Your search keyword '"Skopp G"' showing total 247 results

201. [Serum norharman and harman analysis using high pressure liquid chromatography/mass spectrometry and value of beta-carbolines as blood alcohol markers].

Author

Pötsch L and Skopp G

Subjects

Alcoholic Intoxication blood, Carbolines, Humans, Predictive Value of Tests, Reference Values, Smoking blood, Alcoholic Intoxication diagnosis, Ethanol blood, Gas Chromatography-Mass Spectrometry, Harmine analogs & derivatives, Harmine blood

Abstract

Firstly, a method for LC-MS/MS-analysis of the beta-carbolines norharman and harman in serum was established and validated. Secondly, serum samples from persons during ethanol loading conditions were investigated (n = 26). Norharman was regularly found positive only in persons with BAC > 1.6@1000. In this subgroup harman was detected in 5 out of 9 cases. The finding of norharman concentrations > 50 pg/mL in the serum of 4 out of 5 control persons was of high interest. In addition serum samples of smokers (n = 9) were analyzed for the beta-carbolines. All samples from smokers were tested positive for norharman with concentrations > 50 pg/mL in 7 cases. These results were in accordance with recent reports in literature and underline that the beta-carbolines norharman and harman do not meet the criteria of alcohol state-markers and positive serum sample testing may result from endogenous as well as from exogenous sources.

Published

2002

202. Short-term stability of lysergic acid diethylamide (LSD), N-desmethyl-LSD, and 2-oxo-3-hydroxy-LSD in urine, assessed by liquid chromatography-tandem mass spectrometry.

Author

Skopp G, Pötsch L, Mattern R, and Aderjan R

Subjects

Chromatography, Liquid, Drug Stability, Humans, Mass Spectrometry, Time Factors, Hallucinogens urine, Lysergic Acid Diethylamide analogs & derivatives, Lysergic Acid Diethylamide urine

Published

2002

203. Affinities of dihydrocodeine and its metabolites to opioid receptors.

Author

Schmidt H, Vormfelde Sv, Klinder K, Gundert-Remy U, Gleiter CH, Skopp G, Aderjan R, and Fuhr U

Subjects

Animals, Binding, Competitive drug effects, Cells, Cultured, Enkephalin, Ala(2)-MePhe(4)-Gly(5)- metabolism, Female, Guinea Pigs, Male, Membranes drug effects, Membranes metabolism, Structure-Activity Relationship, Analgesics, Opioid metabolism, Codeine analogs & derivatives, Codeine metabolism, Receptors, Opioid agonists, Receptors, Opioid metabolism

Abstract

Dihydrocodeine is metabolized to dihydromorphine, dihydrocodeine-6-O-, dihydromorphine-3-O- and dihydromorphine-6-O-glucuronide, and nordihydrocodeine. The current study was conducted to evaluate the affinities of dihydrocodeine and its metabolites to mu-, delta- and kappa-opioid receptors. Codeine, morphine, d,1-methadone and levomethadone were used as controls. Displacement binding experiments were carried out at the respective opioid receptor types using preparations of guinea pig cerebral cortex and the specific opioid agonists [5H]DAMGO (mu-opioid receptor), [3H]DPDPE (delta-opioid receptor) and [3H]U69,593 (K-opioid receptor) as radioactive ligands at concentrations of 0.5, 1.0 and 1.0 nmol/l, respectively. All substances had their greatest affinity to the mu-opioid receptor. The affinities of dihydromorphine and dihydromorphine-6-O-glucuronide were at least 70 times greater compared with dihydrocodeine (Ki 0.3 micromol/l), whereas the other metabolites yielded lower affinities. For the delta-opioid receptor, the order of affinities was similar with the exception that dihydrocodeine-6-O-glucuronide revealed a doubled affinity in relation to dihydrocodeine (Ki 5.9 micromol/l). In contrast, for the K-opioid receptor, dihydrocodeine-6-O- and dihydromorphine-6-O-glucuronide had clearly lower affinities compared to the respective parent compounds. The affinity of nordihydrocodeine was almost identical to that of dihydrocodeine (Ki 14 micromol/l), whereas dihydromorphine had a 60 times higher affinity. These results suggest that dihydromorphine and its 6-O-glucuronide may provide a relevant contribution to the pharmacological effects of dihydrocodeine. The O-demethylation of dihydrocodeine to dihydromorphine is mediated by the polymorphic cytochrome P-450 enzyme CYP2D6, resulting in different metabolic profiles in extensive and poor metabolizers. About 7% of the caucasian population which are CYP2D6 poor metabolizers thus may experience therapeutic failure after standard doses.

Published

2002

204. 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

205. 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

206. 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

207. [Serum beta-glucuronidase activity in polytrauma patients and in centrifuged autopsy blood samples].

Author

Pötsch L and Skopp G

Subjects

Humans, Hydrogen-Ion Concentration, Multiple Trauma enzymology, Multiple Trauma pathology, Reference Values, Autopsy legislation & jurisprudence, Glucuronidase blood, Multiple Trauma diagnosis, Postmortem Changes

Abstract

The serum activity of beta-glucuronidase was investigated in 58 patients after severe trauma as well as in 43 autopsy cases. In 10 cases the enzyme activities in postmortem blood samples from the femoral vein were compared to those present in the correspondent heart blood samples. An elevated activity of beta-glucuronidase was observed in 14% of the patients within the first 36 h after severe trauma increasing to 62% in blood samples collected later on. The activity of beta-glucuronidase in the heart blood samples was always higher than in the corresponding sample from the femoral vein. In cases of prolonged post-mortem interval an elevated activity might have been due to bacterial contamination. In postmortal blood samples from the femoral vein an elevated enzyme activity was found in 70% of the study material. The results of the preliminary study on the activity of beta-glucuronidase in blood samples frequent in forensic routine work indicated that an elevated enzyme activity might be present for the following scenery: after severe trauma, in alcohol/drug abuse, presence of putridity/autolysis, presence of inflammatory processes, in diabetes as well as in carcinoma diseases. The significance of elevated beta-glucuronidase activity concerning alterations of unconjugated drug concentration due to in vitro cleavage of O-glucuronides should be investigated.

Published

2001

208. Analysis of cocaine, benzoylecgonine, ecogonine methyl ester, and ecgonine by high-pressure liquid chromatography-API mass spectrometry and application to a short-term degradation study of cocaine in plasma.

Author

Klingmann A, Skopp G, and Aderjan R

Subjects

Chromatography, High Pressure Liquid methods, Cocaine chemistry, Dopamine Uptake Inhibitors chemistry, Humans, Hydrolysis, Mass Spectrometry, Narcotics chemistry, Sensitivity and Specificity, Specimen Handling, Time Factors, Artifacts, Cocaine analogs & derivatives, Cocaine blood, Dopamine Uptake Inhibitors blood, Narcotics blood

Abstract

A method for the determination of cocaine (COC), benzoylecgonine (BE), ecgonine methyl ester (EME), and ecgonine (ECG) in plasma by liquid chromatography-mass spectrometry (LC-MS-MS) was developed. The analytes were isolated from human plasma by subsequent solid-phase extraction and were separated on a Zorbax Eclipse XDB-C8 narrow-bore column using an ammonium acetate buffer/acetonitrile/methanol gradient. A Turbolonspray source was used for ionization. The analytes were characterized by their particular molecular ion and several fragments. Multiple reaction monitoring (MRM) was used for isolation and quantitation. The assay was rapid, highly sensitive, and reliable. The method was applied to monitor the in vitro degradation of cocaine in plasma. Fresh unpreserved and preserved (0.25% KF) plasma samples were spiked with 1,000 ng cocaine/mL. Aliquots of both series were stored at 4 degrees C and 20 degrees C and were analyzed at selected storage times of up to 15 days. In all samples, degradation of cocaine that was dependent on storage time and temperature and on sample preservation could be observed. The formation of BE did not occur to a significant extent (< 12%, referred to the initial concentration of COC), and its concentration was slightly higher in preserved compared with unpreserved plasma at both storage temperatures chosen. EME was formed in considerably higher amounts compared to BE. As already observed for COC, its formation and degradation were dependent on storage time, temperature, and preservation. EME is suggested to be the major source of ECG, which was detectable in all samples after 1-2 days of storage. Although the degradation of COC was shown to be highly dynamic in nature, the sum of all hydrolysis products of COC accounted for the initial COC concentration at any particular time of storage. Therefore, production of hitherto unknown degradation products of COC seems unlikely. Moreover, the common transformation product of BE and EME appeared to be stable, and ECG is suggested as a promising postcollection artifact.

