanitizer only. In cases of regular alcohol consumption, PEth homologues are not likely to be further influenced. However, results indicated that individuals with a PEth concentration close to 20 ng/mL are at risk of exceeding the threshold by using ethanol-based hand sanitizer., (© The Author(s) 2022. Published by Oxford University Press. All rights reserved. For permissions, please e-mail: journals.permissions@oup.com.)

Published
2023
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29. Chronic alcohol abuse may lead to high skin iron content, but not to hepatic siderosis.

Author

Paulke A, Söhling N, Held H, Wurglics M, Skopp G, and Toennes SW

Subjects
Adolescent, Adult, Aged, Aged, 80 and over, Brain metabolism, Case-Control Studies, Child, Female, Forensic Toxicology, Glucuronates analysis, Hair chemistry, Humans, Iron metabolism, Male, Middle Aged, Pancreas metabolism, Spectrophotometry, Atomic, Spleen metabolism, Vitreous Body metabolism, Young Adult, Alcoholism metabolism, Liver metabolism, Skin metabolism
Abstract

Introduction: In forensic cases, ante mortem chronic alcohol abuse can be of central importance in clarifying circumstances of death. However, reliable markers of alcohol consumption, which are still available postmortem, are needed. In addition to medical history data which may not be always authentic, the determination of ethyl glucuronide (EtG) in hair as a promising parameter is of no value in cases of missing or cosmetically treated hair. On the other hand, there exist reports that iron ions accumulate in liver tissue (siderosis) during chronic, excessive alcohol consumption, which, therefore, may be useful to serve as alcohol abuse correlate. However, the influence of ethanol on iron stored in the liver has not been adequately investigated and the study situation appears to be inconsistent., Aims: The aim of the present study was to assess the suitability of assaying iron concentrations in liver and other tissues as postmortem alcoholism marker., Methods: The iron concentration in tissue samples (liver, brain, skin, pancreas, spleen), vitreous fluid and blood taken during autopsy was analyzed by atomic absorption spectroscopy. The analytical method has been validated before. Cases were divided into two groups: chronic alcohol abusers and non-chronic alcohol consumers including total abstainers using ethyl glucuronide levels in hair as well as anamnestic data as criteria., Results: No elevated iron concentrations in the liver of chronic alcohol abusers were detected. Surprisingly, the iron concentration in skin tissue was found to be significantly higher in cases of chronic alcohol abuse, independent on whether fatty liver or liver cirrhosis was present (as diagnosedduring autopsy). In 18.5% of the cases, chronic alcohol abuse was not confirmed by the EtG concentration in hair. Thus, anamnestic data should not be overestimated., Conclusion: The general assumption that chronic alcohol abuse induces hepatic siderosis, i.e. high iron concentrations in liver tissue, has not been supported by results of the present study. However, there seems to exist a correlation between chronic alcohol abuse and high iron concentrations in the skin., (Copyright © 2019 Elsevier B.V. All rights reserved.)

Published
2019
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30. Minor contribution of cytochrome P450 3A activity on fentanyl exposure in palliative care cancer patients.

Author

Geist MJP, Ziesenitz VC, Bardenheuer HJ, Burhenne J, Skopp G, and Mikus G

Subjects
Aged, Aged, 80 and over, Analgesics, Opioid administration & dosage, Female, Fentanyl administration & dosage, Fentanyl metabolism, Fentanyl pharmacokinetics, Humans, Male, Metabolic Clearance Rate, Midazolam administration & dosage, Midazolam metabolism, Midazolam pharmacokinetics, Middle Aged, Neoplasms complications, Transdermal Patch, Analgesics, Opioid pharmacokinetics, Cancer Pain drug therapy, Cytochrome P-450 CYP3A metabolism, Fentanyl analogs & derivatives, Neoplasms therapy, Palliative Care methods
Abstract

Transdermal fentanyl is widely used to control pain in cancer patients. The high pharmacokinetic variability of fentanyl is assumed to be due to cytochrome P450 3A-mediated (CYP3A) N-dealkylation to norfentanyl in humans. However, recently published clinical studies question the importance of the described metabolic pathway. In this small study in palliative cancer patients under real-life clinical conditions, the influence of CYP3A on fentanyl variability was investigated. In addition to the determination of midazolam plasma concentration to reveal CYP3A activity, plasma concentrations of fentanyl and its metabolite, norfentanyl, were measured in identical blood samples of 20 patients who participated in an ongoing trial and had been on transdermal fentanyl. Fentanyl, norfentanyl, midazolam, and 1'-OH-midazolam were quantified by liquid chromatography/tandem mass spectrometry. Plasma concentrations of fentanyl and norfentanyl exhibited a large variability. Mean estimated total clearance of fentanyl and mean metabolic clearance of midazolam (as a marker of CYP3A activity) were 75.5 and 36.3 L/h. Both clearances showed a weak correlation and hence a minimal influence of CYP3A on fentanyl elimination.

Published
2019
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31. Determination of hydroxy metabolites of cocaine from hair samples and comparison with street cocaine samples.

