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2. Identification of drug metabolites with infrared ion spectroscopy – application to midazolam in vitro metabolism

Author

Rianne van Outersterp, Jonathan Martens, Giel berden, Arnaud Lubin, Filip Cuyckens, and Jos Oomens

Abstract

The identification of biotransformation products of drug compounds is a crucial step in drug development. Over the last decades, liquid chromatography-mass spectrometry (LC-MS) has become the method of choice for metabolite profiling because of its high sensitivity and selectivity. However, determining the full molecular structure of the detected metabolites, including the exact biotransformation site, remains challenging on the basis of MS alone. Here we explore infrared ion spectroscopy (IRIS) as a novel MS-based method for the elucidation of metabolic pathways in drug metabolism research. Using the drug midazolam as an example, we identify several biotransformation products directly from an in vitro drug incubation sample. We show that IR spectra of the aglycone MS/MS fragment ions of glucuronide metabolites establish a direct link between detected phase I and phase II metabolites. Moreover, using quantum-chemically computed IR spectra of candidate structures, we are able to assign the exact sites of biotransformation in absence of reference standards. Additionally, we demonstrate the utility of IRIS for structural elucidation by identifying several ring-opened midazolam derivatives formed in an acidic environment.

Published
2022
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3. Flexible nano- and microliter injections on a single liquid chromatography–mass spectrometry system: Minimizing sample preparation and maximizing linear dynamic range

Author

Patrick Augustijns, Sheng Sheng, Filip Cuyckens, Deirdre Cabooter, and Arnaud Lubin

Subjects
0301 basic medicine, Detection limit, Analyte, Chromatography, Chemistry, Dynamic range, 010401 analytical chemistry, Organic Chemistry, Analytical chemistry, General Medicine, Tandem mass spectrometry, 01 natural sciences, Biochemistry, Chemistry Techniques, Analytical, Specimen Handling, 0104 chemical sciences, Analytical Chemistry, Dilution, 03 medical and health sciences, 030104 developmental biology, Adsorption, Tandem Mass Spectrometry, Liquid chromatography–mass spectrometry, Sample preparation, Chromatography, Liquid
Abstract

Lack of knowledge on the expected concentration range or insufficient linear dynamic range of the analytical method applied are common challenges for the analytical scientist. Samples that are above the upper limit of quantification are typically diluted and reanalyzed. The analysis of undiluted highly concentrated samples can cause contamination of the system, while the dilution step is time consuming and as the case for any sample preparation step, also potentially leads to precipitation, adsorption or degradation of the analytes. ispartof: Journal of Chromatography A vol:1524 pages:101-107 ispartof: location:Netherlands status: published

Published
2017
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4. Strategies and analytical workflows to extend the dynamic range in quantitative LC-MS/MS analysis

Author

Tania Aerts, Lieve Dillen, Emmanuel Njumbe Ediage, Arnaud Lubin, Tom Verhaeghe, and Filip Cuyckens

Subjects
Quality Control, Bioanalysis, Computer science, Dynamic range, 010401 analytical chemistry, Clinical Biochemistry, Clinical Chemistry Tests, General Medicine, 010402 general chemistry, 01 natural sciences, 0104 chemical sciences, Analytical Chemistry, Dilution, Workflow, Medical Laboratory Technology, Tandem Mass Spectrometry, Lc ms ms, Injection volume, Calibration, General Pharmacology, Toxicology and Pharmaceutics, Biological system, Chromatography, Liquid
Abstract

Aim: To evaluate alternative analytical strategies to extend the dynamic range in quantitative LC–MS/MS. Methods & results: Two approaches based on prior or no prior knowledge of expected exposure levels were evaluated. These approaches make use of two analytical strategies, which include the use of more than one injection volume or dilution of sample extract with solvents or solvent mixtures. A total of 16 compounds with varying logP values were classified into polar and nonpolar groups and used in this evaluation. From the two analytical strategies, three workflows were derived. Conclusion: All three workflows were successfully evaluated and resulted in good accuracy (80–120%) for all the compound groups.

Published
2019

5. Enhanced performance for the analysis of prostaglandins and thromboxanes by liquid chromatography-tandem mass spectrometry using a new atmospheric pressure ionization source

Author

Steve Bajic, Rob J. Vreeken, Suzy Geerinckx, Patrick Augustijns, Deirdre Cabooter, Filip Cuyckens, and Arnaud Lubin

Subjects
0301 basic medicine, Spectrometry, Mass, Electrospray Ionization, Electrospray, Colon, Swine, Electrospray ionization, Analytical chemistry, 01 natural sciences, Biochemistry, Chemistry Techniques, Analytical, Analytical Chemistry, Mice, 03 medical and health sciences, Tandem Mass Spectrometry, Liquid chromatography–mass spectrometry, Ionization, Animals, Humans, Sample preparation, chemistry.chemical_classification, Chromatography, Atmospheric pressure, Chemistry, 010401 analytical chemistry, Organic Chemistry, Reproducibility of Results, Thromboxanes, General Medicine, 0104 chemical sciences, Atmospheric Pressure, 030104 developmental biology, Prostaglandins, Eicosanoids, lipids (amino acids, peptides, and proteins), Polyunsaturated fatty acid
Abstract