Published

2001

209. [Passive exposure in detection of low blood and urine cannabinoid concentrations].

Author

Skopp G and Pötsch L

Subjects

Automobile Driving legislation & jurisprudence, Dronabinol pharmacokinetics, Humans, Marijuana Smoking metabolism, Metabolic Clearance Rate physiology, Social Environment, Cannabinoids pharmacokinetics, Marijuana Smoking legislation & jurisprudence, Substance Abuse Detection legislation & jurisprudence, Tobacco Smoke Pollution

Abstract

Whenever small amounts of drugs are present in blood or urine samples, especially of substances that are preferentially smoked such as cannabinoids, the discrimination between active and passive inhalation may cause severe problems. The statement of a passive exposure by marijuana smoke has been scrutinized reviewing the literature. The pharmacokinetics of smoked marijuana as well as experimental data on cannabinoid concentrations in plasma and urine samples following passive exposure are summarized. As a conclusion it seems urgent to enlarge the existing data base.

Published

2001

210. In vitro stability of cocaine in whole blood and plasma including ecgonine as a target analyte.

Author

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

Subjects

Chromatography, High Pressure Liquid, Humans, Hydrolysis, Indicators and Reagents, Mass Spectrometry, Plasma chemistry, Specimen Handling, Temperature, Cocaine analogs & derivatives, Cocaine blood

Abstract

The in vitro stability of cocaine (COC) was monitored in fresh whole blood and plasma stabilized with potassium fluoride (0.25%) for as long as 15 days. The samples were stored at 4 degreesC, 20 degreesC and 40 degreesC. Additionally, fresh plasma samples containing either benzoylecgonine (BZE), ecgonine methyl ester (EME) or ecgonine (ECG) were stored at 4 degreesC and 20 degreesC. Data were established using subsequent solid-phase extraction procedures and high-performance liquid chromatography coupled to atmospheric pressure ionization mass spectrometry for isolation and quantitation of COC, BZE, EME, and ECG. COC, BZE, and EME concentrations decreased with increasing storage temperature and time after an apparent first-order reaction kinetic. Only ECG appeared to be stable at storage temperatures as high as 20 degreesC for the entire observation period. At 40 degreesC, the amount of ECG produced from hydrolysis of COC still totalled 80% of the initial COC concentration. Hydrolysis of COC to EME occurred more rapidly in plasma than in blood. The dynamic degradation profiles obtained were dependent on the storage temperature. The conversion of COC to BZE, EME, and ECG appeared to be stoichiometric at all time intervals at storage temperatures of 4 degreesC and 20 degreesC. The presence of any hydrolysis product of COC in blood or plasma constitutes confirmatory evidence of COC incorporation, and determination of ECG seems most promising even in samples stored under unfavorable conditions.

Published

2001

211. [Detection of cocaine in blood stains].

Author

Skopp G and Pötsch L

Subjects

Blood Preservation, Germany, Humans, Predictive Value of Tests, Accidents, Traffic legislation & jurisprudence, Blood Stains, Cocaine analysis

Abstract

Cocaine is rapidly degraded in blood samples, and its degradation was found to be highly dynamic in nature. The analysis of blood spots dried on filter paper may provide a method to minimize the break-down of cocaine and to largely preserve the analytical profile of the parent drug and its hydrolysis products at the time of sampling. The short term stability of cocaine in 100 microL blood spots prepared from unpreserved and preserved (sodium fluoride, 0.25%) blood samples was compared to the stability of the particular whole blood specimens stored in tubes at ambient temperature and at -20 degrees C. Due to dehydration, both the chemical and the enzymatic hydrolysis of cocaine and its products could be stopped in dried blood spots. More than 75% of the initial cocaine concentration could be detected in the blood spots, and the analytical profile was ensured for 17 days. Provided its practical suitability, the spot technology should offer a simple approach to detect actual impairment of motorists taken in police custody in the view of section 24a of the German traffic act as well as in cocaine associated criminal cases.

Published

2001

212. Saliva testing after single and chronic administration of dihydrocodeine.

Author

Skopp G, Pötsch L, Klinder K, Richter B, Aderjan R, and Mattern R

Subjects

Biotransformation, Codeine pharmacokinetics, Codeine therapeutic use, Double-Blind Method, Heroin Dependence drug therapy, Heroin Dependence metabolism, Humans, Codeine analogs & derivatives, Codeine analysis, Saliva chemistry, Substance Abuse Detection methods

Abstract

In the present study, concentrations of dihydrocodeine and its metabolites in saliva and serum were compared after single low-dose and chronic high-dosage administration of the drug. In the first investigation, blood and saliva were collected periodically from six subjects after oral administration of 60 mg dihydrocodeine. In the second study, 20 subjects on oral dihydrocodeine maintenance provided single samples of blood and saliva simultaneously. Serum protein binding of salivary analytes and their recovery from the adsorbing material of the collection device as well as pH values of saliva samples were determined. The fluids were analyzed for dihydrocodeine and the major metabolites by high-performance liquid chromatography. In the single dose study dihydrocodeine was the only analyte found in saliva for up to 12-24 h post-dose. The half-life of dihydrocodeine in saliva was about twice that found in blood. The ratios of saliva/serum concentrations ranged from 1.2 to 17.0. After chronic high-dosage use, dihydrocodeine was the main salivary analyte and N-nordihydrocodeine was present in a few samples. Saliva/serum concentration ratios of dihydrocodeine were strongly dependent on the pH value of saliva and, to a lesser extent, on serum-protein binding. The saliva/serum ratios were more similar after chronic administration. The data suggest a passive diffusion process as the underlying mechanism for the transport of dihydrocodeine into saliva. After both single and chronic use, the presence of the drug in saliva can be used as evidence of recent substance administration.

Published

2001

213. 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

214. Stability of cannabinoids in hair samples exposed to sunlight.

Author

Skopp G, Pötsch L, and Mauden M

Subjects

Cannabidiol analysis, Cannabidiol radiation effects, Cannabinoids analysis, Cannabinol analysis, Dronabinol analysis, Hair chemistry, Humans, Specimen Handling, Cannabinoids radiation effects, Hair radiation effects, Substance Abuse Detection methods, Sunlight

Published

2000

215. [Distribution of morphine and morphine glucuronides in body tissue and fluids--postmortem findings in brief survival].

