Your search keyword '"Michel J.X. Hillebrand"' showing total 43 results

1. Bottom-up sample preparation for the LC-MS/MS quantification of anti-cancer monoclonal antibodies in bio matrices

Author

Hilde Rosing, Jos H. Beijnen, Michel J.X. Hillebrand, Alwin D. R. Huitema, Karen Am de Jong, and Suse J van Breugel

Subjects

medicine.drug_class, Clinical Biochemistry, Antineoplastic Agents, Mass spectrometry, Monoclonal antibody, 030226 pharmacology & pharmacy, 01 natural sciences, Analytical Chemistry, 03 medical and health sciences, 0302 clinical medicine, Tandem Mass Spectrometry, Lc ms ms, medicine, Humans, Sample preparation, General Pharmacology, Toxicology and Pharmaceutics, Chromatography, Chemistry, 010401 analytical chemistry, Cancer, Antibodies, Monoclonal, General Medicine, medicine.disease, 0104 chemical sciences, Medical Laboratory Technology, Chromatography, Liquid

Abstract

Therapeutic monoclonal antibodies (mAbs) are rapidly taking over the treatment of many malignancies, and an astonishing number of mAbs is in development. This causes a high demand for quantification of mAbs in biomatrices both for measuring therapeutic mAb concentrations and to support pharmacokinetics and pharmacodynamics studies. Conventionally, ligand-binding assays are used for these purposes, but LC–MS is gaining popularity. Although intact (top-down) and subunit (middle-down) mAb quantification is reported, signature peptide (bottom-up) quantification is currently most advantageous. This review provides an overview of the reported bottom-up mAb quantification methods in biomatrices as well as general recommendations regarding signature peptide and internal standard selection, reagent use and optimization of digestion in bottom-up quantification methods.

Published

2020

2. Quantitative determination of azacitidine triphosphate in peripheral blood mononuclear cells using liquid chromatography coupled with high-resolution mass spectrometry

Author

Eric Laille, Hilde Rosing, Michel J.X. Hillebrand, Jos H. Beijnen, Jan H.M. Schellens, Ellen J. B. Derissen, and Hans M. M. B. Otten

Subjects

Male, Antimetabolites, Antineoplastic, Cytidine triphosphate, viruses, Clinical Biochemistry, Azacitidine, Pharmaceutical Science, Mass spectrometry, Orbitrap, Mass Spectrometry, Analytical Chemistry, law.invention, chemistry.chemical_compound, law, Drug Discovery, medicine, Humans, heterocyclic compounds, Spectroscopy, Aged, Uridine triphosphate, Chromatography, Cytidine, Middle Aged, Triple quadrupole mass spectrometer, enzymes and coenzymes (carbohydrates), chemistry, Leukocytes, Mononuclear, Feasibility Studies, Female, Monoisotopic mass, Chromatography, Liquid, medicine.drug

Abstract

Azacitidine is a cytidine analog used in the treatment of myelodysplastic syndromes, chronic myelomonocytic leukemia and acute myeloid leukemia. The pharmacological effect of azacitidine arises after incorporation into the DNA and RNA. To this end, the drug first has to be converted into its triphosphate forms. This paper describes the development of an assay for quantitative determination of azacitidine triphosphate (aza-CTP) in peripheral blood mononuclear cells (PBMCs). To quantify aza-CTP, separation from the endogenous nucleotides cytidine triphosphate (CTP) and uridine triphosphate (UTP) is required. This was a challenge as the structures of these nucleotides are highly similar and the monoisotopic molecular masses of aza-CTP, UTP and the naturally occurring [(13)C]- and [(15)N]-isotopes of CTP differ less than 0.02 Da. Efforts to select a specific MS(2)-fragment for aza-CTP using a triple quadrupole mass spectrometer remained without success. Therefore, we investigated the feasibility to separate these highly resembling nucleotides based on accurate mass spectrometry using a linear trap quadrupole (LTQ) coupled with an Orbitrap. The LTQ-Orbitrap was able to differentiate between aza-CTP and the endogenous nucleotides UTP and [(13)C]-CTP. There was no baseline resolution between aza-CTP and [(15)N]-CTP, but the [(15)N]-CTP interference was low. For quantification, extracted ion chromatograms were obtained for the accurate m/z window of the aza-CTP product ion. The assay was able to determine aza-CTP concentrations in PBMC lysate from 40.7 to 281 nM. Assuming that an average cell suspension extracted from 16 mL blood contains 10 to 42 million PBMCs per mL, this range corresponds with 2.58/10.9-17.8/74.9 pmol aza-CTP per million PBMCs. Intra-assay accuracies were between -1.1 and 9.5% deviation and coefficient of variation values were ≤13.2%. The assay was successfully applied to quantify aza-CTP in samples from two patients treated with azacitidine. Aza-CTP concentrations up to 19.0 pmol per million PBMCs were measured. This is the first time that aza-CTP concentrations were quantified in PBMCs from patients treated with azacitidine.

Published

2014

3. A sensitive combined assay for the quantification of paclitaxel, docetaxel and ritonavir in human plasma using liquid chromatography coupled with tandem mass spectrometry

Author

Jeroen J M A Hendrikx, Bas Thijssen, Michel J.X. Hillebrand, Jan H.M. Schellens, Hilde Rosing, Alfred H. Schinkel, and Jos H. Beijnen

Subjects

Spectrometry, Mass, Electrospray Ionization, Analyte, Electrospray, Paclitaxel, Calibration curve, Clinical Biochemistry, Docetaxel, Tandem mass spectrometry, Sensitivity and Specificity, Biochemistry, High-performance liquid chromatography, Analytical Chemistry, Tandem Mass Spectrometry, Liquid chromatography–mass spectrometry, Neoplasms, Antineoplastic Combined Chemotherapy Protocols, medicine, Humans, Chromatography, High Pressure Liquid, Ritonavir, Chromatography, Chemistry, Cell Biology, General Medicine, Taxoids, medicine.drug

Abstract

A combined assay for the determination of paclitaxel, docetaxel and ritonavir in human plasma is described. The drugs were extracted from 200 μL human plasma using liquid-liquid extraction with tertiar-butylmethylether, followed by high performance liquid chromatography analysis using 10 mM ammonium hydroxide pH 10:methanol (3:7, v/v) as mobile phase. Chromatographic separation was obtained using a Zorbax Extend C(18) column. Labelled analogues of the analytes are used as internal standards. For detection, positive ionization electrospray tandem mass spectrometry was used. Method development including optimisation of the mass transitions and response, mobile phase optimisation and column selection are discussed. The method was validated according to FDA guidelines and the principles of Good Laboratory Practice (GLP). The validated range was 0.5-500 ng/mL for paclitaxel and docetaxel and 2-2000 ng/mL for ritonavir. For quantification, quadratic calibration curves were used (r(2)>0.99). The total runtime of the method is 9 min and the assay combines analytes with differences in ionisation and desired concentration range. Inter-assay accuracy and precision were tested at four concentration levels and were within 10% and less than 10%, respectively, for all analytes. Carry-over was less than 6% and endogenous interferences or interferences between analytes and internal standards were less than 20% of the response at the lower limit of quantification level. The matrix factor and recovery were determined at low, mid and high concentration levels. The matrix factor was around 1 for all analytes and total recovery between 77.5 and 104%. Stability was investigated in stock solutions, human plasma, dry extracts, final extracts and during 3 freeze/thaw cycles. The described method was successfully applied in clinical studies with oral administration of docetaxel or paclitaxel in combination with ritonavir.

Published

2011

4. Brain accumulation of sunitinib is restricted by P-glycoprotein (ABCB1) and breast cancer resistance protein (ABCG2) and can be enhanced by oral elacridar and sunitinib coadministration

Author

Birk Poller, Nienke A.G. Lankheet, Jurjen S. Lagas, Seng Chuan Tang, Alfred H. Schinkel, Jos H. Beijnen, Michel J.X. Hillebrand, and Hilde Rosing

Subjects

Male, Cancer Research, ATP Binding Cassette Transporter, Subfamily B, Indoles, Abcg2, medicine.drug_class, Administration, Oral, Antineoplastic Agents, Pharmacology, urologic and male genital diseases, Blood–brain barrier, Tyrosine-kinase inhibitor, Mice, Dogs, Pharmacokinetics, In vivo, Tetrahydroisoquinolines, Sunitinib, medicine, ATP Binding Cassette Transporter, Subfamily G, Member 2, Animals, Humans, Pyrroles, Tissue Distribution, ATP Binding Cassette Transporter, Subfamily B, Member 1, P-glycoprotein, Mice, Knockout, biology, business.industry, Brain, Biological Transport, Transporter, Drug Resistance, Multiple, female genital diseases and pregnancy complications, medicine.anatomical_structure, Oncology, Blood-Brain Barrier, biology.protein, Acridines, ATP-Binding Cassette Transporters, sense organs, business, medicine.drug

Abstract

Sunitinib is an orally active, multitargeted tyrosine kinase inhibitor which has been used for the treatment of metastatic renal cell carcinoma and imatinib-resistant gastrointestinal stromal tumors. We aimed to investigate the in vivo roles of the ATP-binding cassette drug efflux transporters ABCB1 and ABCG2 in plasma pharmacokinetics and brain accumulation of oral sunitinib, and the feasibility of improving sunitinib kinetics using oral coadministration of the dual ABCB1/ABCG2 inhibitor elacridar. We used in vitro transport assays and Abcb1a/1b(-/-) , Abcg2(-/-) and Abcb1a/1b/Abcg2(-/-) mice to study the roles of ABCB1 and ABCG2 in sunitinib disposition. In vitro, sunitinib was a good substrate of murine (mu)ABCG2 and a moderate substrate of human (hu)ABCB1 and huABCG2. In vivo, the systemic exposure of sunitinib after oral dosing (10 mg kg(-1) ) was unchanged when muABCB1 and/or muABCG2 were absent. Brain accumulation of sunitinib was markedly (23-fold) increased in Abcb1a/b/Abcg2(-/-) mice, but only slightly (2.3-fold) in Abcb1a/b(-/-) mice, and not in Abcg2(-/-) mice. Importantly, a clinically realistic coadministration of oral elacridar and oral sunitinib to wild-type mice resulted in markedly increased sunitinib brain accumulation, equaling levels in Abcb1a/1b/Abcg2(-/-) mice. This indicates complete inhibition of the blood-brain barrier (BBB) transporters. High-dose intravenous sunitinib could saturate BBB muABCG2, but not muABCB1A, illustrating a dose-dependent relative impact of the BBB transporters. Brain accumulation of sunitinib is effectively restricted by both muABCB1 and muABCG2 activity. Complete inhibition of both transporters, leading to markedly increased brain accumulation of sunitinib, is feasible and safe with a clinically realistic oral elacridar/sunitinib coadministration.

Published

2011

5. A validated assay for the quantitative analysis of vatalanib in human EDTA plasma by liquid chromatography coupled with electrospray ionization tandem mass spectrometry

Author

Marlies H.G. Langenberg, Michel J.X. Hillebrand, A.G. Lankheet, Emile E. Voest, A. D. R. Huitema, Jos H. Beijnen, Jan H.M. Schellens, and Hilde Rosing

Subjects

Spectrometry, Mass, Electrospray Ionization, Electrospray, Chromatography, Molecular Structure, Pyridines, Chemistry, Elution, Electrospray ionization, Clinical Biochemistry, Selected reaction monitoring, Reproducibility of Results, Cell Biology, General Medicine, Tandem mass spectrometry, Mass spectrometry, Biochemistry, Analytical Chemistry, Triple quadrupole mass spectrometer, Humans, Phthalazines, Quantitative analysis (chemistry), Chromatography, Liquid

Abstract

A sensitive and accurate method for the determination of vatalanib in human EDTA plasma was developed using high-performance liquid chromatography and detection with tandem mass spectrometry. Stable isotopically labeled imatinib was used as internal standard. Plasma proteins were precipitated and an aliquot of the supernatant was directly injected onto a Phenomenex Gemini C18 analytical column (50 mm x 2.0 mm ID, 5.0 microm particle size) and then compounds were eluted with a linear gradient. The outlet of the column was connected to a Sciex API 365 triple quadrupole mass spectrometer and ions were detected in positive multiple reaction monitoring mode. The lower limit of quantification was 10 ng/mL (S/N approximately 10, CV < or = 8.4%). This method was validated over a linear range from 10 to 2500 ng/mL, and results from the validation study demonstrated a good intra- and inter-assay accuracy (inaccuracy < or = 9.57%) and precision (CV < or = 8.81%). This method has been used to determine plasma vatalanib concentrations in patients with advanced solid tumor, enrolled in a phase I pharmacokinetic trial with the drug.