Eicosanoids, including prostaglandins and thromboxanes are lipid mediators synthetized from polyunsaturated fatty acids. They play an important role in cell signaling and are often reported as inflammatory markers. LC-MS/MS is the technique of choice for the analysis of these compounds, often in combination with advanced sample preparation techniques. Here we report a head to head comparison between an electrospray ionization source (ESI) and a new atmospheric pressure ionization source (UniSpray). The performance of both interfaces was evaluated in various matrices such as human plasma, pig colon and mouse colon. The UniSpray source shows an increase in method sensitivity up to a factor 5. Equivalent to better linearity and repeatability on various matrices as well as an increase in signal intensity were observed in comparison to ESI. publisher: Elsevier articletitle: Enhanced performance for the analysis of prostaglandins and thromboxanes by liquid chromatography-tandem mass spectrometry using a new atmospheric pressure ionization source journaltitle: Journal of Chromatography A articlelink: http://dx.doi.org/10.1016/j.chroma.2016.02.055 content_type: article copyright: Copyright © 2016 Elsevier B.V. All rights reserved. ispartof: Journal of Chromatography A vol:1440 pages:260-5 ispartof: location:Netherlands status: published

Published
2016
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6. One drop chemical derivatization - DESI-MS analysis for metabolite structure identification

Author

Filip Cuyckens, Arnaud Lubin, Deirdre Cabooter, and Patrick Augustijns

Subjects
Hydroxylation, chemistry.chemical_compound, Analyte, Electrospray, Chromatography, chemistry, Metabolite, Desorption, Hydrogen–deuterium exchange, Derivatization, Mass spectrometry, Spectroscopy
Abstract

Structural elucidation of metabolites is an important part during the discovery and development process of new pharmaceutical drugs. Liquid Chromatography (LC) in combination with Mass Spectrometry (MS) is usually the technique of choice for structural identification but cannot always provide precise structural identification of the studied metabolite (e.g. site of hydroxylation and site of glucuronidation). In order to identify those metabolites, different approaches are used combined with MS data including nuclear magnetic resonance, hydrogen/deuterium exchange and chemical derivatization followed by LC-MS. Those techniques are often time-consuming and/or require extra sample pre-treatment. In this paper, a fast and easy to set up tool using desorption electrospray ionization-MS for metabolite identification is presented. In the developed method, analytes in solution are simply dried on a glass plate with printed Teflon spots and then a single drop of derivatization mixture is added. Once the spot is dried, the derivatized compound is analyzed. Six classic chemical derivatizations were adjusted to work as a one drop reaction and applied on a list of compounds with relevant functional groups. Subsequently, two successive reactions on a single spot of amoxicillin were tested and the methodology described was successfully applied on an in vitro incubated alprazolam metabolite. All reactions and analyses were performed within an hour and gave useful structural information by derivatizing functional groups, making the method a time-saving and efficient tool for metabolite identification if used in addition or in some cases as an alternative to common methods.

Published
2015
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7. An atmospheric pressure ionization source using a high voltage target compared to electrospray ionization for the LC/MS analysis of pharmaceutical compounds

Author

Ronald de Vries, Arnaud Lubin, Filip Cuyckens, Patrick Augustijns, and Deirdre Cabooter

Subjects
Electrospray, Spectrometry, Mass, Electrospray Ionization, Chromatography, Chemistry, Electrospray ionization, 010401 analytical chemistry, Clinical Biochemistry, Analytical chemistry, Extractive electrospray ionization, Pharmaceutical Science, Atmospheric-pressure chemical ionization, 010402 general chemistry, Mass spectrometry, 01 natural sciences, 0104 chemical sciences, Analytical Chemistry, Atmospheric Pressure, Liquid chromatography–mass spectrometry, Ionization, Drug Discovery, Direct electron ionization liquid chromatography–mass spectrometry interface, Spectroscopy, Chromatography, High Pressure Liquid, Chromatography, Liquid
Abstract

The type and design of an ionization source can have a significant influence on the performances of a bioanalytical method. It is, therefore, of high interest to evaluate the performances of newly introduced sources to highlight their benefits and limitations in comparison to other well established sources. In this paper, liquid chromatography - mass spectrometry (LC/MS) performances of a new atmospheric pressure ionization (API) source, commercialized as UniSpray, is evaluated. The dynamic range of 24 pharmaceutical and biological compounds is compared between the new API source and electrospray ionization (ESI) for 3 different mobile phase conditions. Matrix effects are also compared with ESI on a refined selection of 19 pharmaceutical and biological compounds in 4 matrices commonly encountered in bioanalysis. A slightly better dynamic range towards lower concentrations was often observed with the new API source. Matrix effects were quite similar between the two sources with a small, but statistically significant, lower percentage of matrix effects observed for the new API source in plasma and bile in the positive ion mode, and bile in negative ion mode for ESI. Finally, the sensitivity of late eluting compounds could be improved on the new API source by post-column addition of water.