Author

Klingmann A, Skopp G, Pedal I, Pötsch L, and Aderjan R

Subjects

Autopsy legislation & jurisprudence, Female, Humans, Middle Aged, Morphine pharmacokinetics, Tissue Distribution, Drug Overdose pathology, Morphine poisoning, Morphine Derivatives pharmacokinetics, Postmortem Changes, Suicide legislation & jurisprudence

Abstract

An intoxication following administration of morphine, tramadol and atracurium in a suicide case is reported. The route of administration and the amount of the particular drug were known from the investigation of the death scene and the findings of the postmortem examination. Tramadol was present in the gastric contents as well as in blood, liver, kidney and brain samples, whereas the drug could not be detected in muscle. All body fluids and tissues investigated contained morphine as well as its 3- and 6-glucuronides with the exception of muscle tissue. The concentrations of morphine and its glucuronide metabolites were determined by LC/MS following solid phase extraction. Interestingly, the concentration of M6G in brain, liver and kidney were close to the concentration of M3G in the particular tissue. This phenomenon might be explained by a preferential hydrolysis of M3G or by a preferential formation of M6G postmortem. Measurement of morphine and M6G in femoral blood and cerebrospinal fluid may be a useful indicator in rapid deaths.

Published

2000

216. [Serotonin, 5-hydroxyindolylacetic acid and cholesterol content in blood, cerebrospinal fluid and brain areas for differentiation of suicidal from non-suicidal cause of death].

Author

Walendzik H, Zimmer G, and Skopp G

Subjects

Adult, Aged, Cause of Death, Female, Humans, Male, Middle Aged, Postmortem Changes, Predictive Value of Tests, Reference Values, Brain Chemistry, Cholesterol analysis, Hydroxyindoleacetic Acid analysis, Serotonin analysis, Suicide legislation & jurisprudence

Abstract

In the present study serotonin and its metabolite 5-hydroxyindoleacetic acid was investigated in the cerebrospinal fluid and in discrete brain areas of the left and right hemisphere collected from 34 bodies. Sixteen subjects were suicide victims, and 18 were matched as controls. Matching was done for gender, age, sex and cause of death. In suicide victims the concentration of 5-hydroxyindoleacetic acid in cerebrospinal fluid (occipital) was significantly decreased whereas there was no difference comparing the particular results established from the various brain areas. Nevertheless, there was a non-significant trend towards a higher concentration of serotonin in the thalamic area and towards a lower level in samples collected from the mesencephalon in suicide brains. In suicide subjects, the level of 5-hydroxyindoleacetic acid was often found to be increased in the hippocampus and to be decreased in the thalamus. A differentiation between suicide and homicide seems promising only on condition that the distribution of serotonin and metabolite concentrations in various brain areas is considered. The amount of total cholesterol in blood is suggested to be of limited value.

Published

2000

217. Ethyl glucuronide in human hair.

Author

Skopp G, Schmitt G, Pötsch L, Drönner P, Aderjan R, and Mattern R

Subjects

Biomarkers analysis, Case-Control Studies, Humans, Skin chemistry, Alcohol Drinking, Alcoholism diagnosis, Glucuronates analysis, Hair chemistry

Abstract

Ethyl glucuronide (EtG) is considered to be a promising candidate marker of alcohol consumption, but exhibits a short window of detection in blood or urine. Keratinized tissues are known to retain foreign substances and to provide a greater retrospective window of detection than body fluids. Therefore, post-mortem hair, skin swabs, and stratum corneum samples were collected from four subjects with a reported history of alcohol misuse and from seven subjects with a report of regular, socially accepted drinking behaviour, and were investigated for EtG. Additionally, certain specimens were collected from three children, who had not yet consumed any alcoholic beverages. EtG was detectable in most of the hair and stratum corneum samples as well as in perspiration stains from alcohol-consuming subjects. The results indicated that EtG might be formed locally in very small and highly variable amounts. The most important finding was that EtG cannot be expected to be generally detectable in keratinized tissues or perspiration stains from alcohol-drinking subjects, whereas a positive result is always associated with recent alcohol consumption.

Published

2000

218. Effect of the shampoo Ultra Clean on drug concentrations in human hair.

Author

Röhrich J, Zörntlein S, Pötsch L, Skopp G, and Becker J

Subjects

Forensic Medicine methods, Humans, Hair chemistry, Hair Preparations, Substance Abuse Detection

Abstract

The influence of the special shampoo Ultra Clean (Zydot Unlimited, Tulsa, Oklahoma) on the results of hair analyses was investigated. Hair samples from persons (n = 14) with a known history of drug abuse were collected at autopsy. The hair samples were divided into separate strands which were analyzed both after washing with Ultra Clean and without treatment. Hair analyses were performed by methanol extraction under sonication, purification by solid phase extraction and GC/MS in SIM mode according to routine procedures for tetrahydrocannabinol (THC), cocaine, amphetamine, methylenedioxyamphetamine (MDA), methylenedioxymethamphetamine (MDMA), methylenedioxyethylamphetamine (MDE), heroin, 6-monoacetylmorphine (6-MAM), morphine, codeine, dihydrocodeine and methadone. All drugs originally present in the hair fibers were still detected after a single application of Ultra Clean. However, a slight decrease in drug concentrations could mostly be observed e.g. cocaine (n = 10) -5%, 6-MAM (n = 12) -9%, morphine (n = 12) -26%, THC (n = 4) -36%. The findings clearly demonstrated that drug substances had not been sufficiently removed from human hair by a single Ultra Clean treatment to drop their concentrations below the limit of detection of the analytical method applied.

Published

2000

219. Report on intrauterine drug exposure during second trimester of pregnancy in a heroin-associated death.

Author

Pötsch L, Skopp G, Emmerich TP, Becker J, and Ogbuhui S

Subjects

Adolescent, Amniotic Fluid chemistry, Autopsy, Body Fluids chemistry, Codeine analysis, Fatal Outcome, Female, Fetus chemistry, Gas Chromatography-Mass Spectrometry, Hair chemistry, Humans, Male, Morphine Derivatives analysis, Pregnancy, Pregnancy Trimester, Second, Tissue Distribution, Fetus metabolism, Heroin metabolism, Heroin poisoning, Maternal-Fetal Exchange, Opioid-Related Disorders metabolism, Pregnancy Complications metabolism

Abstract

A 17-year-old girl was found dead in a public toilet with fresh needle puncture marks. She was 18-20 weeks pregnant with a male fetus. Drug screening of her blood and urine indicated recent heroin use. Chronic drug use was confirmed by hair analysis. Amniotic fluid as well as fetal and maternal tissues and body fluids were analyzed by GC/MS and HPLC. All the fetal specimens were investigated, and the following levels of drugs were found: 6-monoacetyl-morphine (blood: 152 ng/g; amniotic fluid: 128 ng/g; brain: 140 ng/g; lung: 110 ng/g; liver: 2 ng/g; kidney: 40 ng/g), morphine (blood: 1360 ng/g; amniotic fluid: 604 ng/g; brain: 710 ng/g; lung: 1030 ng/g; liver: 2060 ng/g; kidney: 1100 ng/g), codeine (blood: 70 ng/g; brain: 60 ng/g; lung: 60 ng/g; liver: 90 ng/g; kidney: 70 ng/g), and morphine-3-glucuronide (amniotic fluid: 209 ng/g; brain: 170 ng/g; lung: 325 ng/g; kidney: 231 ng/g). Morphine-6-glucuronide was present in the maternal circulation but could not be detected in the fetal circulation.

Published

1999

220. The influence of the route of administration: a comparative study at steady state of oral sustained release morphine and morphine sulfate suppositories.