Published

2009

6. Development and validation of a quantitative assay for the measurement of miltefosine in human plasma by liquid chromatography-tandem mass spectrometry

Author

Michel J.X. Hillebrand, Jos H. Beijnen, Thomas P. C. Dorlo, Hilde Rosing, Peter J. de Vries, Teunis A. Eggelte, Infectious diseases, and KIT: Biomedical Research

Subjects

Miltefosine, Chromatography, Chemistry, Phosphorylcholine, Electrospray ionization, Clinical Biochemistry, Antiprotozoal Agents, Cell Biology, General Medicine, Mass spectrometry, Tandem mass spectrometry, Sensitivity and Specificity, Biochemistry, Analytical Chemistry, Column chromatography, Pharmacokinetics, Tandem Mass Spectrometry, Liquid chromatography–mass spectrometry, medicine, Humans, Quantitative analysis (chemistry), Chromatography, Liquid, medicine.drug

Abstract

A sensitive and specific liquid chromatography-tandem mass spectrometry (LC-MS/MS) assay for the quantification of miltefosine is presented. A 250 mu L human EDTA plasma aliquot was spiked with miltefosine and extracted by a solid-phase extraction method. Separation was performed on a Gemini C 18 column (150 mm x 2.0 mm I.D., 5 mu m) using an alkaline eluent. Detection was performed by positive ion electrospray ionization followed by triple-quadrupole mass spectrometry. The assay has been validated for miltefosine from 4 to 2000 ng/mL using 250 mu L human EDTA plasma samples. Results from the validation demonstrate that miltefosine can be accurately and precisely quantified in human plasma. At the lowest level, the intra-assay precision was lower than 10.7%, the inter-assay precision was 10.6% and accuracies were between 95.1 and 109%. This assay is successfully used in a clinical pharmacokinetic study with miltefosine. (c) 2008 Elsevier B.V. All rights reserved

Published

2008

7. Phase I and pharmacokinetic study of combined treatment with perifosine and radiation in patients with advanced solid tumours

Author

R. Dubbelman, Stefan R. Vink, Jan H.M. Schellens, Gemi Moppi, Harry Bartelink, Herbert Sindermann, Marcel Verheij, Michel J.X. Hillebrand, Jürgen Engel, and Jos H. Beijnen

Subjects

Adult, Male, Radiation-Sensitizing Agents, medicine.medical_specialty, Nausea, Phosphorylcholine, medicine.medical_treatment, Antineoplastic Agents, Gastroenterology, chemistry.chemical_compound, Neoplasms, Internal medicine, medicine, Humans, Radiology, Nuclear Medicine and imaging, Aged, Pneumonitis, Aged, 80 and over, Chemotherapy, Bladder cancer, Dose-Response Relationship, Drug, business.industry, Hematology, Middle Aged, medicine.disease, Perifosine, Surgery, Radiation therapy, Oncology, Tolerability, chemistry, Vomiting, Female, medicine.symptom, business

Abstract

Purpose Perifosine is an orally applicable, membrane-targeted alkylphosphocholine analogue with antitumour activity and radiosensitising properties in preclinical models. The purpose of this phase I study was to determine the feasibility and tolerability of concurrent daily perifosine and radiation in patients with advanced cancer. Patients and methods Starting dose of perifosine was 50mg/day; dose escalation was in steps of 50mg. Daily administration commenced 2 days before radiotherapy and was continued throughout the radiation treatment. At least three patients were entered at each dose level; at the 150mg/day level 10 patients were included. Pharmacokinetic sampling was performed weekly pre-dosing. Twenty-one patients were entered. Tumour types included NSCLC ( n =17), prostate, oesophageal, colon and bladder cancer. Most patients (16/21) had received prior chemotherapy; none radiotherapy. Median number of daily perifosine administrations was 31 (range 24–53). Mean radiation dose (BED 10 ) was 59.8Gy (range 50.7–87.5Gy in 13–28 fractions). Results Major drug-related toxicities according to CTC criteria were nausea in 57%, fatigue in 48%, vomiting in 38%, diarrhoea in 38% and anorexia in 19%. No bone marrow toxicity was observed. DLT (nausea/vomiting) was encountered in two of five patients at the 200mg/day dose level. Dose-dependent steady-state plasma levels were reached after 1 week. Major radiotherapy-related acute toxicity consisted of dysphagia in 38% and pneumonitis in 29%. Conclusion Perifosine can be safely combined with fractionated radiotherapy. A dosage of 150mg/day, to be started at least 1 week prior to radiotherapy, is recommended for phase II evaluation.

Published

2006

8. Pharmacokinetics and pharmacodynamics of high doses of pharmaceutically prepared heroin, by intravenous or by inhalation route in opioid-dependent patients

Author

Jan M. van Ree, Elisabeth J. Rook, Alwin D. R. Huitema, Michel J.X. Hillebrand, Vincent M. Hendriks, Wim van den Brink, Jos H. Beijnen, ANS - Amsterdam Neuroscience, and Adult Psychiatry

Subjects

Adult, Male, Side effect, Blood Pressure, Chasing the dragon, Pharmacology, Toxicology, Heroin, Pharmacokinetics, Double-Blind Method, Heart Rate, Administration, Inhalation, mental disorders, medicine, Reaction Time, Humans, Inhalation, Maintenance dose, business.industry, General Medicine, Middle Aged, Opioid-Related Disorders, Bioavailability, Analgesics, Opioid, Anesthesia, Injections, Intravenous, Morphine, business, Methadone, medicine.drug

Abstract

A pharmacokinetic-pharmacodynamic study was performed in opioid-dependent patients in the Netherlands, who were currently treated with high doses of pharmaceutically prepared heroin on medical prescription. Besides intravenous heroin, heroin was prescribed for inhalation by "chasing the dragon" method. In this technique, heroin base is heated on aluminium foil, and heroin vapours are inhaled into the lungs. Not much is known about the pharmacokinetics profile and bioavailability of this specific administration method. Therefore, a study was performed on pharmacokinetics and pharmacodynamics of heroin inhalation and intravenous use. Eleven patients who injected heroin and 9 patients who inhaled heroin entered the study. They were on steady-state heroin treatment for at least 12 months. For safety reasons, there was no crossing-over between heroin injection or inhalation. In a double-blind randomised study, 67-100-150% of the regular heroin maintenance dose was administered to each patient. Maximal single heroin dose was 450 mg. Plasma concentrations of heroin and its metabolites 6-monoacetylmorphine, morphine and morphine-glucuronides were analysed using LC-MS-MS. Blood pressure, heart rate, skin temperature and reaction time were assessed. Furthermore, visual analogue scales regarding craving and appreciation of heroin effect were scored by the subjects. Both in inhaling and injecting patients, the areas under curve of heroin and all measured metabolites were linearly related to heroin dose. Mean C(max) of heroin and its metabolites were 2-6 times lower after inhalation, than after intravenous injection. Bioavailability (F) of heroin inhalation was estimated as 52% (95% CI 44-61%). Heroin was rapidly cleared from plasma. Cl/F was 930 l/hr (95% CI 799-1061 l/hr) after intravenous administration, and 1939 l/hr (95% CI 1661-2217 l/hr) after inhalation. Heroin Cl and Vd were correlated to body weight (R(2) 15-19%). Morphine-glucuronides levels were inversely related to creatinine clearance. After heroin administration, the reaction time was significantly prolonged with 28+/-5.3 msec. in injecting and 13+/-4.9 msec. in inhaling patients. Cardiovascular changes were only mild after heroin administration. Craving-scores declined immediately after heroin administration in both administration groups. Subjective heroin effect was rated more positively in heroin inhaling than in injecting patients, despite the lower C(max) levels following heroin inhalation. In both groups, in this blinded study heroin dose increments were more appreciated than dose reductions. Increments of 50% of the regular heroin dose did not cause any serious side effect.

Published

2006

9. The quantitative analysis of heroin, methadone and their metabolites and the simultaneous detection of cocaine, acetylcodeine and their metabolites in human plasma by high-performance liquid chromatography coupled with tandem mass spectrometry

Author

Jan M. van Ree, Jos H. Beijnen, Hilde Rosing, Elisabeth J. Rook, and Michel J.X. Hillebrand

Subjects

Narcotics, Spectrometry, Mass, Electrospray Ionization, Time Factors, Metabolite, Clinical Biochemistry, Biochemistry, High-performance liquid chromatography, Analytical Chemistry, chemistry.chemical_compound, Cocaine, Administration, Inhalation, medicine, Humans, Solid phase extraction, Chromatography, High Pressure Liquid, Chromatography, Codeine, Heroin Dependence, Chemistry, Selected reaction monitoring, Reproducibility of Results, Cell Biology, General Medicine, Norcocaine, Triple quadrupole mass spectrometer, Heroin, Benzoylecgonine, Methadone, medicine.drug

Abstract

For a pharmacokinetic-pharmacodynamic study in opioid tolerant patients, who were treated with heroin in combination with methadone, a liquid chromatographic assay with tandem mass spectrometry detection (LC-MS/MS) was developed for the simultaneous determination of heroin, methadone, heroin metabolites 6-monoacetylmorphine, morphine, and morphine-6 and 3-glucuronide and methadone metabolite EMDP. To detect any abuse of substances besides the prescribed opioids the assay was extended with the detection of cocaine, its metabolites benzoylecgonine and norcocaine and illicit heroin adulterants acetylcodeine and codeine. Heroin-d6, morphine-d3, morphine-3-glucuronide-d3 and methadone-d9 were used as internal standards. The sample pre-treatment consisted of solid phase extraction using mixed mode sorbent columns (MCX Oasis). Chromatographic separation was performed at 25 degrees C on a reversed phase Zorbax column with a gradient mobile phase consisting of ammonium formate (pH 4.0) and acetonitrile. The run time was 15 min. MS with relatively mild electrospray ionisation under atmospheric pressure was applied. The triple quadrupole MS was operating in the positive ion mode and multiple reaction monitoring (MRM) was used for drug quantification. The method was validated over a concentration range of 5-500 ng/mL for all analytes. The total recovery of heroin varied between 86 and 96% and of the heroin metabolites between 76 and 101%. Intra-assay and inter-assay accuracy and precision of all analytes were always within the designated limits (< or =20% at lower limit of quantification (LLQ) and < or =15% for other samples). This specific and sensitive assay was successfully applied in pharmacokinetic studies with medically prescribed heroin and toxicological cases.

Published

2005

10. Human metabolism of [14C]indisulam following i.v. infusion in cancer patients

Author

Dick Pluim, S. Murray Yule, Jos H. Beijnen, Jan H.M. Schellens, Michel J.X. Hillebrand, Jan-Hendrik Beumer, Karen Foley, and Hilde Rosing

Subjects

Spectrometry, Mass, Electrospray Ionization, Glucuronidation, Antineoplastic Agents, Urine, Chemical Fractionation, Pharmacology, Tandem mass spectrometry, Hydroxylation, chemistry.chemical_compound, Glucuronides, Sulfation, Pharmacokinetics, Neoplasms, medicine, Humans, Pharmacology (medical), Carbon Radioisotopes, Infusions, Intravenous, Biotransformation, Chromatography, High Pressure Liquid, Sulfonamides, Chromatography, Chemistry, Metabolism, Oncology, Mechanism of action, Cholinesterase Inhibitors, medicine.symptom

Abstract

Indisulam is a new anticancer drug with a unique mechanism of action, arresting the cell cycle at the G1/S transition. The major excretory pathway of indisulam is via the urine, accounting for 63% of the radioactive dose ([(14)C]indisulam) administered in a human mass balance study. Radiochromatographic profiling of urine samples resulted in the detection of several radioactive peaks. The purpose of the present investigation was to elucidate the chemical structures of these observed indisulam metabolites. We collected fractions after chromatographic separation of the urine samples. These fractions were analysed using tandem mass spectrometry. We propose the chemical structure of 15 indisulam metabolites in urine. The metabolism of indisulam is very complex, consisting of oxidative dechlorination, hydroxylation, hydrolysis, acetylation, sulphation and glucuronidation. The clinical relevance of the observed indisulam metabolites needs further investigation.