Author

Franz T, Scheufler F, Stein K, Uhl M, Dame T, Schwarz G, Sachs H, Skopp G, and Musshoff F

Subjects
Chromatography, Liquid, Cocaine-Related Disorders diagnosis, Environmental Exposure, Humans, Mass Spectrometry, Narcotics analysis, Substance Abuse Detection, Cocaine analogs & derivatives, Cocaine analysis, Hair chemistry
Abstract

Drugs which are commonly smoked or sniffed (e.g. cocaine), can contaminate hair through smoke or dust; therefore testing for metabolites, especially hydroxy metabolites, is highly recommended. The presence of hydroxy metabolites in street-cocaine (COC) has been discussed. To check if detection of hydroxy metabolites definitely proves ingestion, the presence of these metabolites in street COC samples has to be checked. It is expected that the more hydrophilic hydroxy metabolites of COC are incorporated into the hair-matrix to a lesser extent. For this study 576 COC positive hair samples (≥0.1ng COC/mg hair) were analysed by LC-MS/MS for benzoylecgonine (BE), norcocaine (NC), cocaethylene (CE), ortho-, meta- and para-hydroxy COC (o-, m-, p-OH-COC), meta- and para-hydroxy BE (m-, p-OH-BE), and meta- and para-hydroxy NC (m-, p-OH-NC). The results were compared with the respective metabolite/COC concentration ratios in 146 street COC samples, confiscated by the Bavarian police. Peak areas were used to estimate BE/COC, NC/COC, CE/COC and hydroxy metabolites/COC. Similar metabolic ratios were found for o-OH-COC in 88% of the samples, but for p-OH-COC and m-OH-COC only in 5.1% and 6.8%, respectively. Notably, p- and m-OH-BE as well as p- and m-OH-NC could not be identified from seized samples. We propose that area ratios exceeding the ratios of street COC more than twice or identification of OH-BE and OH-NC enable to differentiate COC consumption from contamination. Using these criteria, consumption of the drug could be proven in 92% of COC positive samples. As detection of meta- and para-hydroxy metabolites using the above mentioned criteria is a reliable tool to distinguish between ingestion and external contamination, it is recommended to implement their measurement into daily routine work., (Copyright © 2018 Elsevier B.V. All rights reserved.)

Published
2018
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32. Alcohol Biomarkers in Clinical and Forensic Contexts.

Author

Andresen-Streichert H, Müller A, Glahn A, Skopp G, and Sterneck M

Subjects
Alcohol Drinking metabolism, Alcohol Drinking urine, Biomarkers analysis, Biomarkers blood, Biomarkers urine, Ethyl Ethers analysis, Ethyl Ethers metabolism, Forensic Sciences methods, Forensic Sciences standards, Glucuronates analysis, Glucuronates blood, Glycerophospholipids analysis, Glycerophospholipids blood, Hair enzymology, Hair metabolism, Hair pathology, Humans, Jurisprudence, Middle Aged, Sulfuric Acid Esters analysis, Sulfuric Acid Esters blood, Sulfuric Acid Esters urine, Time Factors, Transferrin analogs & derivatives, Transferrin analysis, gamma-Glutamyltransferase analysis, gamma-Glutamyltransferase blood, Alcohol Drinking blood, Weights and Measures standards
Abstract

Background: Biomarkers of alcohol consumption are important not only in forensic contexts, e.g., in child custody proceedings or as documentation of alcohol abstinence after temporary confiscation of a driver's license. They are increasingly being used in clinical medicine as well for verification of abstinence or to rule out the harmful use of alcohol., Methods: This review is based on pertinent publications that were retrieved by a selective literature search in PubMed concerning the direct and indirect alcohol markers discussed here, as well as on the authors' experience in laboratory analysis and clinical medicine., Results: Alongside the direct demonstration of ethanol, the available markers of alcohol consumption include the classic indirect markers carbohydrate-deficient transferrin (CDT), gamma-glutamyltransferase (GGT), and mean corpuscular volume (MCV) as well as direct alcohol markers such as ethyl glucuronide (EtG) and ethyl sulfate (EtS) in serum and urine and EtG and fatty acid ethyl esters (FAEE) in hair. Phosphatidylethanol (PEth) is a promising parameter that com - plements the existing spectrum of tests with high specificity (48-89%) and sensi - tivity (88-100%). In routine clinical practice, the demonstration of positive alcohol markers often leads patients to admit previously denied alcohol use. This makes it possible to motivate the patient to undergo treatment for alcoholism., Conclusion: The available alcohol biomarkers vary in sensitivity and specificity with respect to the time period over which they indicate alcohol use and the minimum extent of alcohol use that they can detect. The appropriate marker or combination of markers should be chosen in each case according to the particular question that is to be answered by laboratory analysis.

Published
2018
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33. Improved detection of alcohol consumption using the novel marker phosphatidylethanol in the transplant setting: results of a prospective study.

Author

Andresen-Streichert H, Beres Y, Weinmann W, Schröck A, Müller A, Skopp G, Pischke S, Vettorazzi E, Lohse A, Nashan B, and Sterneck M

Subjects
Adult, Aged, Alcohol Drinking metabolism, Biomarkers analysis, Biomarkers urine, Ethanol urine, False Positive Reactions, Female, Glucuronates urine, Glycerophospholipids analysis, Glycerophospholipids urine, Hair chemistry, Humans, Liver Diseases, Alcoholic metabolism, Male, Methanol urine, Middle Aged, Prospective Studies, Retrospective Studies, Sensitivity and Specificity, Surveys and Questionnaires, Transferrin analogs & derivatives, Transferrin urine, Alcohol Drinking urine, Liver Diseases, Alcoholic surgery, Liver Diseases, Alcoholic urine, Liver Transplantation
Abstract