Author

Du X, Skopp G, and Aderjan R

Subjects

Administration, Oral, Administration, Rectal, Analgesics, Opioid blood, Area Under Curve, Chemistry, Pharmaceutical, Chromatography, High Pressure Liquid, Delayed-Action Preparations, Female, Humans, Male, Middle Aged, Morphine blood, Morphine Derivatives blood, Pain, Intractable drug therapy, Suppositories, Analgesics, Opioid administration & dosage, Analgesics, Opioid pharmacokinetics, Morphine administration & dosage, Morphine pharmacokinetics, Morphine Derivatives administration & dosage, Morphine Derivatives pharmacokinetics

Abstract

Steady state pharmacokinetics of morphine (M), morphine-3-glucuronide (M3G) and morphine-6-glucuronide (M6G) were investigated in 6 patients with intractable cancer pain administered orally with MST (Mundipharma, Limburg, Germany) and, subsequently, rectally with MSR to make a judgment whether orally administered morphine can be replaced by rectally administered morphine. The parent drug and glucuronide metabolites were measured simultaneously using high-performance liquid chromatography (HPLC) and native fluorescence detection. The mean morphine area under the curve (AUC) value (0-8 h) was smaller (434.3 +/- 170.2 nmolL(-1)h) in the oral administration than in the rectal administration (574.8 +/- 285.0 nmolL(-1)h) (p < 0.05). The rectal administration resulted in less production of M3G and M6G. There were no significant differences in the mean steady state concentrations (C(ss)) of morphine, M3G, and M6G between the oral and rectal administrations (p > 0.05). The median AUC ratio--M3G/M and M6G/M, 12.58 and 1.85--following MSR rectal administration was smaller than following MST oral administration in 6 patients (19.97 and 2.59; p < 0.05), whereas the median AUC ratio M3G/M6G in the rectal dosing was 6.24 (range 5.2-7.6) was almost the same as the median ratio M3G/M6G in the oral dosing was 6.49 (range 5.8-8.5; p > 0.1). Four of the 6 patients had a greater Cmax of M3G and M6G after oral administration than after rectal administration. The same 4 had lower fluctuation rates for morphine, M3G (p < 0.05), and M6G (p < 0.05) after rectal administration. Therefore, during chronic morphine treatment, it still seems difficult to decide whether oral administration can be replaced by rectal administration.

Published

1999

221. The detection of dihydrocodeine and its main metabolites in cases of fatal overdose.

Author

Klinder K, Skopp G, Mattern R, and Aderjan R

Subjects

Adult, Analgesics, Opioid metabolism, Chromatography, High Pressure Liquid, Codeine metabolism, Codeine poisoning, Dihydromorphine metabolism, Drug Overdose, Forensic Medicine, Humans, Male, Poisoning diagnosis, Analgesics, Opioid poisoning, Codeine analogs & derivatives

Abstract

The levels of dihydrocodeine found in impaired individuals and in fatalities show a wide overlap in the ranges. Among other factors, the genetically controlled metabolism of dihydrocodeine should play an important role in dihydrocodeine toxicity. For the first time, the most important metabolites of dihydrocodeine were investigated in femoral blood from three fatal cases by simultaneous determination using HPLC and native fluorescence for detection. The amount of parent drug always exceeded dihydrocodeine-glucuronide formation and dihydromorphine concentrations ranged from 0.16-0.21 mg/L. The similar binding affinities of dihydromorphine and morphine to mu-opioid receptors suggest similar pharmacological effects and adverse reactions. The determination of the pharmacologically active metabolites should help to clarify the cause of death in fatal cases especially if a relatively low concentration of the parent drug is found.

Published

1999

222. Perspiration versus saliva--basic aspects concerning their use in roadside drug testing.

Author

Skopp G and Pötsch L

Subjects

Drug Monitoring, Humans, Illicit Drugs pharmacokinetics, Sensitivity and Specificity, Illicit Drugs analysis, Saliva chemistry, Substance Abuse Detection legislation & jurisprudence, Sweat chemistry

Abstract

Various aspects concerning the practical application and forensic interpretation of data obtained by saliva drug testing and drug monitoring from the skin surface are discussed. Basic information on the composition of saliva and skin secretions and their particular transport mechanisms, as far as known, are given. For drugs of abuse secretion into saliva is suggested to be by passive diffusion and to depend on lipid solubility, pKa, plasma protein binding and on the pH of saliva. Drug molecules from blood are considered to reach the skin surface by various routes such as by sweat and sebum as well as by inter- and/or transcellular diffusion. The role of the stratum corneum as a temporary drug reservoir exceeding positive drug findings in urine is outlined. Current data on opioids, cocaine metabolites, cannabinoids and amphetamines detected in saliva and on the skin surface are reviewed. Aspects of collection, processing and analysis of the samples for implementation in roadside testing are addressed. The requirement of test sensitivity covering the broad concentration ranges and the importance of test specificity bearing in mind that the parent drug is the main analyte present in those specimens is stressed. Theoretical and practical findings on frequently abused drugs are discussed with regard to the possibilities and limitations of drug monitoring from saliva and perspiration to support a suspicion of actual or recent drug administration.

Published

1999

223. Hemoglobin diffusion across a venous wall: an experimental study.

Author

Skopp G, Pötsch L, Lutz R, Ganssmann B, and Mattern R

Subjects

Diffusion, Hemolysis, Humans, Hydrogen-Ion Concentration, In Vitro Techniques, Permeability, Hemoglobins metabolism, Veins metabolism

Abstract

The aim of this study was to investigate the permeation behavior of a large molecule through a venous wall; hemoglobin was chosen as a model substance. In vitro experiments were performed using a Chien-Valia diffusion chamber. Postmortem, hemolyzed, and fresh nonhemolyzed blood samples were investigated as permeants. Vein patches from vena cava inferior and vena jugularis interna were used as diffusion barriers. Applying this technique, extravasation of hemoglobin was detectable. The portion of hemoglobin molecules passing through the vascular wall depended on time, vein type, and graduation of hemolysis. The passage of hemoglobin across the wall of a large vein suggests intravascular changes in drug concentrations from postmortem blood samples not to be restricted on the unbound portion of the particular drug.

Published

1998

224. Formation and clearance of active and inactive metabolites of opiates in humans.

Author

Aderjan RE and Skopp G

Subjects

Analgesics, Opioid blood, Chromatography, High Pressure Liquid, Codeine blood, Codeine pharmacokinetics, Drug Overdose, Heroin blood, Humans, Narcotics blood, Toxicology methods, Analgesics, Opioid pharmacokinetics, Codeine analogs & derivatives, Heroin pharmacokinetics, Narcotics pharmacokinetics

Abstract

The results of recent investigations of the analgesic and the nonanalgesic effects of opioid glucuronides are relevant to the research on drug abuse in forensic toxicology. As has been shown for heroin, knowledge of the state of distribution and elimination of active and inactive metabolites and glucuronides offers new possibilities in forensic interpretation of analytic results. Because of similar metabolic degradation, calculation of the time-dependent ratio of the concentration of morphine and its glucuronide metabolites in blood or serum allows a rough estimation of increased dosage and of time elapsed since the last application. Drug effects can be examined with respect to individual case histories, including overdose and survival time if the patient died. However, different methods of administration and the strong influence of different volumes or compartments of distribution of parent compounds and metabolites on concentrations in human body tissues require careful use of glucuronide concentration data. In Germany, dihydrocodeine (DHC) is prescribed as a heroin substitute, and relative overdoses are needed to be effective. DHC metabolism was studied in three patients who died from overdoses. All metabolites (dihydrocodeine-6-glucuronide [DHC6], nor-DHC [NDHC], dihydromorphine [DHM], nor-DHM [NDHM], and DHM-3- and 6-glucuronide [DHM3G, DHM6G]) were determined using HPLC and fluorescence detection. Concentrations of DHM (0.16 mg/L to 0.22 mg/L serum) were found. The DHM glucuronide ratios were similar to those of morphine. Receptor binding studies showed that the binding affinity of DHM to porcine mu-receptor was higher than that of morphine, and DHM6G's binding affinity was as high as that of morphine-6-glucuronide (M6G). Metabolites may play an important role in the effectiveness of DHC in substitution and toxicity. Because of enzyme polymorphism, the formation of DHC poses a risk for proper dosage in patients who are either poor or extensive metabolizers. The distribution of opioid glucuronides in cerebral spinal fluid in relation to transcellular transport in central nervous tissue is discussed with respect to the receptor binding of opiates and drug effect.