Published

2005

11. Deuterodiacetylmorphine as a marker for use of illicit heroin by addicts in a heroin-assisted treatment program

Author

Elisabeth J. Rook, Michel J.X. Hillebrand, Marjolein G. Klous, Jos H. Beijnen, Wim van den Brink, Jan M. van Ree, Amsterdam Neuroscience, and Adult Psychiatry

Subjects

Male, Health, Toxicology and Mutagenesis, media_common.quotation_subject, Urine, Chasing the dragon, Toxicology, Sensitivity and Specificity, Mass Spectrometry, Analytical Chemistry, Heroin, Administration, Inhalation, mental disorders, medicine, Humans, Environmental Chemistry, media_common, Illicit heroin, Chemical Health and Safety, Chromatography, Heroin Dependence, Chemistry, Addiction, Diacetylmorphine, Reference Standards, Substance Abuse Detection, Heroin-assisted treatment, Biomarkers, Chromatography, Liquid, medicine.drug, Methadone

Abstract

In preparation for a treatment program concerning the medical coprescription of heroin and methadone to treatment-resistant addicts in the Netherlands, we studied a novel strategy for monitoring co-use of illicit (nonprescribed) heroin. A deuterated analogue of heroin was added (1:20) to pharmaceutical, smokable heroin (a powder mixture of 75% w/w diacetylmorphine base and 25% w/w caffeine anhydrate), to be used by inhalation after volatilization ("chasing the dragon"). Plasma and urine samples were collected from nine male patients who had used pharmaceutical, smokable heroin during a four-day stay in a closed clinical research unit, and these samples were analyzed by liquid chromatography coupled with tandem mass spectrometry. Ratios of deuterated and undeuterated diacetylmorphine and 6-acetylmorphine (MAM/MAM-d3) in plasma and urine were calculated from peak areas of these substances in the respective chromatograms. The MAM/MAM-d3 ratios in plasma and urine were normally distributed (with small standard deviations) and independent from concentrations of 6-acetylmorphine and from time after use of pharmaceutical heroin. A MAM/MAM-d3 ratio in urine above 32.8 was considered indicative of co-use of illicit heroin, and this value was associated with a false-positive rate of only 1% (95% confidence interval: -1 to 3%). The MAM/MAM-d3 ratio was detectable in urine for 4-9.5 h after use of pharmaceutical, smokable heroin. Addition of stable, isotopically labelled heroin to pharmaceutical, smokable heroin is considered to be a feasible strategy for the detection of co-use of illicit heroin by patients in heroin-assisted treatment.

Published

2005

12. Simultaneous quantification of fludarabine and cyclophosphamide in human plasma by high-performance liquid chromatography coupled with electrospray ionization tandem mass spectrometry

Author

L. H. H. Silvertand, P. Weigl, Hilde Rosing, F. Vazvaei, Michel J.X. Hillebrand, Jos H. Beijnen, and M. J. van Maanen

Subjects

Spectrometry, Mass, Electrospray Ionization, Chromatography, Molecular Structure, Chemistry, Electrospray ionization, Organic Chemistry, Selected reaction monitoring, Reproducibility of Results, Antineoplastic Agents, Tandem mass spectrometry, Sensitivity and Specificity, High-performance liquid chromatography, Sample preparation in mass spectrometry, Analytical Chemistry, Triple quadrupole mass spectrometer, Fludarabine, medicine, Cladribine, Humans, Cyclophosphamide, Chromatography, High Pressure Liquid, Vidarabine, Spectroscopy, Stock solution, medicine.drug

Abstract

Fludarabine and cyclophosphamide are anticancer agents mainly used in the treatment of hematologic malignancies. We have developed and validated an assay using high-performance liquid chromatography (HPLC) coupled with electrospray ionization tandem mass spectrometry for the quantification of fludarabine in combination with cyclophosphamide in human heparin and human EDTA plasma. Sample pre-treatment consisted of a protein precipitation with cold acetonitrile (−20°C) using 250 µL of plasma. Separation was performed on an Extend C18 column (150 × 2.1 mm i.d.; 5 µm) with a stepwise gradient using 1 mM ammonia solution and acetonitrile at a flow rate of 400 µL/min. The analytical run time was 12 min. The triple quadrupole mass spectrometer was operated in the positive ion mode and multiple reaction monitoring was used for drug quantification. The method was validated over a concentration range of 1 to 100 ng/mL for fludarabine and cyclophosphamide in human heparin and human EDTA plasma. The coefficients of variation were

Published

2005

13. Quantitative determination of the novel anticancer drug E7070 (indisulam) and its metabolite (1,4-benzenedisulphonamide) in human plasma, urine and faeces by high-performance liquid chromatography coupled with electrospray ionization tandem mass spectrometry

Author

Hilde Rosing, Albert J. R. Heck, Michel J.X. Hillebrand, Karen Foley, Jan H.M. Schellens, Jan H. Beumer, Lianda G. A. H. Nan-Offeringa, Jos H. Beijnen, and S. Murray Yule

Subjects

Spectrometry, Mass, Electrospray Ionization, Sulfonamides, Analyte, Chromatography, medicine.diagnostic_test, Metabolite, Electrospray ionization, Organic Chemistry, Ethyl acetate, Reproducibility of Results, Antineoplastic Agents, Urine, Tandem mass spectrometry, Sensitivity and Specificity, High-performance liquid chromatography, Analytical Chemistry, Feces, chemistry.chemical_compound, chemistry, Therapeutic drug monitoring, Injections, Intravenous, medicine, Humans, Chromatography, High Pressure Liquid, Spectroscopy

Abstract

E7070 (indisulam) is a novel anticancer drug currently undergoing clinical investigation. We present a sensitive and specific method for the quantitative determination of E7070 and its metabolite M1 (1,4-benzenedisulphonamide) in human plasma, urine and faeces. The analytes and their tetra-deuterated analogues, which were used as internal standards, were isolated from the biological matrix by solid-phase extraction with OASIS cartridges (0.5 mL plasma or 1 mL urine) and by liquid-liquid extraction with ethyl acetate at pH 5 (1 mL faecal homogenate). The analytes were separated on a C8 reversed-phase chromatographic column and analyzed using electrospray ionization and tandem mass spectrometric detection in the negative ion mode. The validated concentration ranges in plasma were 0.1–20 μg/mL for E7070 and 0.01–2 μg/mL for M1. In urine and faecal homogenate, a concentration range from 0.05–10 μg/mL or μg/g, respectively, was validated for both analytes. Validation of the plasma assay was performed according to the most recent FDA guidelines. The assay fulfilled all generally accepted requirements for linearity (r > 0.99, residuals between −8 and 10%), accuracy (−13.5 to 1.4%) and precision (all less than 11%) in the tested matrices. We investigated recovery, stability (working solutions at −20°C and at room temperature, biological matrices at −20°C, room temperature and after 3 freeze/thaw cycles; final extracts at room temperature) and robustness. All these parameters were found acceptable. This method is suited for mass balance studies or therapeutic drug monitoring, as demonstrated by a case example showing plasma concentrations and cumulative excretion of E7070 and M1 in urine and faeces. Furthermore, we show the presence of E7070 metabolites in patient urine. Copyright © 2004 John Wiley & Sons, Ltd.

Published

2004

14. Method development and validation for the quantification of dasatinib, erlotinib, gefitinib, imatinib, lapatinib, nilotinib, sorafenib and sunitinib in human plasma by liquid chromatography coupled with tandem mass spectrometry

Author

A. D. R. Huitema, Nienke A.G. Lankheet, Hilde Rosing, Jan H.M. Schellens, Michel J.X. Hillebrand, and Jos H. Beijnen

Subjects

Clinical Biochemistry, Pharmacology, Lapatinib, Biochemistry, Sensitivity and Specificity, Analytical Chemistry, Gefitinib, Tandem Mass Spectrometry, Drug Discovery, medicine, Humans, Molecular Biology, Protein Kinase Inhibitors, Chromatography, Chemistry, Sunitinib, Selected reaction monitoring, Poverty-related infectious diseases [N4i 3], General Medicine, respiratory tract diseases, Dasatinib, Nilotinib, Erlotinib, Drug Monitoring, Tyrosine kinase, medicine.drug, Chromatography, Liquid

Abstract

Item does not contain fulltext To support pharmacokinetic-guided dosing in individual patients, a fast and accurate method for simultaneous determination of anticancer tyrosine kinase inhibitors (TKIs) dasatinib, erlotinib, gefitinib, imatinib, lapatinib, nilotinib, sorafenib and sunitinib in human plasma was developed using high-performance liquid chromatography and detection with tandem mass spectrometry (HPLC-MS/MS). Stable isotopically labeled compounds of the eight different TKIs were used as internal standards. Plasma proteins were precipitated and an aliquot of supernatant was directly injected onto a reversed phase chromatography system consisting of a Gemini C18 column (50 x 2.0 mm i.d., 5.0 microm particle size) and then compounds were eluted with a gradient. The outlet of the column was connected to a triple quadrupole mass spectrometer with electrospray interface. Ions were detected in the positive multiple reaction monitoring mode. This method was validated over a linear range from 20.0 to 10,000 ng/mL for erlotinib, gefitinib, imatinib, lapatinib, nilotinib and sorafenib, and from 5.00 to 2500 ng/mL for dasatinib and sunitinib. Results from the validation study demonstrated good intra- and inter-assay accuracy (

Published

2013

15. Quantification of cabazitaxel, its metabolite docetaxel and the determination of the demethylated metabolites RPR112698 and RPR123142 as docetaxel equivalents in human plasma by liquid chromatography-tandem mass spectrometry

Author

Hilde Rosing, Michel J.X. Hillebrand, Anita Kort, Emile E. Voest, Jos H. Beijnen, G.A. Cirkel, A.H. Schinkel, and J. H. M. Schellens

Subjects

Metabolite, Clinical Biochemistry, Docetaxel, Biochemistry, Sensitivity and Specificity, Analytical Chemistry, chemistry.chemical_compound, Drug Stability, Liquid chromatography–mass spectrometry, Tandem Mass Spectrometry, medicine, Humans, Least-Squares Analysis, Taxane, Chromatography, Extraction (chemistry), Selected reaction monitoring, Reproducibility of Results, Cell Biology, General Medicine, Ammonium hydroxide, chemistry, Cabazitaxel, Taxoids, medicine.drug, Chromatography, Liquid

Abstract

We present a sensitive validated LC–MS/MS assay for the simultaneous determination of cabazitaxel and docetaxel in human plasma, with calibration ranges of 1.0–150 ng/mL for cabazitaxel and 0.1–15 ng/mL for docetaxel. Sample pretreatment consisted of liquid–liquid extraction with tert -butyl methyl ether. Chromatographic separation was achieved on a Zorbax Extend C 18 column using a gradient mixture of 10 mM ammonium hydroxide and methanol. Mass detection was carried out by turbo ion spray ionization in positive ion multiple reaction monitoring mode. All inter-day accuracies and precisions were within ±15% of the nominal value and within ±20% at the lower limit of quantitation. Demethylations of cabazitaxel yielding the metabolites RPR112698 and RPR123142 were monitored semi-quantitatively and quantified as ng docetaxel equivalents. Plasma samples of a prostate cancer patient treated with cabazitaxel were analyzed to demonstrate the usefulness of the presented assay for clinical drug monitoring. In conclusion, this method can be applied to support clinical pharmacokinetic studies with the novel anticancer drug cabazitaxel.

Published

2012

16. Quantitative determination of capecitabine and its six metabolites in human plasma using liquid chromatography coupled to electrospray tandem mass spectrometry

Author

Jos H. Beijnen, Maarten J. Deenen, Hilde Rosing, Michel J.X. Hillebrand, and Jan H.M. Schellens

Subjects

Analyte, Bioanalysis, Electrospray, Clinical Biochemistry, Tandem mass spectrometry, Biochemistry, Deoxycytidine, Sensitivity and Specificity, Mass Spectrometry, Analytical Chemistry, Capecitabine, Drug Stability, Tandem Mass Spectrometry, medicine, Protein precipitation, Humans, Prodrugs, Chromatography, High Pressure Liquid, Chromatography, Chemistry, Hydrophilic interaction chromatography, Reproducibility of Results, Cell Biology, General Medicine, Reversed-phase chromatography, Linear Models, Fluorouracil, medicine.drug

Abstract

Capecitabine is the oral prodrug of the anticancer drug 5-fluorouracil (5-FU). The purpose of this study was to quantify capecitabine and its metabolites including 5'-deoxy-5-fluorocytidine (5'-dFCR), 5'-deoxy-5-fluorouridine (5'-dFUR), 5-FU, dihydro-5-fluorouracil (FUH(2)), α-fluoro-ureidopropionic acid (FUPA) and fluoro-β-alanine (FBAL) in human plasma using liquid chromatography coupled to electrospray tandem mass spectrometry. To this end two individual assays were developed: one for the simultaneous quantification of capecitabine, 5'-dFCR and 5'-dFUR using reversed phase chromatography and gradient elution, and one assay for 5-FU, FUH(2), FUPA and FBAL using hydrophilic interaction chromatography and isocratic elution. Both assays were fully validated according to current FDA guidelines. Total run time for the capecitabine assay was 9.0min, and of the 5-FU assay 5.0min. Analyte extraction was performed by protein precipitation. Stable labeled isotopes for each of the analytes were used as internal standards. The linear ranges of the analytes were 50-6000ng/mL for the capecitabine assay and 50-5000ng/mL for the 5-FU assay. Validation results demonstrate that capecitabine and its metabolites can be rapidly, accurately, precisely and robustly quantified in human plasma with the presented methods. Both assays are currently in extensive use in support of pharmacokinetic studies in patients treated with capecitabine or 5-FU.