Phosphatidylethanol (PEth) is a new, highly specific alcohol marker. The aim of this study was to assess its diagnostic value in the liver transplant setting. In 51 pre- and 61 post-transplant patients with underlying alcoholic liver disease PEth, ethanol, methanol, carbohydrate-deficient transferrin (CDT), and ethyl glucuronide in urine (uEtG) and hair (hEtG) were tested and compared with patients' questionnaire reports. Twenty-eight (25%) patients tested positive for at least one alcohol marker. PEth alone revealed alcohol consumption in 18% of patients. With respect to detection of alcohol intake in the preceding week, PEth showed a 100% sensitivity. PEth testing was more sensitive than the determination of ethanol, methanol, CDT or uEtG alone [sensitivity 25% (confidence interval (CI) 95%, 7-52%), 25% (7-52%), 21% (6-45%) and 71% (41-91%), respectively], or ethanol, methanol and uEtG taken in combination with 73% (45-92%). Specificity of all markers was 92% or higher. Additional testing of hEtG revealed alcohol consumption in seven patients, not being positive for any other marker. Phosphatidylethanol was a highly specific and sensitive marker for detection of recent alcohol consumption in pre- and post-transplant patients. The additional determination of hEtG was useful in disclosing alcohol consumption 3-6 months retrospectively., (© 2017 Steunstichting ESOT.)

Published
2017
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34. Formation and inhibition of ethyl glucuronide and ethyl sulfate.

Author

Stachel N and Skopp G

Subjects
Area Under Curve, Humans, Mass Spectrometry, Substance Abuse Detection, Alcohol Drinking, Biomarkers metabolism, Glucuronates metabolism, Polyphenols antagonists & inhibitors, Sulfuric Acid Esters metabolism
Abstract

Ethyl glucuronide (EtG) und ethyl sulfate (EtS) are widely accepted biomarkers in forensic and clinical settings. Even though, levels of EtG and EtS in blood and urine increase with increasing doses of alcohol, a high inter-individual variability in their production has been noticed. Therefore, we investigated the influence of dietary plant phenols on the formation of EtG and EtS and tentatively estimated the magnitude of in vivo inhibitory interactions from our in vitro results. To address these issues, formation of EtS and EtG was investigated using recombinant glucuronosyl- and sulfotransferases as well as human liver microsomes and liver cytosol. After respective kinetics had been established, inhibition experiments using quercetin, kaempferol and resveratrol were performed. These polyphenols are subject to extensive glucuronidation and/or sulfonation. EtG and EtS were determined by LC-MS/MS following solid phase extraction for EtG due to severe matrix effects and by direct injection for EtS. All enzymes investigated were involved in the conjugation of ethanol. Maximal EtG and EtS formation rates were observed with HLM and SULT1A1, respectively. All kinetics could best be described by Michaelis-Menten kinetics. Resveratrol was a competitive inhibitor of UGT1A1, UGT1A9 and HLM; quercetin and kaempferol were inhibitors of all transferases under investigation except UGT2B15. Findings for quercetin with regard to UGT2B7 and SULT2A1 and for kaempferol with regard to SULT1E1 and SULT2A1 suggested a mechanism based inhibition. Competitive inhibition of the glucuronidation and sulfonation of ethanol was estimated as weak to negligible and as moderate to weak, respectively. Beside the known polymorphisms of the transferases involved in EtG and EtS formation, prediction of the inhibitory potential indicates that polyphenols may contribute to the variable formation rate of EtG and EtS., (Copyright © 2016 Elsevier Ireland Ltd. All rights reserved.)

Published
2016
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35. Identification and preliminary characterization of UDP-glucuronosyltransferases catalyzing formation of ethyl glucuronide.

Author

Schwab N and Skopp G

Subjects
Biocatalysis, Ethanol metabolism, Glucuronates chemistry, Humans, Isoenzymes chemistry, Isoenzymes metabolism, Kinetics, Glucuronates metabolism, Glucuronosyltransferase chemistry, Glucuronosyltransferase metabolism
Abstract

Ethyl glucuronide (EtG), a minor metabolite of ethanol, is used as a marker of alcohol consumption in a variety of clinical and forensic settings. At present there are very few studies of UDP-glucuronosyltransferases (UGT), responsible for catalyzing EtG formation, and the possible effect of nutritional components, e.g. flavonoids, which are extensively glucuronidated, on EtG formation has not been addressed at all. The following incubation conditions were optimized with regard to previously published conditions: buffer, substrate concentration, and incubation time. Isolation of EtG from the incubation mixture was also optimized. Recombinant UGT enzymes (UGT1A1, 1A3, 1A4, 1A6, 1A9, 2B7, 2B10, 2B15) were screened for their activity towards ethanol, and kinetic data were then established for all enzymes. It was decided to study the effect of the flavonoids quercetin and kaempferol on glucuronidation of ethanol. Isolation was by solid-phase extraction (SPE) to minimize matrix effects. Analysis was performed by liquid chromatography-tandem mass spectrometry (LC-MS-MS), with EtG-d5 as the internal standard. SPE was vital to avoid severe ion suppression after direct injection of the incubation solution. EtG formation was observed for all enzymes under investigation; their kinetics followed the Michaelis-Menten model, meaning the maximum reaction rate achieved at saturating substrate concentrations (V(max)) and the substrate concentration at which the reaction rate is half of V(max) (Michaelis-Menten constant, K(m)) could be calculated. The highest rate of glucuronidation was observed with UGT1A9 and 2B7. After co-incubation with both flavonoids, formation of EtG was significantly reduced for all enzymes except for UGT2B15, whose activity did not seem to be affected. Results reveal that multiple UGT isoforms are capable of catalyzing glucuronidation of ethanol; nevertheless, the effect of UGT polymorphism on glucuronidation of ethanol needs further study. Formation of EtG is inhibited by the flavonoids under investigation. Obviously, nutritional components affect conversion of ethanol to EtG. This observation may serve as a partial explanation of its variable formation in man.