Published

1998

225. A preliminary study on the distribution of morphine and its glucuronides in the subcompartments of blood.

Author

Skopp G, Pötsch L, Ganssmann B, Aderjan R, and Mattern R

Subjects

Centrifugation, Erythrocytes chemistry, Hematocrit, Humans, Morphine Derivatives blood, Morphine Derivatives pharmacokinetics, Morphine blood, Morphine pharmacokinetics

Abstract

The distribution of morphine, morphine-3-glucuronide (M3G), and morphine-6-glucuronide (M6G) in whole blood, plasma, and packed erythrocytes was studied. Parameters investigated were the hematocrit values (10, 42, 44, and 71%) and the water content of the samples. The blood-to-plasma ratio of morphine concentrations was unaffected by variations in hematocrit and water content, whereas the corresponding ratios for M3G and M6G were strongly influenced. Ratios were 0.53 to 0.65 and 0.52 to 0.62 in specimens with average hematocrit values (42 and 44%, respectively), and the ratios were 0.81 or 0.89 (hematocrit 10%) and 0.27 or 0.28 (hematocrit 71%) in blood samples with different hematocrit values. In contrast to the morphine conjugates, morphine was highly bound to or partitioned into red blood cells (beta e = 55.9). Although the present data are limited, they already demonstrate that conclusions drawn from pharmacokinetic studies and transferred to parent drug to metabolite ratios resulting from forensic blood samples may be biased by the particular biological matrix under investigation.

Published

1998

226. [Fatal poisoning with clozapine and perazine. A case report].

Author

Ganssmann B, Skopp G, Aderjan R, and Mattern R

Subjects

Adult, Antipsychotic Agents therapeutic use, Cause of Death, Clozapine therapeutic use, Dose-Response Relationship, Drug, Drug Therapy, Combination, Female, Humans, Male, Perazine therapeutic use, Psychotic Disorders drug therapy, Psychotic Disorders mortality, Suicide, Attempted legislation & jurisprudence, Antipsychotic Agents poisoning, Clozapine poisoning, Drug Overdose etiology, Perazine poisoning, Suicide legislation & jurisprudence

Abstract

An intoxication following an apparent overdose of clozapine (Leponex) and perazine (Taxilan) is reported. There was a wide range of variation in postmortem blood and tissue concentrations of clozapine, desmethyclozapine and perazine. Clozapine/norclozapine blood and tissue ratios and perazine-pill-fragments in the gastric content could be used as a sign of suspected acute clozapine and perazine overdose.

Published

1998

227. A preliminary study on the stability of benzodiazepines in blood and plasma stored at 4 degrees C.

Author

Skopp G, Pötsch L, König I, and Mattern R

Subjects

Chromatography, Gas, Forensic Medicine, Humans, Linear Models, Reference Values, Refrigeration, Benzodiazepines pharmacokinetics, Blood metabolism, Plasma metabolism, Specimen Handling, Substance Abuse Detection

Abstract

An approach to determine the stability of benzodiazepines and some of their metabolites (n = 13) by means of a routinely applied gas chromatographic method using electron capture detection was made in this preliminary study. Validation data of the method are given. Spiked blood and plasma samples were stored at 4 degrees C and analysed at selected times up to 240 days. The concentrations of all analytes had decreased to at least 60% of the original levels at the end of the observation period. A clear pattern of breakdown could not be established. The data obtained suggest that results from long-term stored samples should be interpreted cautiously. Further investigations concerning the stability of drugs in blood and plasma samples, additional methods of identification and determination as well as the establishment of optimal storage conditions seem necessary.

Published

1998

228. Surgical management of intraosseous skull base tumors with aid of Operating Arm System.

Author

Schul C, Wassmann H, Skopp GB, Marinov M, Wölfer J, Schuierer G, Joos U, and Willich N

Subjects

Adult, Chordoma surgery, Female, Humans, Magnetic Resonance Imaging, Male, Meningioma surgery, Middle Aged, Tomography, X-Ray Computed, Skull Base Neoplasms surgery, Therapy, Computer-Assisted methods

Abstract

Invasion of bone and critical neurovascular structures often impedes complete resection of intraosseous skull base neoplasms, and these lesions tend to recur unless all infiltrated bone is removed. Evolving experience with image guidance over the past few years indicates the potential value of neuronavigation in skull base lesions diffusely infiltrating or fixed to bone structures. We report our early experience with the Radionics Operating Arm System (OAS), specifically emphasizing its utility as an adjunct in the treatment of intraosseous skull base tumors, mainly meningiomas. In April 1995 the OAS was introduced into clinical use at the neurosurgical university clinic in Münster, Germany. Since then, the system's utility has been explored in 10 patients out of the total neuronavigation series presenting with intraosseous skull base tumors (nine females and one male, mean age 47 years; nine meningiomas, one chordoma). For navigational planning, both 3-mm computed tomography scans and a set of 3-mm fat-suppression magnetic resonance images were chosen. At least four adhesive skin markers were used for system calibration. The system was technically usable in all cases in this small series. Because of the relative immobility of the bone structures and/or the tumor, no significant deviation from the preoperative registration accuracy was noted at the end of the procedures. The main advantages were easier localization and resection of infiltrated bone, which is often not grossly identifiable, even under the microscope. Our preliminary experience with the OAS suggests that image guidance is helpful in this type of lesion, providing better anatomical orientation during surgery and delineating tumor margins and their relation to critical neurovascular structures. The problem of a possible intracranial tumor and brain shift can be neglected in these lesions. The system facilitates resection by volumetric contour information, allowing more aggressive and complete resection.

Published

1998

229. Influence of pigmentation on the codeine content of hair fibers in guinea pigs.

Author

Pötsch L, Skopp G, and Moeller MR

Subjects

Animals, Binding Sites, Drinking, Forensic Medicine methods, Gas Chromatography-Mass Spectrometry, Guinea Pigs, Codeine pharmacokinetics, Hair metabolism, Hair Color, Melanins metabolism

Abstract

Tortoise shell guinea pigs (n = 7) were administered codeine (1 mg/mL codeine-base) in their drinking water for 3 weeks. Black, reddish-brown and white hair was collected separately from each animal before and after treatment. The hair samples were analyzed by GC/MS. The experiment showed positive results for all hair fibers with large individual variability of drug incorporation. Low drug intake resulted in small differences of the drug content in hair fibers different in color, whereas in cases of high drug intake a strong influence of hair pigmentation on the analytical results was observed. The highest drug content was always found in black hair samples, non-pigmented hair showed the lowest drug concentrations and the drug content in reddish-brown fibers was less than in black hair samples from the same animal. From the results it was concluded, that eumelanins rather than phenomelanins are the decisive factor for codeine-melanin binding in hair and the amount of drug intake was suggested to determine the relevance of hair pigmentation on the analytical results.