Published

2012

17. Lethal morphine intoxication in a patient with a sickle cell crisis and renal impairment: case report and a review of the literature

Author

Desiderius P M Brandjes, Jurjen S. Lagas, Jos H. Beijnen, Cornelis H. W. Koks, Alwin D. R. Huitema, Michel J.X. Hillebrand, Jiri F. P. Wagenaar, and Victor E. A. Gerdes

Subjects

Male, Anemia, Health, Toxicology and Mutagenesis, Central nervous system, Poison control, Anemia, Sickle Cell, Toxicology, Cerebrospinal fluid, Fatal Outcome, Medicine, Humans, Renal Insufficiency, Respiratory system, Morphine Derivatives, Morphine, business.industry, Brain, General Medicine, Morphine-6-glucuronide, Middle Aged, medicine.disease, Heart Arrest, medicine.anatomical_structure, Anesthesia, Toxicity, business, medicine.drug

Abstract

Morphine-6-glucuronide, the active metabolite of morphine, and to a lesser extent morphine itself are known to accumulate in patients with renal failure. A number of cases on non-lethal morphine toxicity in patients with renal impairment report high plasma concentrations of morphine-6-glucuronide, suggesting that this metabolite achieves sufficiently high brain concentrations to cause long-lasting respiratory depression, despite its poor central nervous system penetration. We report a lethal morphine intoxication in a 61-year-old man with sickle cell disease and renal impairment, and we measured concentrations of morphine and morphine-6-glucuronide in blood, brain and cerebrospinal fluid. There were no measurable concentrations of morphine-6-glucuronide in cerebrospinal fluid or brain tissue, despite high blood concentrations. In contrast, the relatively high morphine concentration in the brain suggests that morphine itself was responsible for the cardiorespiratory arrest in this patient. Given the fatal outcome, we recommend to avoid repeated or continuous morphine administration in renal failure.

Published

2010

18. Identification and profiling of circulating metabolites of atazanavir, a HIV protease inhibitor

Author

Michel J.X. Hillebrand, A. D. R. Huitema, Hilde Rosing, E.C.M. van Gorp, R. ter Heine, Jos H. Beijnen, and J. W. Mulder

Subjects

Drug, Spectrometry, Mass, Electrospray Ionization, Pyridines, Omptin, Metabolite, media_common.quotation_subject, Atazanavir Sulfate, Pharmaceutical Science, Pharmacology, Hydroxylation, Specimen Handling, chemistry.chemical_compound, Tandem Mass Spectrometry, medicine, HIV Protease Inhibitor, Humans, Biotransformation, Chromatography, High Pressure Liquid, media_common, chemistry.chemical_classification, biology, Hydrolysis, virus diseases, HIV Protease Inhibitors, Atazanavir, Enzyme, Biochemistry, chemistry, Enzyme inhibitor, Dealkylation, Toxicity, biology.protein, Indicators and Reagents, Oligopeptides, medicine.drug

Abstract

Atazanavir is a commonly prescribed protease inhibitor for treatment of HIV-1 infection. Thus far, only limited data are available on the in vivo metabolism of the drug. Three systemic circulating metabolites have been reported, but their chemical structures have not been released publicly. Atazanavir metabolites may contribute to its effectiveness but also to its toxicity and interactions. Thus, there is a need for extensive metabolic profiling of atazanavir. Our goals were to screen and identify previously unknown atazanavir metabolites and to develop a sensitive metabolite profiling method in plasma. Five atazanavir metabolites were detected and identified in patient samples using liquid chromatography coupled to linear ion trap mass spectrometry: one N-dealkylation product (M1), two metabolites resulting from carbamate hydrolysis (M2 and M3), a hydroxylated product (M4), and a keto-metabolite (M5). For sensitive semiquantitative analysis of the metabolites in plasma, the method was transferred to liquid chromatography coupled to triple quadrupole mass spectrometry. In 12 patient samples, all the metabolites could be detected, and possible other potential atazanavir keto-metabolites were found. Atazanavir metabolite levels were positively correlated with atazanavir levels, but interindividual variability was high. The developed atazanavir metabolic screening method can now be used for further clinical pharmacological research with this antiretroviral agent.

Published

2009

19. Quantification of the HIV-integrase inhibitor raltegravir and detection of its main metabolite in human plasma, dried blood spots and peripheral blood mononuclear cell lysate by means of high-performance liquid chromatography tandem mass spectrometry

Author

Jos H. Beijnen, Hilde Rosing, J. W. Mulder, A. D. R. Huitema, E.C.M. van Gorp, R. ter Heine, and Michel J.X. Hillebrand

Subjects

Acetonitriles, Drug Storage, Clinical Biochemistry, Pharmaceutical Science, HIV Infections, Tandem mass spectrometry, High-performance liquid chromatography, Antiviral Agents, Sensitivity and Specificity, Analytical Chemistry, Drug Stability, Tandem Mass Spectrometry, Raltegravir Potassium, Drug Discovery, Blood plasma, Freezing, medicine, Protein precipitation, Humans, HIV Integrase Inhibitors, Desiccation, Particle Size, Spectroscopy, Chromatography, High Pressure Liquid, Chromatography, medicine.diagnostic_test, Molecular Structure, Chemistry, Methanol, Selected reaction monitoring, Reproducibility of Results, Water, Reference Standards, Pyrrolidinones, Zinc Sulfate, Triple quadrupole mass spectrometer, Solutions, Therapeutic drug monitoring, Calibration, Leukocytes, Mononuclear, Biological Assay, Drug Monitoring, Quantitative analysis (chemistry)

Abstract

For the quantification of the HIV-integrase inhibitor raltegravir in human plasma, dried blood spots and peripheral blood mononuclear cell (PBMC) lysate, an assay was developed and validated, using liquid chromatography coupled with tandem mass spectrometry. The assay also allowed detection, but no quantification due to absence of reference substance, of the main metabolite, raltegravir-glucuronide. Raltegravir was extracted from plasma by means of protein precipitation with a mixture of methanol and acetonitrile using only 50microL plasma. Extraction from dried blood spots was performed with a simple one-step extraction with a mixture of methanol, acetonitrile and 0.2M zincsulphate in water (1:1:2, v/v/v) and extraction from cell lysate was performed in 50% methanol in water. Chromatographic separation was performed on a reversed phase C18 column (150mmx2.0mm, particle size 5microm) with a quick stepwise gradient using an acetate buffer (pH 5) and methanol, at a flow rate of 0.25mL/min. The analytical run time was 10min. The triple quadrupole mass spectrometer was operated in the positive ion-mode and multiple reaction monitoring was used for drug quantification. The method was validated over a range of 50-10,000ng/mL in plasma and dried blood spots and a range of 1-500ng/mL in PBMC lysate. Dibenzepine was used as the internal standard. The method was proven to be specific, accurate, precise and robust. Accuracies ranged from 104% to 105% in plasma, from 93% to 105% in dried blood spots and from 82% to 113% in PBMC lysate. Precision over the complete concentration range was less than 6%, 11% and 13% in plasma, dried blood spots and PBMC lysate, respectively. The method is now applied for therapeutic drug monitoring and pharmacological research in HIV-infected patients treated with raltegravir.

Published

2008

20. Determination of Benzo[a]pyrene Diol Epoxide--DNA Adducts in White Blood Cell DNA From Coke-Oven Workers: The Impact of Smoking

Author

Michel J.X. Hillebrand, M. E. de Rijke, S. Oosterink, E. Kriek, F.J. van Schooten, F.E. van Leeuwen, Augustinus A. M. Hart, and H. G. van Veen

Subjects

Adult, Cancer Research, 7,8-Dihydro-7,8-dihydroxybenzo(a)pyrene 9,10-oxide, Epoxide, Enzyme-Linked Immunosorbent Assay, Air Pollutants, Occupational, Urine, complex mixtures, Dihydroxydihydrobenzopyrenes, Excretion, chemistry.chemical_compound, Personal hygiene, White blood cell, Leukocytes, polycyclic compounds, medicine, Humans, Polycyclic Compounds, Food science, Coke, Carcinogen, Pyrenes, Smoking, technology, industry, and agriculture, DNA, Middle Aged, Coal, medicine.anatomical_structure, Oncology, chemistry, Benzo(a)pyrene, Pyrene, Mutagens

Abstract

We have undertaken a study among coke-oven workers to test the feasibility of an enzyme-linked immunosorbent assay with anti-trans-7,8-dihydroxy-9,10-epoxy-7,8,9,10-tetrahydro-benzo[a]pyrene- DNA antibodies for monitoring occupational exposure to polycyclic aromatic hydrocarbons (PAH). Coke-oven workers are occupationally exposed to relatively high levels of PAH and are at increased risk for lung cancer. Three blood samples were collected from each of the 56 coke-oven workers exposed to PAH and 44 unexposed workers employed in a steel-rolling factory of the same plant. In addition, PAH levels were measured in ambient air by personal sampling, and the excretion of 1-hydroxypyrene in urine was also measured on 3 consecutive working days. All participants were interviewed regarding working conditions, personal hygiene, and smoking habits. The results showed that the coke-oven workers were exposed to substantial concentrations of atmospheric PAH (1-186 micrograms/m3), including benzo[a]pyrene (0.1-7.8 micrograms/m3) and pyrene (0.6-23.6 micrograms/m3). Both benzo[a]pyrene and pyrene were shown to be representative for the whole group of PAH. Forty-seven percent of the coke-oven workers had detectable levels of PAH-DNA adducts in their white blood cells, compared with 30% of the controls. In both groups, smokers had significantly higher levels of PAH-DNA adducts than did nonsmokers. At one site, we found the correlation positive between DNA adducts and the duration of exposure (r = .47, P = .005). Generally, the correlation was not significant between PAH-DNA adducts in blood and the concentration of PAH in the air and 1-hydroxypyrene in urine.

Published

1990

21. Polycyclic aromatic hydrocarbon-DNA adducts in lung tissue from lung cancer patients

Author

Michel J.X. Hillebrand, E. Kriek, N. van Zandwijk, J.T. Lutgerink, F.J. van Schooten, H.M. Jansen, F.E. van Leeuwen, and Other departments

Subjects

Cancer Research, Pathology, medicine.medical_specialty, Lung Neoplasms, 7,8-Dihydro-7,8-dihydroxybenzo(a)pyrene 9,10-oxide, Polycyclic aromatic hydrocarbon, Enzyme-Linked Immunosorbent Assay, Dihydroxydihydrobenzopyrenes, Adduct, DNA Adducts, chemistry.chemical_compound, DNA adduct, medicine, Humans, Polycyclic Compounds, Lung cancer, Lung, Carcinogen, chemistry.chemical_classification, Smoking, DNA, DNA, Neoplasm, General Medicine, Environmental exposure, medicine.disease, Molecular biology, chemistry, Autoradiography, Pyrene, Phosphorus Radioisotopes

Abstract

In an attempt to probe for polycyclic aromatic hydrocarbon (PAH)-DNA adducts in human subjects resulting from smoking (or other chronic environmental exposure), lung tissue and lung tumours were obtained from patients hospitalized for lung cancer. DNA was isolated from the tissue samples and examined both in an ELISA using a polyclonal antibody against (+/-)trans-7,8-dihydroxy-anti-9,10-epoxy-7,8,9,10- tetrahydrobenzo[a]pyrene (BPDE)-DNA as well as by the nuclease P1-mediated modification of the 32P-post-labelling technique. The ELISA results showed BPDE-DNA antigenicity in lung DNA from 6 out of 21 patients, and adduct levels ranged from 2 to 134 adducts per 10(8) nucleotides. For all 21 patients, the autoradiographs of chromatograms of 32P-postlabelled digests of DNA from non-tumorous lung tissue showed a strong diagonal radioactive zone (DRZ). This DRZ was generally absent in tumorous tissue. DNA samples that were positive in the ELISA contained a dominant spot within the DRZ that co-chromatographed with the major BPDE-DNA adduct (BPDE-dG). The quantities of the BPDE-dG spots ranged from 2.1 to 42 adducts in 10(9) nucleotides. These values were lower than the levels found in the ELISA but correlated well with the ELISA results (Kendall W = 0.97; P = 0.00). The levels of the DRZ adducts ranged from 1.9 to 34 adducts in 10(8) nucleotides. Correlations between smoking and DNA adduct levels were poor because of the small number of current smokers (n = 13). However, smokers of filter cigarettes had significantly lower DNA adduct levels compared with smokers of cigarettes without a filter (P = 0.02 by Fischer's exact test).