Published
2014
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36. An in vitro experiment on the interaction of charcoal or wheat bran with 11-nor-9-carboxy-Δ(9)-tetrahydrocannabinol and its glucuronide.

Author

Skopp G and Mikus G

Subjects
Dietary Fiber metabolism, Dronabinol chemistry, Dronabinol metabolism, Glucuronides metabolism, Humans, Intestinal Mucosa metabolism, Kinetics, Models, Biological, Charcoal chemistry, Dietary Fiber analysis, Dronabinol analogs & derivatives, Glucuronides chemistry
Abstract

The rather long yet variable terminal half-lives and detection times since last use of urinary cannabinoids may partly be attributed to their enterohepatic circulation which generally can be interrupted or restricted by chemical adsorbents. Therefore, an in vitro experiment was performed to study the adsorption/binding of 11-nor-9-carboxy-Δ9-tetrahydrocannabinol (THC-COOH) and its glucuronide to activated charcoal and wheat bran; remaining concentrations were determined by liquid chromatography/tandem mass spectrometry. Adsorption/binding of 1,000 ng/mL of free or conjugated THC-COOH was complete using as little as 5 mg of charcoal whereas adsorption/binding to wheat bran increased with increasing amounts. Taking of remedies affecting enterohepatic recycling of THC-COOH and its glucuronide may challenge interpretation of cannabinoid concentrations used to detect or assess frequency of drug use or the time since last drug consumption.

Published
2013
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37. Postmortem blood and tissue concentrations of R- and S-enantiomers of methadone and its metabolite EDDP.

Author

Jantos R and Skopp G

Subjects
Adult, Chromatography, Liquid methods, Female, Forensic Toxicology, Humans, Male, Mass Spectrometry, Postmortem Changes, Stereoisomerism, Tissue Distribution, Young Adult, Methadone blood, Methadone pharmacokinetics, Narcotics blood, Narcotics pharmacokinetics, Pyrrolidines blood, Pyrrolidines pharmacokinetics
Abstract

Body fluids and tissues in 16 methadone (MTD)-associated fatalities were investigated to find out whether analysis of MTD and its metabolite 2-ethylidine-1,5-dimethyl-3,3-diphenylpyrrolidine (EDDP) following enantioselective separation of both compounds may assist in the interpretation of MTD findings. Individual case histories were shortly described. R- and S-MTD as well as R- and S-EDDP concentrations were determined by chiral LC-MS/MS. In all cases under investigation total MTD was present in sufficient quantities to kill or to contribute to death; concentrations were highest in lungs (MTD) and kidneys (EDDP). It appears that both MTD and EDDP undergo postmortem redistribution. In three cases, only the pharmacologically active R-MTD isomer was present. R-MTD mainly contributing to the drug's pharmacological effects, the enantiomeric ratio of MTD and EDDP may indicate whether MTD intoxication might have contributed to death or not. Further, it may be helpful to establish whether racemic MTD or enantiomerically pure R-MTD has been administered last, especially if R/S-ratios of MTD and EDDP significantly differ. It could be shown, that in vivo racemization occurs for neither MTD nor EDDP in any body fluid or tissue sample. Significantly higher MTD R/S-ratios in femoral and heart blood were present in individuals having participated in a MTD maintenance program. Overall, R/S-ratios of MTD and EDDP allow a more detailed interpretation of analytical results in MTD-associated deaths. Thus, determination of MTD and EDDP by enantioselective methods and calculation of their R/S-ratios should be favored., (Copyright © 2013 Elsevier Ireland Ltd. All rights reserved.)

Published
2013
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38. LC-MS/MS analysis of phosphatidylethanol in dried blood spots versus conventional blood specimens.

Author

Faller A, Richter B, Kluge M, Koenig P, Seitz HK, Thierauf A, Gnann H, Winkler M, Mattern R, and Skopp G

Subjects
Alcoholism blood, Biomarkers blood, Humans, Blood Chemical Analysis, Chromatography, Liquid, Dried Blood Spot Testing methods, Glycerophospholipids blood, Mass Spectrometry
Abstract

Phosphatidylethanol (PEth), which is formed extrahepatically by the action of phospholipase D on phosphatidylcholine in the presence of ethanol, has been suggested as a promising marker of alcohol misuse. Analysis of dried blood spots (DBS) is particularly advantageous for the determination of delicate analytes such as PEth. Therefore, measurement of PEth species (18:1/18:1, 16:0/18:1) in DBS versus whole blood was performed to ascertain whether respective results are directly comparable. Samples were obtained from subjects (n = 40) undergoing alcohol detoxification treatment. Analysis involved liquid-liquid extraction from both, DBS and whole blood (100 μL, respectively), with phosphatidylpropanol as the internal standard. Extracts were subjected to LC gradient separation using multiple reaction monitoring of deprotonated molecules. Results from measurements of corresponding DBS and whole blood specimens were compared by estimating the respective mean values and by a Bland and Altman analysis. Concentrations of PEth 18:1/18:1 ranged from 46.1 to 3,360 ng/mL in whole blood (mean, 461.7 ng/mL) and from 35.8 to 3,360 ng/mL in DBS (mean, 457.6 ng/mL); for PEth 16:0/18:1, concentrations were from 900 to 213,000 ng/mL (mean, 23,375 ng/mL) and 922-213,000 ng/mL (mean, 23,470 ng/mL) in blood and DBS, respectively. Estimated mean differences were -4.3 ng/mL for PEth 18:1/18:1 and 95.8 ng/mL for PEth 16:0/18:1. The Bland-Altman plot of both PEth species showed that the variation around the mean difference was similar all through the range of measured values and that all differences except one were within the limits of agreement. It could be shown that the determination of PEth species in DBS is as reliable as in whole blood samples. This assay may facilitate monitoring of alcohol misuse.