Published

1997

230. Ethyl glucuronide concentration in serum of human volunteers, teetotalers, and suspected drinking drivers.

Author

Schmitt G, Droenner P, Skopp G, and Aderjan R

Subjects

Adult, Automobile Driving, Female, Gas Chromatography-Mass Spectrometry, Humans, Male, Middle Aged, Alcohol Drinking blood, Alcoholic Intoxication blood, Ethanol pharmacokinetics, Forensic Medicine methods, Glucuronates blood, Tea

Abstract

The kinetic profile of ethanol and ethyl glucuronide (EtG) in serum was investigated in three subject groups: 1) Healthy, moderately drinking volunteers (daily intake less than 30 g ethanol) who ingested a single dose of ethanol. In this group the maximum of serum ethyl glucuronide concentration (SEtGC) and of serum ethanol concentration (SEC) did not exceed 3.7 mg/L and 1.5 g/L respectively. EtG peaked 2 to 3.5 h later than ethanol. EtG was eliminated with a terminal half-life of 2 to 3 h. EtG decreased slower than ethanol--the metabolite could still be determined in serum up to 8 h after complete ethanol elimination. 2) In serum samples of teetotalers neither ethanol nor EtG could be found. 3) In 37 of 50 serum samples of drivers suspected of driving under the influence of ethanol, SEtGC was found between the limit of detection (0.1 mg/L) and 20 mg/L. If the SEC is less than 1 g/L and the SEtGC is significantly higher than 5 mg/L, we assume alcohol misuse.

Published

1997

231. A case report on drug screening of nail clippings to detect prenatal drug exposure.

Author

Skopp G and Pötsch L

Subjects

Female, Humans, Infant, Male, Mass Spectrometry, Pregnancy, Substance-Related Disorders, Tricuspid Valve abnormalities, Cocaine analysis, Nails chemistry, Narcotics analysis, Prenatal Exposure Delayed Effects, Sudden Infant Death

Abstract

In a case of a sudden infant death syndrome-related death of a 3-month-old infant, nail clippings were positive for cocaine by gas chromatography-mass spectroscopy analysis that revealed a prenatal exposure to the drug substance. In utero exposure to drugs has been investigated using amniotic fluid, neonatal urine, meconium, and hair samples. Nail analysis offers some advantage over hair analysis because of its continuous growth and persistence after delivery. Nail material is easy to sample in suitable amounts. Currently, the cocaine finding cannot be related to the underlying cause of death. However, this observation indicates that nail analysis may be a new and valuable tool to screen newborns for intrauterine drug exposure. In addition, it can help collect information on the prevalence of possible embryotoxic effects and the link to postnatal manifestations of different dysfunctions in infants who are born by drug abusing mothers.

Published

1997

232. [Storage stability of flunitrazepam, flurazepam, diazepam and metabolites in blood and plasma].

Author

König I, Skopp G, Schmitt G, and Mattern R

Subjects

Biotransformation, Drug Stability, Drug Storage, Humans, Pilot Projects, Temperature, Anti-Anxiety Agents pharmacokinetics, Blood Preservation, Diazepam pharmacokinetics, Flunitrazepam pharmacokinetics, Flurazepam pharmacokinetics

Abstract

The stability of flunitrazepam, flurazepam, diazepam and some of their metabolites in spiked blood and plasma samples was studied bei GC-ECD analysis at defined time intervals up to 240 days. Validation data of the method are given. The blood or plasma samples were stored either at 22 degrees C or at 4 degrees C, and were exposed to global natural light irradiation or protected from light. All substances considerably decreased during the time interval studied. Flunitrazepam soon disappeared completely at room temperature (22 degrees C), while diazepam and flurazepam proved to be more stable, but a clear pattern of breakdown could not be established. The data obtained suggest a result from a long-term stored sample to be cautiously interpreted. Further investigation concerning the stability of drugs and the establishment of optimal storage conditions seem necessary.

Published

1997

233. An in vitro experiment for postmortem vascular permeation. The passage of morphine and morphine glucuronides across a vascular wall.

Author

Skopp G, Lutz R, Pötsch L, Ganssmann B, Klinder K, Schmidt A, Aderjan R, and Mattern R

Subjects

Biological Transport, Diffusion Chambers, Culture, Dose-Response Relationship, Drug, Fluorescent Dyes, Humans, Rhodamines, Vena Cava, Inferior metabolism, Endothelium, Vascular metabolism, Morphine pharmacokinetics, Morphine Derivatives pharmacokinetics, Postmortem Changes

Abstract

A venous blood sample taken at autopsy cannot be considered to represent the antemortem blood concentration of a particular substance. Autolytic processes cause disintegration and increasing permeability of the physiological and anatomical barriers such as vascular walls and lead to changes in substance concentrations. In the present study, the experimental design represents an in vitro postmortem simulation of a drug substance crossing a venous wall. The postmortem behavior of morphine, morphine-3- and morphine-6-glucuronide was investigated. A Chien-Valia-diffusion chamber with a patch of inferior vena cava as diffusion barrier was used. For optimal simulation of postmortem events, vein sampling was restricted to selected autopsy cases. Parameters for the analysis of diffusion across the vascular tissue were dependence on time, temperature, and initial substance concentrations. The penetration behavior simulating venous efflux and influx of the substances was studied by different orientation of the venous wall in the experiments. Rhodamine B was used as a model substance to visualize the binding to the tissue and the passage across the venous wall. The permeation of morphine, morphine-3- and morphine-6-glucuronide across a vein tissue was found to be mainly dependent on the disintegration of the vascular wall and on the postmortem time period as well as on concentration gradients. From the data of this preliminary in vitro study, it can be concluded that a lag time for transvascular diffusion exists postmortem. However, it could be demonstrated, that adsorption to and penetration into the vascular tissue may alter intraluminal blood concentrations even at an early stage of the postmortem time period.

Published

1997

234. Plasma concentrations of heroin and morphine-related metabolites after intranasal and intramuscular administration.

Author

Skopp G, Ganssmann B, Cone EJ, and Aderjan R

Subjects

Administration, Intranasal, Adult, Chromatography, High Pressure Liquid, Heroin administration & dosage, Humans, Injections, Intramuscular, Male, Morphine administration & dosage, Morphine Derivatives blood, Narcotics administration & dosage, Heroin blood, Morphine blood, Narcotics blood

Abstract

The disposition of heroin and its metabolites was investigated in four healthy male volunteers following intranasal administration of 6 and 12 mg heroin hydrochloride. In addition, two doses of 6 mg heroin hydrochloride were injected intramuscularly for comparison of pharmacokinetic parameters. Serum samples were analyzed for heroin, 6-acetylmorphine, and morphine by solid-phase extraction-gas chromatography-mass spectrometry. The concentration of morphine glucuronides was determined by high-performance liquid chromatography based on the native fluorescence of the conjugates. Major findings were rapidly rising and declining terminal phases for heroin and 6-acetylmorphine and slowly declining phases of morphine and metabolites after both routes of administration. The area under the curve values of morphine-3-glucuronide depended on dose but not on route of administration. The apparent terminal half-lives of morphine-3-glucuronide ranged from 2.2 to 5.2 h for intranasally administered heroin and were 3.0 and 1.7 h for the intramuscularly applied drug. A mean morphine-3-glucuronide-heroin area-under-curve ratio of 93 for the intranasal route as compared with 38 for the intramuscular route demonstrated that circulating amounts of heroin were about half the size after intranasal administration of the same dose.