Published

1990

22. Multidrug resistance proteins 2 and 3 provide alternative routes for hepatic excretion of morphine-glucuronides

Author

Annemieke Kuil, Maria L. H. Vlaming, Michel J.X. Hillebrand, Noam Zelcer, Koen van de Wetering, Wouter Feddema, Alfred H. Schinkel, Jos H. Beijnen, Piet Borst, Other departments, AII - Amsterdam institute for Infection and Immunity, CCA -Cancer Center Amsterdam, Pathology, and Medical Biochemistry

Subjects

Metabolite, Glucuronidation, Biology, Pharmacology, Spodoptera, Cell Line, Excretion, chemistry.chemical_compound, Mice, In vivo, Animals, Humans, Secretion, Glucuronosyltransferase, Morphine Derivatives, Multidrug resistance-associated protein 2, Membrane Transport Proteins, Apical membrane, Multidrug Resistance-Associated Protein 2, chemistry, Biochemistry, Liver, Molecular Medicine, Multidrug Resistance-Associated Proteins, Intracellular

Abstract

Glucuronidation is a major hepatic detoxification pathway for endogenous and exogenous compounds, resulting in the intracellular formation of polar metabolites that require specialized transporters for elimination. Multidrug resistance proteins (MRPs) are expressed in the liver and can transport glucuronosyl-conjugates. Using morphine as a model aglycone, we demonstrate that morphine-3-glucuronide (M3G), the predominant metabolite, is transported in vitro by human MRP2 (ABCC2), a protein present in the apical membrane of hepatocytes. Loss of biliary M3G secretion in Mrp2(-/-) mice results in its increased sinusoidal transport that can be attributed to Mrp3. Combined loss of Mrp2 and Mrp3 leads to a substantial accumulation of M3G in the liver, from which it is transported across the sinusoidal membrane at a low rate, resulting in the prolonged presence of M3G in plasma. Our results show that murine Mrp2 and Mrp3 provide alternative routes for the excretion of a glucuronidated substrate from the liver in vivo.

Published

2007

23. Quantitative analysis of EO9 (apaziquone) and its metabolite EO5a in human plasma by high-performance liquid chromatography under basic conditions coupled to electrospray tandem mass spectrometry

Author

Dorla Mirejovsky, Luigi Lenaz, Jos H. Beijnen, Van Huynh, Hilde Rosing, Michel J.X. Hillebrand, Liia D. Vainchtein, and Jan H.M. Schellens

Subjects

Quality Control, Electrospray, Spectrometry, Mass, Electrospray Ionization, Chromatography, Metabolite, Aziridines, Ethyl acetate, Reproducibility of Results, Reference Standards, Tandem mass spectrometry, High-performance liquid chromatography, chemistry.chemical_compound, Column chromatography, chemistry, Calibration, Humans, Sample preparation, Indolequinones, Quantitative analysis (chemistry), Antineoplastic Agents, Alkylating, Spectroscopy, Chromatography, High Pressure Liquid

Abstract

A sensitive and specific LC-MS/MS assay for the quantitative determination of EO9 and its metabolite EO5a is presented. A 200-µl human plasma aliquot was spiked with a mixture of deuterated internal standards EO9-d3 and EO5a-d4 and extracted with 1.25 ml ethyl acetate. Dried extracts were reconstituted in 0.1 M ammonium acetate—methanol (7 : 3, v/v) and 25 µl-volumes were injected into the HPLC system. Separation was achieved on a 150 × 2.1 mm C18 column using an alkaline eluent (1 mM ammonium hydroxide—methanol (gradient system)). Detection was performed by positive ion electrospray followed by tandem mass spectrometry. The assay quantifies a range from 5 to 2500 ng/ml for EO9 and from 10 to 2500 ng/ml EO5a using 200 µl of human plasma samples. Validation results demonstrate that EO9 and EO5a concentrations can be accurately and precisely quantified in human plasma. This assay will be used to support clinical pharmacologic studies with EO9. Copyright © 2006 John Wiley & Sons, Ltd.

Published

2006

24. Sensitive inductively coupled plasma mass spectrometry assay for the determination of platinum originating from cisplatin, carboplatin, and oxaliplatin in human plasma ultrafiltrate

Author

Jan H.M. Schellens, Michel J.X. Hillebrand, Markus Joerger, Jos H. Beijnen, Elke E.M. Brouwers, Matthijs M. Tibben, and Hilde Rosing

Subjects

Quality Control, Bioanalysis, endocrine system diseases, Organoplatinum Compounds, chemistry.chemical_element, Ultrafiltration, Antineoplastic Agents, Mass spectrometry, Mass Spectrometry, Carboplatin, Matrix (chemical analysis), chemistry.chemical_compound, medicine, Humans, Inductively coupled plasma mass spectrometry, Spectroscopy, Platinum, Cisplatin, Chromatography, Chemistry, Reproducibility of Results, Reference Standards, female genital diseases and pregnancy complications, Oxaliplatin, Calibration, Indicators and Reagents, medicine.drug

Abstract

We present a highly sensitive, rapid method for the determination of platinum originating from the anticancer agents cisplatin, carboplatin, and oxaliplatin in human plasma ultrafiltrate. The method is based on the quantification of platinum by inductively coupled plasma mass spectrometry and allows quantification of 7.50 ng l-1 platinum in only 150 microl of matrix. Sample pretreatment involves dilution of samples with 1% HNO3. Validation fulfilled the most recent FDA guidelines for bioanalytical method validation. Validated ranges of quantification were 7.50 ng l-1 to 1.00x10(5) ng l-1 in plasma ultrafiltrate for all three platinum compounds. The assay is now successfully used to support pharmacokinetic studies in cancer patients treated with cisplatin, carboplatin, or oxaliplatin.

Published

2006

25. Screening for illicit heroin use in patients in a heroin-assisted treatment program

Author

Michel J.X. Hillebrand, Alwin D. R. Huitema, Wim van den Brink, Jan M. van Ree, Jos H. Beijnen, Elisabeth J. Rook, Amsterdam Neuroscience, and Adult Psychiatry

Subjects

Adult, Male, medicine.medical_specialty, Time Factors, Health, Toxicology and Mutagenesis, Toxicology, Mass Spectrometry, Analytical Chemistry, Heroin, Internal medicine, Surveys and Questionnaires, mental disorders, medicine, Environmental Chemistry, Humans, In patient, Illicit heroin, Clinical Trials as Topic, Chemical Health and Safety, Chromatography, medicine.diagnostic_test, business.industry, Codeine, Heroin Dependence, Illicit Drugs, Mass spectrometric, Substance Abuse Detection, Heroin-assisted treatment, Therapeutic drug monitoring, Female, business, Biomarkers, Methadone, medicine.drug, Chromatography, Liquid

Abstract

The aim of this study was to investigate the use of illicit heroin among patients in a heroin-assisted treatment program. In this program, pharmaceutical-grade heroin was administered to heroin-addicted patients. Monitoring of illicit heroin use was considered important for the evaluation of this treatment program. Acetylcodeine and codeine, common adulterants of "street" heroin, were used as markers for illicit heroin. A liquid chromatography method with tandem mass spectrometric detection (LC-MS-MS) was developed, for quantitative analysis of heroin and methadone, their metabolites, and the simultaneous detection of acetylcodeine. One-hundred patients in a heroin-assisted treatment program were screened for acetylcodeine in plasma. Furthermore, patients were interviewed about illicit heroin use, and they were tested for alcohol and cocaine use. In plasma samples of 16% of the patients, acetylcodeine was detected. Overall agreement between self-report and plasma samples was 95% (kappa: 0.81). Patients who tested positive for acetylcodeine had visited the outpatients' clinics significantly less frequently than the patients who tested negative. Alcohol and cocaine use was more common in patients who tested positive for acetylcodeine. Illicit heroin use was observed in a limited percentage of patients. Overall agreement between self-report and markers of illicit heroin use was good.

Published

2006

26. Metabolism of trabectedin (ET-743, Yondelis) in patients with advanced cancer

Author

Luis Lopez-Lazaro, Jan H. Beumer, Michel J.X. Hillebrand, Jeany M. Rademaker-Lakhai, Jos H. Beijnen, Jan H.M. Schellens, Hilde Rosing, and Tessa M. Bosch

Subjects

Cancer Research, Metabolite, Urine, Dioxoles, Pharmacology, Biology, Toxicology, Mass Spectrometry, Excretion, chemistry.chemical_compound, Feces, Glucuronides, Pharmacokinetics, Neoplasms, Tetrahydroisoquinolines, medicine, Humans, Pharmacology (medical), CYP2C9, Antineoplastic Agents, Alkylating, Trabectedin, Chromatography, Polymorphism, Genetic, Cancer, medicine.disease, Oncology, chemistry, Glucuronide, medicine.drug

Abstract

Trabectedin (ET-743, Yondelis™) is a novel anti-cancer drug currently undergoing phase II–III evaluation, that has shown remarkable activity in pre-treated patients with soft tissue sarcoma. Despite extensive pharmacokinetic studies, the human disposition and metabolism of trabectedin remain largely unknown. We aimed to determine the metabolic profile of trabectedin and to identify its metabolites in humans. We analysed urine and faeces (the major excretory route) from eight cancer patients after a 3 or 24 h intravenous administration of [14C]trabectedin. Using liquid chromatography with tandem quadrupole mass spectrometric detection (LC-MS/MS) and radiochromatography with off-line radioactivity detection by liquid scintillation counting (LC-LSC), we characterised the metabolic profile in 0–24 h urine and 0–120 h faeces. By radiochromatography, a large number of trabectedin metabolites were detected. Incubation with β-glucuronidase indicated the presence of a glucuronide metabolite in urine. Trabectedin, ET-745, ET-759A, ETM-259, ETM-217 (all available as reference compounds) and a proposed new metabolite coined ET-731 were detected using LC-MS/MS. The inter-individual differences in radiochromatographic profiles were small and did not correlate with polymorphisms in drug-metabolising enzymes (CYP2C9, 2C19, 2D6, 2E1, 3A4, GST-M1, P1, T1 and UGT1A1 2B15) as determined by genotyping. Trabectedin is metabolically converted to a large number of compounds that are excreted in both urine and faeces. In urine and faeces we have confirmed the presence of trabectedin, ET-745, ET-759A, ETM-259, ETM-217 and ETM-204. In addition we have identified a putative new metabolite designated ET-731. Future studies should be aimed at further identification of possible metabolites and assessment of their activity.

Published

2006

27. Analysis of diacetylmorphine, caffeine, and degradation products after volatilization of pharmaceutical heroin for inhalation

Author

Wim van den Brink, Michel J.X. Hillebrand, Marjolein G. Klous, WeiChing Lee, Jan M. van Ree, Jos H. Beijnen, ANS - Amsterdam Neuroscience, and Adult Psychiatry

Subjects

Male, Narcotics, Spectrometry, Mass, Electrospray Ionization, Health, Toxicology and Mutagenesis, Chasing the dragon, Toxicology, Analytical Chemistry, Heroin, chemistry.chemical_compound, Caffeine, mental disorders, medicine, Humans, Environmental Chemistry, Chromatography, High Pressure Liquid, Inhalation Exposure, Chemical Health and Safety, Volatilisation, Chromatography, Inhalation, Morphine derivatives, Smoking, Diacetylmorphine, Substance Abuse Detection, chemistry, Central Nervous System Stimulants, Volatilization, medicine.drug, Methadone

Abstract

Pharmaceutical smokable heroin was developed for a clinical trial on medical co-prescription of heroin and methadone. This product, consisting of 75% w/w diacetylmorphine base and 25% w/w caffeine anhydrate, was intended for use via "chasing the dragon", that is, inhalation after volatilization. This procedure involves heating the powder mixture, which may lead to formation of degradation products that could subsequently be inhaled. We developed a method that used a high-performance liquid chromatography system that was compatible with photodiode-array detection and mass spectrometric detection to separate diacetylmorphine- and caffeine-related compounds in a wide polarity range for analysis of the vapor. This method was used to analyze the contents of the plastic drinking straws that were used by patients to inhale the vapors from pharmaceutical heroin used via chasing the dragon, which were considered to be representative of the vapors the patients inhaled. They contained primarily unchanged diacetylmorphine, its main metabolite 6-acetylmorphine, caffeine, and some morphine. Several unidentified peaks were observed in the straw chromatograms. Chemical structures were proposed for nine degradation products: morphine derivatives with different substitution patterns of the C(3), C(6), and/or N(17) positions, which comprised 0.4-9.7% of the straw sample residue weight. Activity and toxicity of most of these compounds are unknown and require further investigation.