Published
2011
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39. A preliminary investigation on the distribution of cannabinoids in man.

Author

Gronewold A and Skopp G

Subjects
Adult, Bile chemistry, Brain Chemistry, Chromatography, Liquid, Forensic Toxicology, Gallbladder chemistry, Gastrointestinal Contents chemistry, Humans, Kidney chemistry, Liver chemistry, Lung chemistry, Male, Mass Spectrometry, Psoas Muscles chemistry, Tissue Distribution, Cannabinoids analysis, Cannabinoids pharmacokinetics
Abstract

An LC/MS/MS procedure to determine THC along with its major metabolites 11-OH-THC, THC-COOH and its glucuronide as well as the cannabinoids CBD and CBN was applied to 5 post mortem cases to study their distribution into some less commonly studied matrices. Analytes were determined in fluids and tissue homogenates following protein precipitation and liquid-liquid extraction. Gall bladder fluid exhibited maximum concentrations of all analytes except THC, which was detectable in high concentrations in muscle tissue along with CBD. THC was also present in lung specimens, whereas its concentration in liver samples was low or not detectable at all. Liver und kidney specimens contained appreciable amounts of THC-COOglu. Findings from bile support extensive enterohepatic recirculation of the glucuronide. Muscle tissue seems an interesting specimen to detect multiple cannabis use, and brain may serve as an alternative specimen for blood; nevertheless, the present findings should be substantiated by further investigations., (Copyright © 2011 Elsevier Ireland Ltd. All rights reserved.)

Published
2011
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40. Buprenorphine and major metabolites in blood specimens collected for drug analysis in law enforcement purposes.

Author

Oechsler S and Skopp G

Subjects
Chromatography, Liquid, Forensic Toxicology, Humans, Spectrometry, Mass, Electrospray Ionization, Substance Abuse Detection, Tandem Mass Spectrometry, Analgesics, Opioid blood, Buprenorphine analogs & derivatives, Buprenorphine blood, Law Enforcement
Abstract

A liquid chromatographic/electrospray ionization tandem mass spectrometric method for the quantification of buprenorphine (BUP), norbuprenorphine (NBUP), buprenorphine-3-beta-D-glucuronide (BUPG) and norbuprenorphine-3-beta-D-glucuronide (NBUPG) in serum samples was developed and validated. Pre-treatment of BUP and NBUP was by liquid-liquid extraction, while glucuronides were favourably isolated by solid phase extraction. Separation in 2 separate runs (2 x 5 min) was achieved using isocratic elution. The method was applied to 20 authentic serum specimens collected for law enforcement purposes where BUP intake had been indicated. The parent drug was not detectable in half of the specimens at a lower limit of detection of 0.2 ng/mL, whereas NBUP could be determined from any sample but one. NBUPG is the major metabolite present, which could be identified along with BUPG in all samples under investigation. In authentic specimens it could be advisable to monitor BUP metabolites along with the parent drug., (2009 Elsevier Ireland Ltd. All rights reserved.)

Published
2010
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41. Doxepin and nordoxepin concentrations in body fluids and tissues in doxepin associated deaths.

Author

Gronewold A, Dettling A, Haffner HT, and Skopp G

Subjects
Adult, Bile chemistry, Brain Chemistry, Chromatography, Liquid, Female, Forensic Toxicology, Gastrointestinal Contents chemistry, Humans, Kidney chemistry, Liver chemistry, Lung chemistry, Male, Mass Spectrometry, Middle Aged, Muscle, Skeletal chemistry, Substance-Related Disorders complications, Antidepressive Agents, Tricyclic analysis, Antidepressive Agents, Tricyclic poisoning, Doxepin analogs & derivatives, Doxepin analysis, Doxepin poisoning
Abstract

Body fluids and tissues in eight doxepin (Dox)-related deaths were investigated in order to prove whether the individual concentration of Dox, the concentration sum of parent drug and its active metabolite N-desmethyldoxepin (NDox) or the concentration ratio Dox/Ndox valuably contribute to making a cause of death determination. Individual case histories were shortly described. Dox and NDox concentrations were determined by LC-MS/MS. Dox concentration measured from two cases was well within a concentration range considered therapeutic, whereas subtherapeutic dosing may have occurred in another two cases. There were two cases of fatal Dox ingestion, as well as a case of high dosage and advanced putrefaction, respectively. The liver concentration sum may be more useful if a fatal ingestion cannot be clearly separated from a person's medication usage. High concentrations could be observed in lung tissue, and combined concentrations of Dox and NDox may also be helpful in making a cause of death determination. There was a trend to a higher concentration sum in the brain with increasing combined levels in blood. Overall, the sum of the absolute figures allows a more accurate interpretation in Dox-related deaths as compared to the molar concentration ratio which may be helpful in acute ingestion. Determination of the N-desmethyl metabolite along with its parent is recommended and analysis should include more than a single specimen.