Published

1997

235. On cosmetically treated hair--aspects and pitfalls of interpretation.

Author

Skopp G, Pötsch L, and Moeller MR

Subjects

Drug Interactions, Gas Chromatography-Mass Spectrometry, Hair drug effects, Humans, Sebum metabolism, Substance Abuse Detection methods, Sweat metabolism, Hair metabolism, Hair Preparations pharmacology, Narcotics pharmacokinetics

Abstract

Popular hair cosmetic treatments like bleaching or permanent waving were found to affect the stability of incorporated drugs and to cause alterations of the fibers at an ultrastructural level. This may result in a partial or complete loss of drug substances, depending on the particular drug molecule and on its concentration prior to the cosmetic treatment. Moreover, from literature, there is some evidence that drug molecules are not only incorporated into the growing fiber by passive diffusion from blood into the matrix cells and melanocytes, but that the substances enter the hair also via perspiration such as sweat and sebum. Since permed and bleached hair shows an enhanced sorption capacity, the risk of false positives or an unusually high drug concentration in cosmetically treated hair was under investigation. Virgin, permed, mildly as well as severely bleached tresses were exposed to artificial sweat or sebum containing cocaine, benzoylecgonine, 6-acetylmorphine, morphine and codeine (500 ng/g). Except codeine, the concentrations measured by GC/MS were very small and quite close to the detection limit indicating a minor importance of drug uptake into hair fiber from the endogenous-exogenous shunt via sebum or sweat. From the results it is concluded that an increased risk of false positive results in hair analysis on bleached and permanent waved hair fibers does exist, but is not particularly severe.

Published

1997

236. Biochemical approach on the conservation of drug molecules during hair fiber formation.

Author

Pötsch L, Skopp G, and Moeller MR

Subjects

Absorption, Animals, Biomarkers, Cell Membrane Permeability, Drug Interactions, Hair growth & development, Humans, Melanins metabolism, Pigmentation drug effects, Structure-Activity Relationship, Biotransformation physiology, Hair metabolism, Pharmaceutical Preparations metabolism

Abstract

A biochemical concept for the endogenous incorporation of drug molecules into growing hair is presented. It is based on the principles of transport across biomembranes, on the principles of biotransformation and drug melanin affinity. The approach gives explanations for current observations in hair analysis, which up to date have not been understood sufficiently. Phenomena such as the ratio of parent drug to metabolite in hair, the dependence of incorporation on the physico-chemical properties of the drug, the independence of drug incorporation on active melanogenesis (incorporation into non-pigmented hair) as well as the dependence of drug content on hair pigmentation are elucidated.

Published

1997

237. A comparison of 3H-cocaine binding on melanin granules and human hair in vitro.

Author

Pötsch L, Skopp G, and Rippin G

Subjects

Animals, Hair Color, Humans, Microscopy, Electron, Scanning, Mollusca, Cocaine metabolism, Hair metabolism, Melanins metabolism

Abstract

The in vitro experiments on the interaction of 3H-cocaine and melanin from Sepia officinalis confirmed the existence of drug binding sites on melanin granules. The results suggested that the binding of 3H-cocaine to melanin could be analyzed by assuming that the binding to the surface of pigment granules is analogous to the adsorption of a drug on a solid and follows Langmuir adsorption isotherm type I. Scatchard analysis indicated heterogeneity of binding sites. Structural and chemical alterations caused by isolation of the melanoproteins, which are heterogeneous in nature and show different physico-chemical properties, are considered to be most crucial. The studies on hair samples confirmed that melanin-drug interaction occur on the surface of melanin granules. These seem to be of minor importance compared to the drug-melanoprotein loading during melanogenesis for the observed influence of pigmentation on the drug content of hair fibers. From the results it was concluded that in vitro studies on melanin provide limited information and even drug-soaked hair must be regarded as inappropriate for the study of melanin-drug-binding in hair.

Published

1997

238. Preliminary practical findings on drug monitoring by a transcutaneous collection device.

Author

Skopp G, Pötsch L, Eser HP, and Möller MR

Subjects

Humans, Methadone therapeutic use, Patient Acceptance of Health Care, Patient Compliance, Permeability, Substance-Related Disorders diagnosis, Sweat metabolism, Theophylline pharmacokinetics, Drug Monitoring methods, Forensic Medicine methods, Specimen Handling methods

Abstract

A noninvasive and nonocclusive skin patch (Sudormed) was investigated for the systematic collection of drugs of abuse over a period of several days. First, the applicability and user friendliness were tested by volunteers. The permeability of the polyurethane dressing from the outside to the inside for an aqueous solution was shown by incubating the outside layer with Rhodamine B. No fluorescence could be detected in the cotton pad beneath. A single dose experiment using theophylline as a model compound showed that there was a delay in time before the substance could be determined in the pad. The drug content decreased with increasing time of patch application. When eight volunteers participating in a methadone treatment were monitored, the substitute drug could always be detected in the patch associated with a minor concentration of EDDP. Besides, in some of the patches investigated, indications for an abuse of cocaine and heroin were found. The so-called sweat patch appears to be a valuable tool in clinical and forensic toxicology, as it offers a longer and prospective surveillance period compared with blood and urine testing.

Published

1996

239. Stability of opiates in hair fibers after exposure to cosmetic treatment.

Author

Pötsch L and Skopp G

Subjects

Bias, Codeine analogs & derivatives, Codeine analysis, Drug Stability, Forensic Medicine, Humans, Morphine analysis, Reproducibility of Results, Substance Abuse Detection methods, Substance-Related Disorders diagnosis, Hair chemistry, Hair Preparations analysis, Narcotics analysis, Substance Abuse Detection standards

Abstract

The stability of opiates in clipped natural human hair was investigated. Hair fibers were incubated with defined solutions of morphine, codeine and dihydrocodeine (pH 7.4) until saturated. Original opiate-positive hair samples collected from drug addicts also were examined. Commercially available bleaching as well as perming formulas (Poly Blonde Ultra, Poly Lock; Henkel, Düsseldorf, Germany) were applied in vitro to the hair strands of both groups under investigation. After these treatments, the drug concentration had decreased for both bleaching and permanent waving. In the spiked hair, only 2-18% of the starting solution could be found after bleaching. About 20-30% of the drug substances could still be detected after perming. In the authentic hair samples, the drug levels of the formerly opiate positive hair fibers had also been reduced but distinct tendencies could not be observed.

Published

1996

240. Fatal poisoning with the antidepressive agent opipramol.

Author

Skopp G, Miltner E, and Aderjan R

Subjects

Adult, Chromatography, High Pressure Liquid, Ethanol blood, Female, Humans, Opipramol pharmacokinetics, Suicide, Tissue Distribution, Opipramol poisoning

Abstract

An ingestion of an unknown quantity ( < or = 3000 mg) of opipramol dihydrochloride in a suicide case is described. Quantitation of opipramol and its deshydroxyethyl metabolite was performed simultaneously after liquid-liquid extraction from alkalinized samples prior to HPLC analysis. Postmortem concentrations of opipramol and of the metabolite in body fluids and organs are given. The distribution pattern of opipramol in tissue was comparable to findings from animal studies. The results showed the high uptake of opipramol in parenchymal tissues resulting in a low blood concentration. A possibly low contribution of deshydroxyethyl opipramol to the antidepressive effect may be concluded as the concentration was considerably lower in brain compared to other organs.

Published

1996

241. Postmortem distribution pattern of morphine and morphine glucuronides in heroin overdose.

Author

Skopp G, Lutz R, Ganssmann B, Mattern R, and Aderjan R

Subjects

Adult, Drug Overdose, Humans, Male, Morphine Derivatives pharmacokinetics, Time Factors, Autopsy methods, Glucuronates pharmacokinetics, Morphine pharmacokinetics, Morphine poisoning, Postmortem Changes

Abstract

The postmortem distribution of morphine and its metabolites was investigated in four cases of heroin overdose to evaluate some of the factors that influence intravasal blood concentrations. Variables included were the chemical stability of morphine conjugates, hemoconcentration, incomplete distribution of the drug and diffusion processes. Blood samples from different sampling sites including the aorta, the infra- and suprarenal portion of the inferior vena cava, the superior vena cava, the femoral and subclavian veins, and the right and left ventricles were examined for morphine, morphine-3-glucuronide and morphine-6-glucuronide, hematocrit and water content. Drug concentrations were determined by HPLC based on the native fluorescence of the analytes. Morphine glucuronides proved to be stable for a time period of 72 h. The water content ranged from 65 to 83% and hematocrit values from 25 to 75%, and were seen as contributory factors to the dramatic differences observed for drug concentrations from different sampling sites. The differences could neither be attributed to incomplete distribution during life-time nor to a diffusion process following the different distribution volumes of morphine and its conjugates. A definite relationship between the ratio of the molar concentrations of morphine and its glucuronides, as assessed in pharmacokinetical studies after morphine dosing, could not be established. For a better understanding more cases and changes over time and tissue concentrations should be analysed.