Published

2006

28. Mice lacking multidrug resistance protein 3 show altered morphine pharmacokinetics and morphine-6-glucuronide antinociception

Author

Noam Zelcer, Annemieke Kuil, Koen van de Wetering, Peter R. Wielinga, Michel J.X. Hillebrand, Jos H. Beijnen, Thomas R. Tephly, Piet Borst, Elise Sarton, Albert Dahan, Other departments, AII - Amsterdam institute for Infection and Immunity, CCA -Cancer Center Amsterdam, and Pathology

Subjects

Glucuronosyltransferase, ATP Binding Cassette Transporter, Subfamily B, Glucuronidation, Pharmacology, Spodoptera, Cell Line, Mice, Pharmacokinetics, medicine, Animals, Bile, Humans, Tissue Distribution, Transport Vesicles, Epithelial polarity, Pain Measurement, Mice, Knockout, Morphine Derivatives, Multidisciplinary, biology, Morphine, Chemistry, Morphine-6-glucuronide, Biological Sciences, In vitro, Transport protein, Protein Transport, Liver, biology.protein, ATP-Binding Cassette Transporters, medicine.drug

Abstract

Glucuronidation is a major detoxification pathway for endogenous and exogenous compounds in mammals that results in the intracellular formation of polar metabolites, requiring specialized transporters to cross biological membranes. By using morphine as a model aglycone, we demonstrate that multidrug resistance protein 3 (MRP3/ABCC3), a protein present in the basolateral membrane of polarized cells, transports morphine-3-glucuronide (M3G) and morphine-6-glucuronide in vitro . Mrp3 (-/-) mice are unable to excrete M3G from the liver into the bloodstream, the major hepatic elimination route for this drug. This results in increased levels of M3G in liver and bile, a 50-fold reduction in the plasma levels of M3G, and in a major shift in the main disposition route for morphine and M3G, predominantly via the urine in WT mice but via the feces in Mrp3 (-/-) mice. The pharamacokinetics of injected morphine-glucuronides are altered as well in the absence of Mrp3, and this results in a decreased antinociceptive potency of injected morphine-6-glucuronide.

Published

2005

29. Pharmacokinetic comparison of two methods of heroin smoking: 'chasing the dragon' versus the use of a heating device

Author

Jan M. van Ree, Michel J.X. Hillebrand, Elisabeth J. Rook, Marjolein G. Klous, Jos H. Beijnen, Vincent M. Hendriks, Alwin D. R. Huitema, Wim van den Brink, Amsterdam Neuroscience, and Adult Psychiatry

Subjects

Adult, Male, Narcotics, Chasing the dragon, Pharmacology, Heroin, Pharmacokinetics, Caffeine, Smoke, mental disorders, Administration, Inhalation, medicine, Humans, Pharmacology (medical), Biological Psychiatry, Psychiatric Status Rating Scales, Inhalation, business.industry, Heroin Dependence, Middle Aged, Mass spectrometric, Psychiatry and Mental health, Neurology, Anesthesia, Plasma concentration, Morphine, Central Nervous System Stimulants, Neurology (clinical), business, medicine.drug, Methadone, Half-Life

Abstract

In preparation for a trial on co-prescription of inhalable heroin and methadone, two methods for inhalation of heroin/caffeine tablets were compared: the commonly used method of 'chasing the dragon' and a standardised procedure for inhalation of volatilised heroin, using a heating device. Five male addicts inhaled a tablet of smokable heroin daily for 5 days, alternating the inhalation method. Plasma concentrations of heroin, 6-acetylmorphine, morphine and morphine-3- and -6-glucuronide were determined using a liquid chromatography method with tandem mass spectrometric detection. The exposure to heroin and its metabolites (expressed as areas under the concentrationtime curve) was significantly lower after smoking via the heating device than after 'chasing the dragon': heroin 80% and 6-acetylmorphine 73% lower (p

Published

2004

30. Simultaneous quantification of cyclophosphamide, 4-hydroxycyclophosphamide, N,N',N'-triethylenethiophosphoramide (thiotepa) and N,N',N'-triethylenephosphoramide (tepa) in human plasma by high-performance liquid chromatography coupled with electrospray ionization tandem mass spectrometry

Author

Alwin D. R. Huitema, Selma M van Dam, Milly E de Jonge, Michel J.X. Hillebrand, Sjoerd Rodenhuis, Hilde Rosing, Jos H. Beijnen, and Other departments

Subjects

Spectrometry, Mass, Electrospray Ionization, Chromatography, Chemistry, Electrospray ionization, Selected reaction monitoring, Reproducibility of Results, ThioTEPA, Mass spectrometry, High-performance liquid chromatography, Sensitivity and Specificity, Triple quadrupole mass spectrometer, Triethylenephosphoramide, Liquid chromatography–mass spectrometry, Neoplasms, medicine, Humans, Sample collection, Drug Monitoring, Antineoplastic Agents, Alkylating, Cyclophosphamide, Spectroscopy, Chromatography, High Pressure Liquid, Thiotepa, medicine.drug

Abstract

The alkylating agents cyclophosphamide (CP) and N, N', N"-triethylenethiophosphoramide (thiotepa) are often co-administered in high-dose chemotherapy regimens. Since these regimens can be complicated by the occurrence of severe and sometimes life-threatening toxicities, pharmacokinetically guided administration of these compounds, to reduce variability in exposure, may lead to improved tolerability. For rapid dose adaptations during a chemotherapy course, we have developed and validated an assay, using liquid chromatography coupled with electrospray tandem mass spectrometry (LC/MS/MS), for the routine quantification of CP, thiotepa and their respective active metabolites 4-hydroxycyclophosphamide (4OHCP) and N, N', N"-triethylenephosphoramide (tepa) in plasma. Because of the instability of 4OHCP in plasma, the compound is derivatized with semicarbazide (SCZ) immediately after sample collection and quantified as 4OHCP-SCZ. Sample pretreatment consisted of protein precipitation with a mixture of methanol and acetronitrile using 100 microl of plasma. Chromatographic separation was performed on an Zorbax Extend C18 column (150 x 2.1 mm i.d., particle size 5 microm), with a quick gradient using 1 mM ammonia solution and acetonitrile, at a flow-rate of 0.4 ml min(-1). The analytical run time was 10 min. The triple quadrupole mass spectrometer was operating in the positive ion mode and multiple reaction monitoring was used for drug quantification. The method was validated over the concentration ranges 200-40,000 ng ml(-1) for CP, 50-5000 ng ml(-1) for 4OHCP-SCZ and 5-2500 ng ml(-1) for thiotepa and tepa, using 100 microl of human plasma. These dynamic concentration ranges proved to be relevant in daily practice. Hexamethylphosphoramide was used as an internal standard. The coefficients of variation were

Published

2004

31. Simultaneous quantification of the new HIV protease inhibitors atazanavir and tipranavir in human plasma by high-performance liquid chromatography coupled with electrospray ionization tandem mass spectrometry

Author

Hilde Rosing, Michel J.X. Hillebrand, Jos H. Beijnen, A. D. R. Huitema, and Kristel M. L. Crommentuyn

Subjects

Spectrometry, Mass, Electrospray Ionization, Pyridines, Electrospray ionization, Clinical Biochemistry, Atazanavir Sulfate, HIV Infections, Tandem mass spectrometry, Biochemistry, High-performance liquid chromatography, Sensitivity and Specificity, Analytical Chemistry, medicine, Protein precipitation, Humans, Chromatography, High Pressure Liquid, Sulfonamides, Chromatography, Chemistry, Selected reaction monitoring, Reproducibility of Results, Cell Biology, General Medicine, HIV Protease Inhibitors, Triple quadrupole mass spectrometer, Atazanavir, Pyrones, Tipranavir, Oligopeptides, medicine.drug

Abstract

We have developed and validated an assay, using liquid chromatography coupled with electrospray tandem mass spectrometry (LC-MS/MS), for the quantification of the novel protease inhibitors (PIs) atazanavir and tipranavir. The sample pre-treatment consisted of protein precipitation with a mixture of methanol and acetronitrile using 100 microl plasma for atazanavir and 50 microl for tipranavir. Chromatographic separation was achieved on an Inertsil ODS3 column (50 mm x 2.0 mm i.d., particle size 5 microm), with a quick stepwise gradient using an acetate buffer (pH 5) and methanol, at a flow rate of 0.5 ml/min. The analytical run time was 5.5 min. The triple quadrupole mass spectrometer operated in the positive ion-mode and multiple reaction monitoring (MRM) was used for drug quantification. The assay was linear over a concentration range of 0.05-10 microg/ml for atazanavir and 0.1-75 microg/ml for tipranavir. Saquinavir-d5 was used as internal standard. The intra- and inter-day coefficients of variation were less than 3.8% for atazanavir and less than 10.4% for tipranavir. Accuracies were within +/-7.3 and +/-7.2% for atazanavir and tipranavir, respectively. Both drugs were stable under various relevant storage conditions. The validated concentration ranges proved to be adequate to measure concentrations of human immunodeficiency virus type-1 (HIV-1)-infected individuals. The developed method could easily be combined with a previously developed LC-MS/MS assay for the quantification of protease inhibitors.

Published

2003

32. Rapid quantification of HIV protease inhibitors in human plasma by high-performance liquid chromatography coupled with electrospray ionization tandem mass spectrometry

Author

Hilde Rosing, Kristel M. L. Crommentuyn, A. D. R. Huitema, Lianda G. A. H. Nan-Offeringa, Michel J.X. Hillebrand, and Jos H. Beijnen

Subjects

Spectrometry, Mass, Electrospray Ionization, Chromatography, Chemistry, Selected reaction monitoring, virus diseases, Reproducibility of Results, Lopinavir, HIV Protease Inhibitors, High-performance liquid chromatography, Sensitivity and Specificity, Amprenavir, Nelfinavir, Liquid chromatography–mass spectrometry, medicine, Humans, Ritonavir, Drug Monitoring, Saquinavir, Spectroscopy, Chromatography, High Pressure Liquid, medicine.drug

Abstract

HIV protease inhibitors are important antiretroviral drugs which have substantially reduced the morbidity and mortality associated with HIV-1 infection. Recent data have shown relationships between plasma concentrations of the protease inhibitors and clinical response, which makes therapeutic drug monitoring valuable. We have developed and validated an assay, using liquid chromatography coupled with electrospray tandem mass spectrometry (LC/MS/MS), for the routine quantification of the six licensed protease inhibitors (amprenavir, indinavir, lopinavir, nelfinavir, ritonavir and saquinavir) and the pharmacologically active nelfinavir metabolite M8 in plasma. The sample pretreatment consisted of protein precipitation with a mixture of methanol and acetronitrile using only 100 µl of plasma. Chromatographic separation was performed on an Inertsil ODS3 column (50 × 2.0 mm i.d., particle size 5 µm), with a quick stepwise gradient using an acetate buffer (pH 5) and methanol, at a flow rate of 0.5 ml min−1. The analytical run time was 5.5 min. The use of a 96-well plate autosampler allowed batch sizes up to 150 patient samples. The triple-quadrupole mass spectrometer was operated in the positive ion mode and multiple reaction monitoring was used for drug quantification. The method was validated over the concentration ranges 0.01–10 µg ml−1 for indinavir and saquinavir, 0.1–10 µg ml−1 for amprenavir, 0.05–10 µg ml−1 for nelfinavir and ritonavir, 0.1–20 µg ml−1 for lopinavir and 0.01–5 µg ml−1 for M8. Saquinavir-d5 and indinavir-d6 were used as internal standards. The coefficients of variation were always

Published

2003

33. A comparison of limited sampling strategies for prediction of Ecteinascidin 743 clearance when administered as a 24-h infusion

Author

Hilde Rosing, Michel J.X. Hillebrand, E. Brain, Jan H.M. Schellens, Cecilia Guzman, J. L. Misset, Luis Lopez-Lazaro, Ron A. A. Mathot, A. Taamma, Charlotte van Kesteren, Esteban Cvitkovic, Jos H. Beijnen, and J. Jimeno

Subjects

Adult, Cancer Research, Time Factors, Population, Bayesian probability, Dioxoles, Toxicology, Pharmacokinetics, Tetrahydroisoquinolines, Linear regression, Statistics, Limited sampling, Humans, Pharmacology (medical), education, Infusions, Intravenous, Antineoplastic Agents, Alkylating, Mathematics, Pharmacology, education.field_of_study, Bayes estimator, Blood Specimen Collection, Dose-Response Relationship, Drug, Bayes Theorem, Stepwise regression, Models, Theoretical, Isoquinolines, Data set, Oncology, Regression Analysis, Forecasting, Half-Life, Trabectedin

Abstract

Purpose: Ecteinascidin 743 (ET-743) is a novel, marine-derived anticancer agent currently under clinical development for the treatment of solid tumors. The aim of this study was to develop and validate limited sampling strategies for the prediction of ET-743 clearance in phase II studies, using two techniques: the stepwise linear regression approach and the Bayesian estimation approach. Methods: Data from a phase I dose-finding study were used with ET-743 administered as a 24-h infusion. Plasma concentration time data from 34 patients treated with 1200, 1500 or 1800 µg/m2 ET-743 were randomly divided into an index data set, used for the development of the strategies, and a validation data set. With the linear regression approach, clearance (obtained by non-compartmental analysis) was correlated with the ratios of dose to the observed concentrations. For the Bayesian approach a three-compartment population pharmacokinetic model was developed; optimal time-points were selected using the D-optimality algorithm. The strategies were compared by assessment of their predictive performance of CL in the validation data set. Results: The linear regression method yielded a single-point sampling schedule with no significant bias and acceptable precision (–0.03% and 21%, respectively). With the Bayesian approach, a three-sample strategy was selected which resulted in less-accurate, but unbiased, predictions (bias 13%, precision 34%). Conclusions: Optimal sampling strategies were developed and validated for estimation of ET-743 clearance. Although the linear regression approach showed slightly better predictive performance, the Bayesian approach is preferred for the current phase II studies as it is more robust and flexible and allows the description of the full pharmacokinetic profile.