Published
2009
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42. Deposition of cannabinoids in hair after long-term use of cannabis.

Author

Skopp G, Strohbeck-Kuehner P, Mann K, and Hermann D

Subjects
Adult, Case-Control Studies, Forensic Toxicology, Gas Chromatography-Mass Spectrometry, Humans, Male, Regression Analysis, Substance Abuse Detection, Time Factors, Cannabinoids analysis, Hair chemistry, Marijuana Abuse diagnosis
Abstract

Hair analysis has shown great potential in the detection and control of drug use. Whether an assay is of quantitative value roughly corresponding to the amount of drug consumed, is still a matter of debate. The present investigation was aimed at a possible relationship between the cannabinoid concentration in hair and the cumulative dose in regular users of cannabis. Hair samples from the vertex region of the scalp were obtained from 12 male regular users of cannabis, and 10 male subjects with no experience of cannabis served as controls. None of the subjects had his hair permed, bleached or colored. Cannabis users provided information on drug use such as the current cannabis dose per day, the cumulative cannabis dose of the last 3 months, as well as the frequency of cannabis use during the last year. The concentration of delta-9-tetrahydrocannabinol (THC), cannabinol (CBN) and cannabidiol (CBD) in hair was determined using gas chromatography-mass spectrometry. Cannabinoids were present in any hair sample of cannabis users, but were not detectable in control specimens. An increase in the amount of cannabinoids in hair with increasing dose was evident. The concentration of major cannabinoids (sum of THC, CBD and CBN) was significantly correlated to either the reported cumulative cannabis dose during the last 3 months or to the cannabis use during the last 3 months estimated from the daily dose and the frequency per year (r=0.68 or 0.71, p=0.023 or 0.014). A significant relationship between THC and the amount of cannabis used could not be established. As a conclusion, the sum of major cannabinoids in hair of regular users may provide a better measure of drug use than THC.

Published
2007
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43. Tissue distribution of mirtazapine and desmethylmirtazapine in a case of mirtazapine poisoning.

Author

Wenzel S, Aderjan R, Mattern R, Pedal I, and Skopp G

Subjects
Aged, Amitriptyline blood, Antidepressive Agents, Tricyclic blood, Bile chemistry, Brain Chemistry, Forensic Pathology, Gas Chromatography-Mass Spectrometry, Gastrointestinal Contents chemistry, Humans, Kidney chemistry, Liver chemistry, Lung chemistry, Male, Mianserin pharmacokinetics, Mianserin poisoning, Mirtazapine, Muscle, Skeletal chemistry, Nortriptyline blood, Sertraline blood, Suicide, Tissue Distribution, Antidepressive Agents, Tricyclic pharmacokinetics, Antidepressive Agents, Tricyclic poisoning, Mianserin analogs & derivatives
Abstract

An ingestion of an unknown quantity of mirtazapine in a suicide attempt leading to death is described. Sertraline and amitriptyline have been co-ingested. Because mirtazapine is reported to be relatively safe in overdose, body fluids and tissues were investigated for both mirtazapine and desmethylmirtazapine by high-pressure liquid chromatography/tandem mass spectrometry following liquid-liquid extraction. The limit of detection was sufficiently low to also apply the assay in pharmacokinetic studies. The levels of amitriptyline and nortriptyline were very low (38 and 19 ng/mL femoral venous blood) and the amount of sertraline in blood taken from the femoral vein (880 ng/mL) was considerably lower than those seen in overdosage. Accumulation of mirtazapine and N-desmethylmirtazapine was evident in fluids and tissues involved in enterohepatic circulation and excretion. The concentration determined in a brain sample suggests a contribution of the metabolite to the drug's pharmacodynamic activity. Based on literature data, significant adverse or synergistic effects among the drugs detected as well as adverse reactions such as a serotonin reaction appeared less probable. Mirtazapine exhibits alpha(1)-antagonistic properties on the cardiac-vascular system and may cause hyponatraemia. In the face of the cardiac findings at autopsy and the lack of an apparent cause of death, these effects of mirtazapine may have initiated a process leading to death.

Published
2006
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44. In vitro contamination of hair by marijuana smoke.

Author

Thorspecken J, Skopp G, and Pötsch L

Subjects
Gas Chromatography-Mass Spectrometry, Humans, Cannabinoids analysis, Hair chemistry, Marijuana Smoking
Abstract

Background: The deposition of cannabinoids on/into hair from environmental smoke can be considered as a potential source of drug findings in hair. We studied external uptake of cannabinoids from marijuana smoke, investigating possible influencing factors on drug uptake and the efficiency of decontamination procedures., Methods: Strands of a natural hair sample were moistened with water, greased with sebum or sebum/sweat, or bleached or permed. Treated and untreated samples were exposed to marijuana smoke for 60 min. Aliquots of each hair strand were either kept unwashed or were washed with methanol, dichloromethane, or 5 g/L dodecyl sulfate in water. Cannabinoid concentrations in unwashed and washed hair samples, as well as in air samples collected from the exposure chamber and in the marijuana sample being combusted, were quantified by gas chromatography-mass spectrometry or gas chromatography., Results: Cannabinoids were deposited on the hair fibers from marijuana smoke. Cannabinoid concentrations were dependent on air concentration and hair pretreatment. Uptake was less in untreated than in pretreated hair. Concentrations were increased in damp hair, but were even higher in greased hair. There was no significant difference in concentration between bleached and permed strands. External contaminants were completely removed by washing with methanol and dichloromethane in untreated hair only. Washing with dodecyl sulfate in water was insufficient in all cases., Conclusions: Exposures of hair to marijuana smoke yields detectable cannabinoids depending on concentrations in the air, hair care habits, and cosmetic treatment. Environmental marijuana smoke exposure may produce false-positive or falsely increased test results in hair.