Published
2017

8. Atmospheric Pressure Ionization Using a High Voltage Target Compared to Electrospray Ionization

Author

Steve Bajic, Deirdre Cabooter, Arnaud Lubin, Patrick Augustijns, and Filip Cuyckens

Subjects
0301 basic medicine, Desorption electrospray ionization, Chemistry, Electrospray ionization, 010401 analytical chemistry, Analytical chemistry, Extractive electrospray ionization, Atmospheric-pressure chemical ionization, Mass spectrometry, 01 natural sciences, 0104 chemical sciences, 03 medical and health sciences, Matrix-assisted laser desorption/ionization, 030104 developmental biology, Structural Biology, Direct electron ionization liquid chromatography–mass spectrometry interface, Spectroscopy, Ambient ionization
Abstract

A new atmospheric pressure ionization (API) source, viz. UniSpray, was evaluated for mass spectrometry (MS) analysis of pharmaceutical compounds by head-to-head comparison with electrospray ionization (ESI) on the same high-resolution MS system. The atmospheric pressure ionization source is composed of a grounded nebulizer spraying onto a high voltage, cylindrical stainless steel target. Molecules are ionized in a similar fashion to electrospray ionization, predominantly producing protonated or deprotonated species. Adduct formation (e.g., proton and sodium adducts) and in-source fragmentation is shown to be almost identical between the two sources. The performance of the new API source was compared with electrospray by infusion of a mix of 22 pharmaceutical compounds with a wide variety of functional groups and physico-chemical properties (molecular weight, logP, and pKa) in more than 100 different conditions (mobile phase strength, solvents, pH, and flow rate). The new API source shows an intensity gain of a factor 2.2 compared with ESI considering all conditions on all compounds tested. Finally, some hypotheses on the ionization mechanism, similarities, and differences with ESI, are discussed. Graphical Abstract ᅟ.

Published
2016

9. One drop chemical derivatization - DESI-MS analysis for metabolite structure identification

Author

Arnaud Lubin, Deirdre Cabooter, Patrick Augustijns, and Filip Cuyckens

Subjects
Spectroscopy
Abstract

Structural elucidation of metabolites is an important part during the discovery and development process of new pharmaceutical drugs. Liquid Chromatography (LC) in combination with Mass Spectrometry (MS) is usually the technique of choice for structural identification but cannot always provide precise structural identification of the studied metabolite (e.g. site of hydroxylation and site of glucuronidation). In order to identify those metabolites, different approaches are used combined with MS data including nuclear magnetic resonance, hydrogen/deuterium exchange and chemical derivatization followed by LC-MS. Those techniques are often time-consuming and/or require extra sample pre-treatment. In this paper, a fast and easy to set up tool using desorption electrospray ionization-MS for metabolite identification is presented. In the developed method, analytes in solution are simply dried on a glass plate with printed Teflon spots and then a single drop of derivatization mixture is added. Once the spot is dried, the derivatized compound is analyzed. Six classic chemical derivatizations were adjusted to work as a one drop reaction and applied on a list of compounds with relevant functional groups. Subsequently, two successive reactions on a single spot of amoxicillin were tested and the methodology described was successfully applied on an in vitro incubated alprazolam metabolite. All reactions and analyses were performed within an hour and gave useful structural information by derivatizing functional groups, making the method a time-saving and efficient tool for metabolite identification if used in addition or in some cases as an alternative to common methods. ispartof: Journal of Mass Spectrometry vol:50 issue:7 pages:871-878 ispartof: location:England status: published

Published
2015

10. One drop chemical derivatization--DESI-MS analysis for metabolite structure identification

Author

Arnaud, Lubin, Deirdre, Cabooter, Patrick, Augustijns, and Filip, Cuyckens

Subjects
Spectrometry, Mass, Electrospray Ionization, Drug Discovery, Biological Assay
Abstract

Structural elucidation of metabolites is an important part during the discovery and development process of new pharmaceutical drugs. Liquid Chromatography (LC) in combination with Mass Spectrometry (MS) is usually the technique of choice for structural identification but cannot always provide precise structural identification of the studied metabolite (e.g. site of hydroxylation and site of glucuronidation). In order to identify those metabolites, different approaches are used combined with MS data including nuclear magnetic resonance, hydrogen/deuterium exchange and chemical derivatization followed by LC-MS. Those techniques are often time-consuming and/or require extra sample pre-treatment. In this paper, a fast and easy to set up tool using desorption electrospray ionization-MS for metabolite identification is presented. In the developed method, analytes in solution are simply dried on a glass plate with printed Teflon spots and then a single drop of derivatization mixture is added. Once the spot is dried, the derivatized compound is analyzed. Six classic chemical derivatizations were adjusted to work as a one drop reaction and applied on a list of compounds with relevant functional groups. Subsequently, two successive reactions on a single spot of amoxicillin were tested and the methodology described was successfully applied on an in vitro incubated alprazolam metabolite. All reactions and analyses were performed within an hour and gave useful structural information by derivatizing functional groups, making the method a time-saving and efficient tool for metabolite identification if used in addition or in some cases as an alternative to common methods.

Published
2015

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