Published

2002

34. Clinical pharmacology of the novel marine-derived anticancer agent Ecteinascidin 743 administered as a 1- and 3-h infusion in a phase I study

Author

John F. Smyth, Andrew Simpson, Ron A. A. Mathôt, Hilde Rosing, Chris Twelves, Cecilia Guzman, Jose Jimeno, Jan H.M. Schellens, Jos H. Beijnen, Klaas Hoekman, Michel J.X. Hillebrand, Luis Lopez-Lazaro, A. Bowman, Jan B. Vermorken, Charlotte van Kesteren, and Other departments

Subjects

Adult, Male, Cancer Research, Time Factors, Maximum Tolerated Dose, Dioxoles, Pharmacology, Ecteinascidia turbinata, law.invention, Pharmacokinetics, law, Tetrahydroisoquinolines, medicine, Dose escalation, Animals, Humans, Pharmacology (medical), Platelet, Urochordata, Infusions, Intravenous, Antineoplastic Agents, Alkylating, Fatigue, Aged, Clinical pharmacology, biology, business.industry, Middle Aged, medicine.disease, biology.organism_classification, Isoquinolines, Pancytopenia, Thrombocytopenia, Phase i study, Oncology, Area Under Curve, Plasma concentration, Female, business, Half-Life, Trabectedin

Abstract

Ecteinascidin 743 (ET-743) is an anticancer agent derived from the Caribbean tunicate Ecteinascidia turbinata. In the present article, the pharmacokinetics and pharmacodynamics of ET-743 are described within a phase I study. Forty patients with solid tumors initially received ET-743 as a 1-h i.v. infusion every 21 days at nine dose levels (50-1100 microg/m(2)). The maximal tolerated dose (MTD) was 1100 microg/m(2), with thrombocytopenia and fatigue as dose-limiting toxicities (DLTs). As this MTD was substantially lower than in parallel phase I studies, dose escalation continued using a prolonged, 3-h infusion. Thirty-two patients were entered at five dose levels (1000-1800 microg/m(2)). The MTD was 1800 microg/m(2) with pancytopenia and fatigue as DLTs. The recommended phase II dose was 1650 microg/m(2) given over 3 h at which 12 patients were treated. Pharmacokinetic monitoring was performed for both treatment schedules. Non-compartmental pharmacokinetic parameters at the recommended dose with the 3-h infusion were (mean value+/-SD): clearance 87+/-30 l/h and mean elimination half-life 26+/-7 h. Pharmacokinetics were linear at the dose range tested with this schedule. The percentage decrease in platelets, white blood cells and neutrophils correlated with the area under the plasma concentration versus time curve (AUC), dose and maximal plasma concentration (C(max)). Hepatic toxicity increased with dose, AUC and C(max). Administration of 1650 microg/m(2) ET-743 over 3 h seemed clinically feasible; pharmacokinetics were linear with this schedule. Hepatic and hematological toxicities correlated with exposure to ET-743.

Published

2002

35. Search for metabolites of ecteinascidin 743, a novel, marine-derived, anti-cancer agent, in man

Author

J. Jimeno, Esteban Cvitkovic, Michel J.X. Hillebrand, Jan H.M. Schellens, van Oosterom At, Jos H. Beijnen, Luis Lopez-Lazaro, Ignacio Manzanares, Hilde Rosing, Rolf W. Sparidans, and van Kesteren C

Subjects

Cancer Research, Urine, Dioxoles, chemistry.chemical_compound, Plasma, Glucuronides, Tetrahydroisoquinolines, Transferase, Humans, Pharmacology (medical), Glucuronosyltransferase, Antineoplastic Agents, Alkylating, Chromatography, High Pressure Liquid, Pharmacology, chemistry.chemical_classification, Chromatography, Chemistry, Metabolism, Isoquinolines, Uridine, In vitro, Enzyme, Oncology, Area Under Curve, Microsome, Microsomes, Liver, Glucuronide, Trabectedin

Abstract

Ecteinascidin 743 (ET-743) is a potent anti-tumoral agent of a marine origin. It is currently being tested in phase II clinical trials using a 3-weekly 24-h i.v. infusion of 1500 microg/m(2) and 3-h infusions of 1650 microg/m(2). Knowledge of the metabolism of ET-743 is, however, still scarce. In the present study, a qualitative chromatographic discovery of metabolites of ET-743 in man is reported. ET-743 and its demethylated analog ET-729 were incubated at 37 degrees C in the presence of enzyme systems, pooled human microsomes, pooled human plasma and uridine 5'-diphosphoglucuronyltransferase, respectively, in appropriate media. Reaction products were investigated chromatographically using photodiode array and ion spray-mass spectrometric detection (LC-MS). The main reaction products in microsomal incubations of ET-743 resulted from a remarkable breakdown of the molecule. In plasma the drugs were deacetylated, and the transferase did actually yield a glucuronide of both ET-743 and ET-729. In contrast, screening of urine, plasma and bile, collected from patients treated with ET-743 at the highest dose levels, using a sensitive LC-MS assay, did not result in detection of ET-729 and metabolites which were generated in vitro. The urinary excretion of ET-743 in man was lower than 0.7% of the administered dose for a 24-h infusion.

Published

2001

36. Phase I and pharmacologic study of weekly doxorubicin and 1 h infusional paclitaxel in patients with advanced breast cancer

Author

Jan H.M. Schellens, van Tellingen O, Michel J.X. Hillebrand, Koopman Fj, R. Dubbelman, Jos H. Beijnen, Hilde Rosing, Vinodh R. Nannan Panday, and ten Bokkel Huinink Ww

Subjects

Oncology, Adult, Glycerol, Cancer Research, medicine.medical_specialty, Neutropenia, Paclitaxel, Antineoplastic Agents, Breast Neoplasms, Drug Administration Schedule, chemistry.chemical_compound, Breast cancer, Pharmacokinetics, Internal medicine, Antineoplastic Combined Chemotherapy Protocols, medicine, Humans, Pharmacology (medical), Doxorubicin, Infusions, Intravenous, Stomatitis, Pharmacology, Dose-Response Relationship, Drug, business.industry, Cancer, Alopecia, Middle Aged, medicine.disease, Metastatic breast cancer, chemistry, Female, business, medicine.drug

Abstract

Doxorubicin and paclitaxel both display strong antitumor activity in the treatment of breast cancer. The optimal schedule of this combination, however, remains undefined. In this phase I and pharmacologic study, we administered weekly 12 mg/m2 doxorubicin as a bolus infusion immediately followed by a 1 h 80 mg/m2 paclitaxel infusion to patients with metastatic breast cancer. A total of 119 weekly courses were delivered to seven patients. Grade IV neutropenia was observed in two patients at the first dose level, thus already defining the maximum tolerated dose. Pronounced non-hematologic toxicities were mild neuropathy (grade I: 39%) and stomatitis (grade I: 19%, grade II: 8%). No signs of cardiac toxicity were observed with this dose schedule. Three partial responses were achieved in this group of heavily pretreated patients. The pharmacokinetics of paclitaxel, doxorubicin and Cremophor EL with this schedule were analyzed. Overall, the schedule was well tolerated and combined with its preliminary response rate justifies further evaluation in phase II studies.

Published

1998

37. High-performance liquid chromatographic analysis of the investigational anticancer drug 9-aminocamptothecin, as the lactone form and as the total of the lactone and the hydroxycarboxylate forms, in micro-volumes of human plasma

Author

Michel J.X. Hillebrand, R. van Gijn, Auke Bult, W.W. ten Bokkel Huinink, Jos H. Beijnen, and V. M. M. Herben

Subjects

chemistry.chemical_classification, Detection limit, Chromatography, Clinical Biochemistry, Pharmaceutical Science, Reproducibility of Results, Antineoplastic Agents, Reversed-phase chromatography, High-performance liquid chromatography, Analytical Chemistry, Lactones, Column chromatography, chemistry, Drug Stability, Drug Discovery, Humans, Camptothecin, Solid phase extraction, Aminocamptothecin, Colorectal Neoplasms, Quantitative analysis (chemistry), Spectroscopy, Lactone, Chromatography, High Pressure Liquid, Aged

Abstract

A high performance liquid chromatographic (HPLC) assay is described for the determination of the investigational anticancer drug 9 aminocamptothecin (9-AC) as the lactone form (9AC(lac)) and as the total of the lactone and hydroxycarboxylate forms (9AC-(tot)), in micro volumes of plasma. The analytical methodology reported here involves a protein precipitation step with cold methanol (-30 degrees C) as sample pretreatment procedure. The methanolic extract is used for the determination of 9AC-(tot). The intact (active) lactone form of 9-AC is separated from the hydroxycarboxylate form in the methanolic plasma extract by solid phase extraction within 48 h after sampling and deproteination. After evaporation to dryness (nitrogen, 40 degrees C) the extract can be stored at -70 degrees C for at least 3 weeks. The drug is analysed by reversed-phase liquid chromatography on a Zorbax SB RP-18 column, using methanol-water eluent (pH 2.2) and fluorescence detection. The presented assay is linear over a concentration range 0.2-100 ng.ml-1 with a detection limit and a limit of quantitation of 0.05 and 0.2 ng.ml-1, respectively, for both 9-AC(tot) and 9-AC(lac) using a 100 ml plasma sample. The proposed method has been implemented in a phase I clinical trial for pharmacokinetic evaluation of this potential new drug.

Published

1998

38. Analysis of Ecteinascidin 743, a new potent marine-derived anticancer drug, in human plasma by high-performance liquid chromatography in combination with solid-phase extraction

Author

Jan B. Vermorken, Jos H. Beijnen, Glynn Faircloth, Auke Bult, Pablo Floriano, Hilde Rosing, L. Cameron, Roland E. C. Henrar, Michel J.X. Hillebrand, A. Gomez, and Jose Jimeno

Subjects

Antineoplastic Agents, Dioxoles, Sensitivity and Specificity, High-performance liquid chromatography, Column chromatography, Tetrahydroisoquinolines, Spectrophotometry, Blood plasma, medicine, Animals, Humans, Urochordata, Solid phase extraction, Chromatography, High Pressure Liquid, Chromatography, medicine.diagnostic_test, Chemistry, Reproducibility of Results, General Chemistry, Isoquinolines, Anticancer drug, Evaluation Studies as Topic, Spectrophotometry, Ultraviolet, Particle size, Quantitative analysis (chemistry), Trabectedin

Abstract

A reversed-phase high-performance liquid chromatographic method has been developed and validated for the quantification of the novel anticancer drug Ecteinascidin 743 in human plasma. The sample pretreatment of the plasma samples involved a solid-phase extraction (SPE) on cyano columns. Propyl-p-hydroxybenzoate was added after the sample pretreatment to correct for variability in injection volumes. The separation was performed on a Zorbax SB-C18 column (75x4.6 mm I.D., particle size 3.5 microm) with acetonitrile-25 mM phosphate buffer, pH 5.0 (70:30, v/v) as the mobile phase. The flow-rate was 1.0 ml/min and the eluent was monitored at 210 nm. The accuracies and precisions of the assay fall within +/-15% for all quality control samples and within +/-20% for the lower limit of quantitation, which was 1.0 ng/ml using 500 microl of plasma. The overall recovery of the sample pretreatment procedure for Ecteinascidin 743 was 87.0+/-5.9%. The drug was found to be stable in human plasma at -30 degrees C for at least 2 months. At room temperature Ecteinascidin 743 was stable in human plasma for 5 h at most.