Published
2004
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45. An investigation of the stability of free and glucuronidated 11-nor-delta9-tetrahydrocannabinol-9-carboxylic acid in authentic urine samples.

Author

Skopp G and Pötsch L

Subjects
Artifacts, Diagnostic Errors, Drug Stability, Humans, Hydrogen-Ion Concentration, Mass Spectrometry, Dronabinol analogs & derivatives, Dronabinol urine, Forensic Medicine methods, Glucuronides urine, Substance Abuse Detection methods, Substance-Related Disorders urine
Abstract

Preanalytical stability of a drug and its major metabolites is an important consideration in pharmacokinetic studies or whenever the analyte pattern is used to estimate drug habits. Firstly, the stability of free and glucuronidated 11-nor-delta9-tetrahydrocannabinol-9-carboxylic acid (THCCOOH, THCCOOglu) in authentic urine samples was investigated. Random urine samples of cannabis users (n = 38) were stored at -20, 4, and 20 degrees C up to 15 days and up to 5 days at 40 degrees C, and alterations of the analyte pattern during storage were followed by liquid chromatography-tandem mass spectrometry. Secondly, the influence of pH (range 5.0-8.0) on the stability of the analytes was studied using spiked urine to elucidate the results obtained from authentic samples. In authentic urine samples, the initial pH ranged from 5.1 to 8.8. The glucuronide was found to be highly labile at a storage temperature of 4 degrees C and above. Initially, 18 urine samples tested positive for THCCOOH. After 2 days storage at 20 degrees C, THCCOOH was detectable in a further 4 samples, and 7 more samples tested positive for THCCOOH (5-81 ng/mL) after 15 days. Depending on time and temperature, the glucuronide concentration decreased, resulting in an increase of THCCOOH concentration. However, a loss in mean total THCCOOH concentration was found, which was significantly higher in deteriorated samples than in samples without signs of deterioration after 15 days of storage at 20 degrees C. In the drug-free urine sample separately spiked with THCCOOglu or THCCOOH, the investigations on the stability of the target analytes at various pH values revealed that THCCOOH was stable at pH 5.0. At higher pH values, its concentration slightly decreased with time, and about 69% of the initial THCCOOH concentration was still present at pH 8.0 on day 5. THCCOOglu concentrations rapidly decreased with increasing pH value. For example, only 72% of the initial THCCOOglu concentration could be detected at pH 5.0 on day 1. Degradation of the glucuronide resulted in formation of THCCOOH, which was observed even at pH 5.0. In light of the present findings, advanced forensic interpretations based on the presence of THCCOOH or the pattern of THCCOOH and THCCOOglu in stored urine samples seems questionable.

Published
2004
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47. Partition coefficient, blood to plasma ratio, protein binding and short-term stability of 11-nor-Delta(9)-carboxy tetrahydrocannabinol glucuronide.

Author

Skopp G, Pötsch L, Mauden M, and Richter B

Subjects
Blood Specimen Collection, Dronabinol blood, Drug Stability, Forensic Medicine, Glucuronides blood, Humans, Mass Spectrometry, Protein Binding, Dronabinol administration & dosage, Dronabinol analogs & derivatives, Dronabinol analysis, Glucuronides analysis
Abstract

11-Nor-Delta(9)-carboxy tetrahydrocannabinol glucuronide (THCCOOglu) is a major metabolite of tetrahydrocannabinol in blood. Despite its mass spectrometric identification already in 1980, further physicochemical data of THCCOOglu have not been established. Therefore, the octanol/buffer partition coefficient P and the blood to plasma ratio b/p for THCCOOglu concentrations of 100 and 500ng/ml were investigated. Protein binding of the glucuronide was established from spiked albumin solutions at a level of 250ng/ml as well as from authentic samples. The data were compared to those of 11-nor-Delta(9)-carboxy tetrahydrocannabinol (THCCOOH). In addition, the short-term stability of THCCOOglu in plasma at different storage temperatures was studied. Analysis was performed by LC/MS/MS. The glucuronide partition coefficient P (mean: 17.4 and 18.0 for 100 and 500ng/ml, respectively) was unexpectedly lipophilic at pH 7.4. Its blood to plasma ratios averaged 0.62 and 0.68 at 100 and 500ng/ml, respectively. THCCOOglu was highly reversibly bound to albumin (mean: 97%), and the mean fraction bound did not differ from that determined from authentic samples. THCCOOglu degraded even at a storage temperature of 4 degrees C and THCCOOH was identified as a major decomposition product.

Published
2002
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48. Stability of 11-nor-delta(9)-carboxy-tetrahydrocannabinol glucuronide in plasma and urine assessed by liquid chromatography-tandem mass spectrometry.