Published

1996

242. Experimental investigations on hair fibers as diffusion bridges and opiates as solutes in solution.

Author

Skopp G, Pötsch L, and Aderjan R

Subjects

Asian People, Diffusion, Hair growth & development, Hair metabolism, Humans, Narcotics pharmacokinetics, Time Factors, White People, Hair chemistry, Narcotics analysis

Abstract

Diffusion experiments were performed using clipped hair fibers as diffusion bridges and aqueous solutions of morphine, codeine and dihydrocodeine. Natural as well as predamaged hair fibers were investigated. The test series were conducted at ambient temperature and at high humidity. After 312 or 372 hours the middle segments of the strands were clipped, washed and analyzed by GC/MS. Only when virgin hair samples were used the solutes passed along the fiber at full length resulting in a positive immunological finding at the end of the diffusion bridge. Most of the washing fluids were positive for opiates. All centerpieces had a high opiate content. The opiate concentration in damaged hair was significantly higher. Radial swelling of the hair fiber with radial diffusion was the first and main process to appear when hair was exposed to water. The diffusion process in hair could not be placed in a simple mathematical treatment.

Published

1996

243. [Congener analysis in a drinking trial with unusually high alcohol content].

Author

Schmitt G, Skopp G, Aderjan R, and Mattern R

Subjects

Accidents, Traffic legislation & jurisprudence, Adult, Alcoholism diagnosis, Alcoholism rehabilitation, Humans, Male, Metabolic Clearance Rate physiology, Alcoholic Intoxication blood, Alcoholism blood, Alcohols pharmacokinetics, Ethanol pharmacokinetics

Abstract

The aforementioned case proves very convincingly that a very high dose of alcohol consumed within a short time span can be absorbed completely within 2 hours. Numerical models based on low to moderate alcohol consumption were lower than expected in cases of severe alcohol intake. The claim of alcohol consumption after an event can best be verified by means of a drinking experiment under intensive medical supervision.

Published

1995

244. [Hair analysis in the diagnosis of toxic hepatitis after Ecstasy abuse].

Author

Skopp G, Aderjan R, and Koster J

Subjects

Adolescent, Chemical and Drug Induced Liver Injury diagnosis, Clinical Enzyme Tests, Humans, Male, Chemical and Drug Induced Liver Injury etiology, Hair chemistry, N-Methyl-3,4-methylenedioxyamphetamine analysis, Substance-Related Disorders diagnosis

Abstract

History and Clinical Findings: A young man, aged 18 years, was admitted to hospital for suspected hepatitis, having developed increasing jaundice without any pain. His urine was light brown in colour and the stools often liquid and pale. Every 14 days for the last 4 months he had been taking 2 tablets of "ecstasy" (methylenedioxyamphetamine; MDMA). Physical examination was unremarkable and the patient was in good general condition., Tests: The activities of GOT, GPT and alkaline phosphatase were raised (to 903, 744 and 270 U/l, respectively) as was the bilirubin concentration (16.8 mg/dl). Tests were negative for: leptospira and the viruses of mumps, HI, varicella zoster, picornavirus, cytomegaly, Coxsackie and hepatitis, A, B and C. Ultrasound revealed hepatomegaly, with a normal echo pattern. Hair analysis demonstrated, in two different hair segments (0-2 cm and 2-4 cm, respectively) both MDMA (6.4 and 4.3 micrograms/g hair) and its metabolite MDA (0.7 and 5.0 micrograms/g hair)., Treatment and Course: No specific treatment was required. After intake of the drug had been stopped the transferase activities and bilirubin concentration became essentially normal., Conclusion: Hair analysis can be valuable in confirming "ecstasy" abuse, especially when it is denied, and thus contribute to clarifying the cause of toxic hepatitis.

Published

1995

245. Morphine and morphine glucuronides in serum of heroin consumers and in heroin-related deaths determined by HPLC with native fluorescence detection.

Author

Aderjan R, Hofmann S, Schmitt G, and Skopp G

Subjects

Chromatography, High Pressure Liquid, Gas Chromatography-Mass Spectrometry, Heroin Dependence mortality, Humans, Heroin Dependence metabolism, Morphine blood, Morphine Derivatives blood

Abstract

A simple, rapid, and sensitive high-performance liquid chromatographic method for the simultaneous determination of serum morphine, morphine-6-glucuronide (M6G), and morphine-3-glucuronide (M3G) based on native fluorescence detection is described. For the extraction of drugs and their metabolites, 200 microL serum was applied to 50 mg of a commercially available octylsilan phase. After isocratic separation in two steps (6.5 min) by reversed phase, the compounds were determined at an excitation wavelength of 245 nm and an emission wavelength of 345 nm (the limit of detection was approximately 5 micrograms/L for each compound). The concentrations of morphine, M6G (with respect to its potential analgesic activity), and M3G were investigated in 20 heroin addicts in police custody and in 10 heroin-associated deaths. The ratios between M6G or M3G and the morphine concentrations and between M6G and M3G are related to the morphine concentration and consequently depend on the time elapsed since the last administration of morphine or heroin. Consequently, the M6G values were found to be higher in cases of death than in the living addicts. By considering the M6G/morphine or M3G/morphine ratios, the narcotic effect of heroin as reflected by morphine and its metabolite concentrations in impaired addicts and cases of fatal poisoning can be better assessed than by use of the morphine concentration alone.

Published

1995

246. Ultrastructural alterations and environmental exposure influence the opiate concentrations in hair of drug addicts.

Author

Pötsch L, Skopp G, and Becker J

Subjects

Female, Fluorescence Polarization Immunoassay, Forensic Medicine, Hair Dyes, Humans, Male, Microscopy, Electron, Scanning, Soil, Water, Environmental Exposure, Hair chemistry, Hair ultrastructure, Narcotics analysis, Opioid-Related Disorders pathology, Substance Abuse Detection methods

Abstract

Hair samples were taken at autopsy from the head of 1 male and 1 female subject both known as drug abusers. Some of the strands were bleached by in-vitro cosmetic treatment. The bleached hair as well as the original hair samples were partly exposed to water or soil prior to further investigations and drug monitoring. The exposure times were 4 weeks or 6 months for water and 6 months for soil. The hair fibers were examined by transmission electron microscope (TEM) and by scanning electron microscope (SEM) investigations. The electron microscope studies confirmed that all experimental conditions had produced morphological alterations in the hair fibers. After exposure to water or to soil for 6 months as well as after storage of the clipped bleached hair in tap water at room temperature for 4 weeks, drug monitoring of formerly positive hair samples gave negative results. After storage of natural hair in soil or in water for 4 weeks the opiate levels had dramatically decreased. The samples were screened by fluorescence polarization immunoassay after enzymatic digestion. The results were confirmed by GC/MS.

Published

1995

247. Separation of cardanols by reversed phase HPLC.

Author

Skopp G and Schwenker G

Published

1984