Published

1998

39. Analytical procedure for the determination of the new antitumour drug N-benzoylstaurosporine and three potential metabolites in human plasma by reversed-phase high-performance liquid chromatography

Author

P. Graf, R. van Gijn, E. Boven, J. H. Beijnen, Michel J.X. Hillebrand, J.J.M. de Clippeleir, S. Schwertz, O. van Tellingen, W.W. ten Bokkel Huinink, and Jan B. Vermorken

Subjects

Male, Analyte, Metabolite, Antineoplastic Agents, High-performance liquid chromatography, Sensitivity and Specificity, chemistry.chemical_compound, Alkaloids, Pharmacokinetics, Drug Stability, In vivo, Freezing, Diisopropyl ether, Animals, Humans, Chromatography, High Pressure Liquid, Protein Kinase C, Detection limit, Chromatography, Molecular Structure, General Chemistry, Staurosporine, Rats, chemistry, Quantitative analysis (chemistry), Ethers

Abstract

The staurosporine derivative, N-benzoylstaurosporine (CGP 41 251; I), is a protein kinase C inhibitor that has been selected for phase I clinical evaluation in cancer patients. We have developed a selective and sensitive assay of the drug and three potential metabolites in human plasma. The method is based on reversed-phase high-performance liquid chromatography with fluorescence detection. The sample pretreatment involves liquid-liquid extraction with diisopropyl ether with recoveries over 88%. The limit of detection and limit of quantitation of the parent compound and two metabolites were 0.5 and 1.0 ng/ml, respectively. For the third metabolite the limit of detection and limit of quantitation were 1.0 and 2.0 ng/ml, respectively. Linear calibration lines were obtained over the range of 1-1000 ng/ml. The between-day and within-day precisions were < 7.1% for all the analytes. In plasma the compounds were stable for at least one month if stored at -30 degrees C or below. The applicability of the method for in vivo studies has been demonstrated in a pharmacokinetic study in rat receiving 0.5 mg/kg of the drug as an intravenous bolus injection. Compound I and two metabolites were detected.

Published

1995

40. Validation of a new fluorometric assay for benzo[a]pyrene diolepoxide-DNA adducts in human white blood cells: comparisons with 32P-postlabeling and ELISA

Author

Michel J.X. Hillebrand, Margarita Rojas, E. Kriek, Helmut Bartsch, Frederik-Jan van Schooten, and Kroum Alexandrov

Subjects

Cancer Research, Lung Neoplasms, Lymphocyte, Enzyme-Linked Immunosorbent Assay, Sensitivity and Specificity, Fluorescence, Adduct, chemistry.chemical_compound, DNA Adducts, polycyclic compounds, medicine, Benzo(a)pyrene, Leukocytes, Humans, Nucleotide, Benzopyrenes, Chromatography, High Pressure Liquid, chemistry.chemical_classification, Detection limit, General Medicine, DNA, Molecular biology, medicine.anatomical_structure, chemistry, Biochemistry, Pyrene, Quantitative analysis (chemistry), Phosphorus Radioisotopes

Abstract

A new fluorometric assay was validated for quantification of benzo[a]pyrene diolepoxide (BPDE)-DNA adducts in white blood cells (WBC) from humans exposed to polycyclic aromatic hydrocarbons (PAH). This assay has a detection limit of 2 pg of r-7,c-10,t-8,t-9-tetrahydroxy-7,8,9,10-tetrahydrobenzo[a]pyrene derived from acid hydrolysis of BPDE-DNA, and can measure 1 BPDE adduct per 10(8) unmodified nucleotides. The quantity of WBC DNA required depends on the modification level and varies between 5 and 500 micrograms. The assay was applied to seven WBC DNA samples from lung cancer patients, six of whom were heavy smokers, and to three WBC DNA samples from healthy subjects employed in an aluminum production plant. High levels of BPDE-DNA adducts, ranging from 62 to 533 adducts/10(8) nucleotides were found in six out of seven DNA samples from the lung cancer patients. In WBC DNA from healthy persons BPDE-DNA adducts were detected only in two non-smokers, but at a much lower level than in lung cancer patients (4-10 adducts/10(8) nucleotides). Using coded WBC DNA samples, BPDE-DNA adduct levels measured by fluorometry of the B[a]P-tetrols, were compared with the results obtained by 32P-postlabeling (nuclease P1 enrichment) and ELISA measurements. A good correlation and proportionality was found between the levels of BPDE-DNA adducts measured by fluorometry and 32P-postlabeling (r = 0.95, P < 0.001, n = 8). The correlation between fluorometry and ELISA was much lower and not significant (r = 0.61, P = 0.1, n = 6). Moreover, the ELISA grossly overestimated BPDE-DNA adduct levels measured by the other two methods. The results demonstrate that the highly sensitive and specific fluorometric assay is suitable for measuring BPDE-DNA adducts in WBC from humans exposed to benzo[a]pyrene.

Published

1994

41. DNA adducts as a measure of lung cancer risk in humans exposed to polycyclic aromatic hydrocarbons

Author

Michel J.X. Hillebrand, F.J. van Schooten, A. P. G. Dijkmans, E. Kriek, A. J. A. De Looff, F.E. van Leeuwen, and L. Den Engelse

Subjects

Lung Neoplasms, DNA damage, Health, Toxicology and Mutagenesis, Aluminum industry, complex mixtures, Adduct, chemistry.chemical_compound, Risk Factors, Occupational Exposure, medicine, Leukocytes, Humans, Polycyclic Compounds, Lung cancer, Coke, Chemistry, Public Health, Environmental and Occupational Health, food and beverages, DNA, medicine.disease, Biological materials, respiratory tract diseases, Occupational Diseases, Increased risk, Environmental chemistry, Occupational exposure, Aluminum, DNA Damage, Research Article

Abstract

Workers in the coking, foundry, and aluminum industry can be exposed to high concentrations of polycyclic aromatic hydrocarbons (PAHs) and are at increased risk for lung cancer, as are cigarette smokers. In recent years several studies on workers in the foundry and coking industries have been reported. In these studies, white blood cell(WBC) DNA was used for analysis of PAH-DNA adducts. Theoretically, DNA adduct formation is a more relevant biological parameter for assessing exposure risk than PAH in the work atmosphere, or the amount of a metabolite in the urine, because adduct levels reflect that part of the dose that escapes detoxification and binds to DNA. We analyzed WBC DNA from coke-oven workers and from workers in an aluminum production plant and demonstrated the presence of PAH-DNA adducts. Forty-seven percent of the coke-oven workers had detectable levels of PAH-DNA adducts in their WBC compared with 27% of the controls (p < 0.05), measured with ELISA. In both groups, smokers had significantly higher levels of PAH-DNA adducts than did nonsmokers. In the aluminum workers, no PAH-DNA adducts were detected by ELISA, although the benzo[a]pyrene concentrations in the work atmosphere were comparable to those of the coke-oven workers. The more sensitive 32P-postlabeling assay showed the presence of PAH-DNA adducts in 91% of the aluminum workers. There was no correlation of WBC adduct levels with the concentration of PAH in the work atmosphere. Recently we showed that total PAH-DNA adduct levels in WBC from lung cancer patients were much higher than those generally found in healthy smokers.(ABSTRACT TRUNCATED AT 250 WORDS)

Published

1993

42. Phase I and Pharmacokinetic Study of a Daily Times 5 Short Intravenous Infusion Schedule of 9-Aminocamptothecin in a Colloidal Dispersion Formulation in Patients With Advanced Solid Tumors

Author

Margaret Schot, V. M. M. Herben, Jan Lieverst, Maria Grazia Porro, Michel J.X. Hillebrand, Nadja E. Schoemaker, Jan H.M. Schellens, Wim W. ten Bokkel Huinink, Jos H. Beijnen, and Roel van Gijn

Subjects

Adult, Male, Cancer Research, medicine.medical_specialty, Neutropenia, medicine.medical_treatment, Urology, Antineoplastic Agents, Drug Administration Schedule, Dosage form, Lactones, Pharmacokinetics, Refractory, Neoplasms, medicine, Humans, In patient, Colloids, Infusions, Intravenous, Aged, Drug Carriers, Chemotherapy, Dose-Response Relationship, Drug, business.industry, Nausea, Middle Aged, medicine.disease, Thrombocytopenia, Hematopoiesis, Surgery, Oncology, Area Under Curve, Camptothecin, Female, Aminocamptothecin, business, Standard therapy

Abstract

PURPOSE: To determine the maximum-tolerated dose (MTD), dose-limiting toxicities (DLT), and pharmacokinetics of 9-aminocamptothecin (9-AC) in a colloidal dispersion (CD) formulation administered as a 30-minute intravenous (IV) infusion over 5 consecutive days every 3 weeks. PATIENTS AND METHODS: Patients with solid tumors refractory to standard therapy were entered onto the study. The starting dose was 0.4 mg/m2/d. The MTD was assessed on the first cycle and was defined as the dose at which ≥ two of three patients or ≥ two of six patients experience DLT. Pharmacokinetic measurements were performed on days 1 and 5 of the first cycle and on day 4 of subsequent cycles using high-performance liquid chromatography. RESULTS: Thirty-one patients received 104+ treatment courses at seven dose levels. The DLT was hematologic. At a dose of 1.3 mg/m2/d, three of six patients experienced grade 3 thrombocytopenia. Grade 4 neutropenia that lasted less than 7 days was observed in four patients. At a dose of 1.1 mg/m2/d, four of nine patients had grade 4 neutropenia of brief duration, which was not dose limiting. Nonhematologic toxicities were relatively mild and included nausea/vomiting, diarrhea, obstipation, mucositis, fatigue, and alopecia. Maximal plasma concentrations and area under the concentration-time curve (AUC) increased linearly with dose, but interpatient variation was wide. Lactone concentrations exceeded 10 nmol/L, the threshold for activity in preclinical tumor models, at all dose levels. Sigmoidal Emax models could be fit to the relationship between AUC and the degree of hematologic toxicity. A partial response was observed in small-cell lung cancer. CONCLUSION: 9-AC CD administered as a 30-minute IV infusion daily times 5 every three weeks is safe and feasible. The recommended phase II dose is 1.1 mg/m2/d.

Published

1999

43. POLYCYCLIC AROMATIC HYDROCARBON-DNA ADDUCTS IN WHITE BLOOD CELLS FROM LUNG CANCER PATIENTS NO CORRELATION WITH ADDUCT LEVELS IN LUNG

Author

L. Den Engelse, E. Kriek, F.J. van Schooten, H.M. Jansen, F.E. van Leeuwen, N. van Zandwijk, Michel J.X. Hillebrand, and Other departments

Subjects

Adult, Male, Cancer Research, Lung Neoplasms, DNA damage, 7,8-Dihydro-7,8-dihydroxybenzo(a)pyrene 9,10-oxide, Polycyclic aromatic hydrocarbon, Enzyme-Linked Immunosorbent Assay, Adduct, chemistry.chemical_compound, DNA Adducts, DNA adduct, medicine, Leukocytes, Humans, Nucleotide, Lung cancer, Lung, Carcinogen, Aged, chemistry.chemical_classification, Aged, 80 and over, Smoking, General Medicine, DNA, Middle Aged, medicine.disease, Molecular biology, chemistry, Biochemistry, Autoradiography, Female, Chromatography, Thin Layer

Abstract

Smokers of cigarettes are exposed to a number of carcinogens, including polycyclic aromatic hydrocarbons (PAHs), and are at a high risk for lung cancer. PAHs exert their carcinogenic activity after metabolic activation to reactive intermediates that can damage DNA through adduct formation. Measuring DNA adducts in peripheral white blood cells (WBC) could serve as a means of monitoring human exposure to genotoxic agents and subsequently risk assessment. In this study, DNA from WBC obtained from 39 lung cancer patients was examined for PAH-DNA adducts both in an ELISA using a polyclonal antibody against benzo[a]pyrene 7,8-diol-9,10-epoxide (BPDE)-DNA and the 32P-post-labeling technique. The ELISA results showed BPDE-DNA antigenicity in WBC DNA from 12/38 (32%) patients and adduct levels ranged from 1.5 to greater than 150 adducts in 10(8) nucleotides. The autoradiographs of chromatograms of 32P-post-labeled digests of WBC DNA from the 38 patients showed a variety of adduct spots; relative adduct labeling (RAL) values ranged from 0.3 to 407 adducts in 10(8) nucleotides. In 18 of the 38 (47%) persons an adduct spot was detected that co-chromatographed with the major BPDE-DNA adduct (BPDE-dG); RAL values ranged from 0.03 to 382 adducts in 10(8) nucleotides. Correlations were not significant between the adduct levels in WBC and smoking habits, age or sex. From 20 patients of the same group lung tissue was collected at surgery and examined for PAH-DNA adducts by ELISA and 32P-post-labeling assay. No significant correlation was found between DNA adduct levels in blood and lung. This finding stresses the limitations of the use of WBC as a surrogate for adduct levels in the target organ.