Author

Skopp G and Pötsch L

Subjects
Blood Specimen Collection, Chromatography, Liquid, Dronabinol blood, Dronabinol urine, Drug Stability, Glucuronides blood, Glucuronides urine, Humans, Mass Spectrometry, Sensitivity and Specificity, Temperature, Time Factors, Dronabinol analogs & derivatives, Dronabinol analysis, Glucuronides analysis
Abstract

Background: Unconjugated 11-nor-Delta(9)-carboxy-tetrahydrocannabinol (THCCOOH) in blood and urine has been proposed as a valuable marker, but the glucuronide (THCCOOglu) is present in considerably higher concentrations than the parent drug. Acyl glucuronides have been shown to be potentially reactive conjugates, which may affect the in vitro metabolite pattern., Methods: Extraction procedures and a liquid chromatography-tandem mass spectrometry assay were developed and validated to investigate the stability of THCCOOglu in urine and plasma. Plasma and urine samples with added THCCOOglu were stored at -20, 4, 20, and 40 degrees C up to 10 days., Results: The glucuronide was stable at -20 degrees C in both matrices, whereas THCCOOglu concentrations decreased at all other storage conditions. For a given storage time and temperature, the decrease in plasma was higher than that in urine. At 20 degrees C, a marked change in concentration could be observed within 2 days of storage. Degradation of THCCOOglu followed an apparent first-order process and led to the formation of THCCOOH. The sum of the molar concentrations of both analytes corresponded only to the initial THCCOOglu in plasma and urine samples stored at 4 degrees C., Conclusions: The in vitro degradation of THCCOOglu prevents clinical conclusions based on the metabolite pattern or the concentration of unconjugated THCCOOH in samples stored at > or =4 degrees C for prolonged periods.

Published
2002

49. Laparoscopic fluorescence diagnosis for intraabdominal fluorescence targeting of peritoneal carcinosis experimental studies.

Author

Gahlen J, Prosst RL, Pietschmann M, Haase T, Rheinwald M, Skopp G, Stern J, and Herfarth C

Subjects
Animals, Colonic Neoplasms pathology, Fluorescence, Laparoscopy, Peritoneal Neoplasms secondary, Protoporphyrins metabolism, Random Allocation, Rats, Rats, Inbred Strains, Tumor Cells, Cultured, Aminolevulinic Acid therapeutic use, Neoplasm Staging methods, Peritoneal Neoplasms diagnosis, Photosensitizing Agents
Abstract

Objective: To assess 5-aminolevulinic acid (ALA)-induced protoporphyrin IX accumulation and fluorescence in peritoneal colon carcinoma metastases and its benefits for laparoscopic fluorescence diagnosis., Summary Background Data: Occult, macroscopically nonvisible peritoneal micrometastases can be missed in laparoscopy or open surgery. Laparoscopic fluorescence diagnosis allows detection of these lesions after intraperitoneal lavage with ALA and subsequent fluorescence induction by blue-light excitation., Methods: A disseminated peritoneal carcinosis was induced by laparoscopic implantation of colon carcinoma cells (CC531) in the peritoneum of 55 WAG/Rij rats. After 12 days of tumor growth the animals were randomized into 11 groups with different photosensitization parameters. Peritoneal lavage was performed either with 1.5% or 3.0% ALA solution, except for one control group. Photosensitization times were 0.5, 1, 2, 4, or 8 hours. Spectrometry was performed using an optical multichannel analyser. ALA and protoporphyrin IX serum levels were measured by high-performance liquid chromatography to determine systemic load., Results: Protoporphyrin IX tumor accumulation and fluorescence peaked 2 to 4 hours after ALA application in both main groups, 1.5% and 3.0% ALA. Tumor detection rate was most effective in the 1.5% ALA group. Compared with conventional white-light laparoscopy alone, blue-light excitation detected 35% additional intraabdominal tumor foci., Conclusions: Laparoscopic fluorescence diagnosis can increase the sensitivity and specificity of diagnostic staging laparoscopy. It allows determination of the extent of peritoneal carcinosis. Improved preoperative assessment helps to avoid unnecessary laparotomies and radical resections.

Published
2002
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50. Stability of morphine, morphine-3-glucuronide, and morphine-6-glucuronide in fresh blood and plasma and postmortem blood samples.

Author

Skopp G, Pötsch L, Klingmann A, and Mattern R

Subjects
Drug Stability, Humans, Hydrogen-Ion Concentration, Light, Morphine analysis, Morphine Derivatives analysis, Temperature, Morphine blood, Morphine Derivatives blood
Abstract

The present study was designed to determine the stability of morphine and its glucuronides in spiked fresh blood and plasma from live individuals as well as in four authentic postmortem blood specimens for a time interval of up to six months. The samples were stored in glass vials at -20 degrees C, 4 degrees C, and 20 degrees C. Additionally, spiked samples were exposed to light through window glass and subjected to a forced-degradation study at 40 degrees C. Data were established using solid-phase extraction and high-performance liquid chromatography coupled to atmospheric pressure ionization mass spectrometry for isolation and quantitation, providing a sensitive and specific detection method for the parent drug in the presence of its glucuronide metabolites. Morphine and its glucuronide metabolites were found to be stable in both blood and plasma at 4 degrees C for the whole observation period. In postmortem blood the analytes were stable only when stored at -20 degrees C. The thermal decomposition of morphine and morphine-6-glucuronide in spiked blood and plasma could be interpreted using pseudo first-order kinetics. Photodegradation of morphine-3-glucuronide in plasma was consistent with a second-order reaction. In postmortem samples the degradation pattern differed completely from that observed in fresh blood and plasma. The elevated morphine levels observed were primarily due to postmortem hydrolysis of morphine glucuronides.

Published
2001
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