Distribution of clomipramine, citalopram, midazolam, and metabolites in skeletal tissue after chronic dosing in rats

Vandenbosch, Michiel; Somers, Tomas; Cuypers, Eva

doi:10.1002/dta.2578

“…During the last decade, the interest in the usage of skeletal tissue as an alternative specimen in forensic toxicology has seen a revival [12][13][14]. It is shown that the bone tissue acts as a depot for certain drugs [12].…”

Section: Introductionmentioning

confidence: 99%

Sample preparation of bone tissue for MALDI-MSI for forensic and (pre)clinical applications

Vandenbosch

¹

,

Nauta

²

,

Svirkova

³

et al. 2020

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In the past decades, matrix-assisted laser desorption/ionization mass spectrometry imaging (MALDI-MSI) has been applied to a broad range of biological samples, e.g., forensics and preclinical samples. The use of MALDI-MSI for the analysis of bone tissue has been limited due to the insulating properties of the material but more importantly the absence of a proper sample preparation protocol for undecalcified bone tissue. Undecalcified sections are preferred to retain sample integrity as much as possible or to study the tissue-bone bio interface in particular. Here, we optimized the sample preparation protocol of undecalcified bone samples, aimed at both targeted and untargeted applications for forensic and preclinical applications, respectively. Different concentrations of gelatin and carboxymethyl cellulose (CMC) were tested as embedding materials. The composition of 20% gelatin and 7.5% CMC showed to support the tissue best while sectioning. Bone tissue has to be sectioned with a tungsten carbide knife in a longitudinal fashion, while the sections need to be supported with double-sided tapes to maintain the morphology of the tissue. The developed sectioning method was shown to be applicable on rat and mouse as well as human bone samples. Targeted (methadone and EDDP) as well as untargeted (unknown lipids) detection was demonstrated. DHB proved to be the most suitable matrix for the detection of methadone and EDDP in positive ion mode. The limit of detection (LOD) is estimated to approximately 50 pg/spot on bone tissue. The protocol was successfully applied to detect the presence of methadone and EDDP in a dosed rat femur and a dosed human clavicle. The best matrices for the untargeted detection of unknown lipids in mouse hind legs in positive ion mode were CHCA and DHB based on the number of tissue-specific peaks and signal-to-noise ratios. The developed and optimized sample preparation method, applicable on animal and human bones, opens the door for future forensic and (pre)clinical investigations.

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“…higher than the quantitation limits of the corresponding published HPLC-ESI-MS/MS methods (0.5 ng mL À1 for clomipramine, [36] 0.1 ng mL À1 for chlorphenamine, [37] and 5.1 ng mL À1 for atenolol [38] )h owever these methods used QQQ MS instruments,w hich offer better quantitative performance and higher sensitivity in the multiple reaction mode (MRM) than the quadrupole Ion Tr ap mass analyzer used here, [39,40] and chlorphenamine method utilized aLLE step in which the extract was evaporated to dryness and reconstituted in as maller volume. [37] Ab etter sensitivity was enabled for pindolol by the in-syringe EkE approach (LOQ of 6.1 ng mL À1 in human serum) compared to the HPLC-ESI-MS/MS method (LOQ of 10 ng mL À1 in human serum [41] ) where the latter used protein precipitation.…”

Section: Forschungsartikelmentioning

confidence: 80%

In‐Syringe Electrokinetic Protein Removal from Biological Samples prior to Electrospray Ionization Mass Spectrometry

Mikhail

¹

,

Tehranirokh²,

Gooley³

et al. 2020

Angewandte Chemie

0

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Here,a ne lectrokinetic extraction (EkE) syringe is presented allowing for on-line electrokinetic removal of serum proteins before ESI-MS.The proposed concept is demonstrated by the determination of pharmaceuticals from human serum within minutes,w ith sample preparation limited to a5 dilution of the sample in the background electrolyte (BGE) and application of voltage,both of which can be performed insyringe.S ignal enhancements of 3.6-32 fold relative to direct infusion of diluted serum and up to 10.8 fold enhancement, were obtained for basic and acidic pharmaceuticals,r espectively.Linear correlations for the basic drugs by EkE-ESI-MS/ MS were achieved,c overing the necessary clinical range with LOQs of 5.3, 7.8, 6.1, and 17.8 ng mL À1 for clomipramine, chlorphenamine,p indolol, and atenolol, respectively.F or the acidic drugs,t he EkE-ESI-MS LOQs were 3.1 mgmL À1 and 2.9 mgmL À1 for naproxen and paracetamol, respectively.T he EkE-ESI-MS and EkE-ESI-MS/MS methods showed good accuracy (%found of 81 %to120 %), precision (20 %), and linearity (r > 0.997) for all the studied drugs in spiked serum samples.

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“…Chemie higher than the quantitation limits of the corresponding published HPLC-ESI-MS/MS methods (0.5 ng mL À1 for clomipramine, [36] 0.1 ng mL À1 for chlorphenamine, [37] and 5.1 ng mL À1 for atenolol [38] )h owever these methods used QQQ MS instruments,w hich offer better quantitative performance and higher sensitivity in the multiple reaction mode (MRM) than the quadrupole Ion Tr ap mass analyzer used here, [39,40] and chlorphenamine method utilized aLLE step in which the extract was evaporated to dryness and reconstituted in as maller volume. [37] Ab etter sensitivity was enabled for pindolol by the in-syringe EkE approach (LOQ of 6.1 ng mL À1 in human serum) compared to the HPLC-ESI-MS/MS method (LOQ of 10 ng mL À1 in human serum [41] ) where the latter used protein precipitation.…”

Section: Methodsmentioning

confidence: 94%

In‐Syringe Electrokinetic Protein Removal from Biological Samples prior to Electrospray Ionization Mass Spectrometry

Mikhail

¹

,

Tehranirokh²,

Gooley³

et al. 2020

View full text Add to dashboard Cite

Here,a ne lectrokinetic extraction (EkE) syringe is presented allowing for on-line electrokinetic removal of serum proteins before ESI-MS.The proposed concept is demonstrated by the determination of pharmaceuticals from human serum within minutes,w ith sample preparation limited to a5 dilution of the sample in the background electrolyte (BGE) and application of voltage,both of which can be performed insyringe.S ignal enhancements of 3.6-32 fold relative to direct infusion of diluted serum and up to 10.8 fold enhancement, were obtained for basic and acidic pharmaceuticals,r espectively.Linear correlations for the basic drugs by EkE-ESI-MS/ MS were achieved,c overing the necessary clinical range with LOQs of 5.3, 7.8, 6.1, and 17.8 ng mL À1 for clomipramine, chlorphenamine,p indolol, and atenolol, respectively.F or the acidic drugs,t he EkE-ESI-MS LOQs were 3.1 mgmL À1 and 2.9 mgmL À1 for naproxen and paracetamol, respectively.T he EkE-ESI-MS and EkE-ESI-MS/MS methods showed good accuracy (%found of 81 %to120 %), precision (20 %), and linearity (r > 0.997) for all the studied drugs in spiked serum samples.

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Distribution of clomipramine, citalopram, midazolam, and metabolites in skeletal tissue after chronic dosing in rats

Cited by 9 publications

References 31 publications

Sample preparation of bone tissue for MALDI-MSI for forensic and (pre)clinical applications

Sample preparation of bone tissue for MALDI-MSI for forensic and (pre)clinical applications

In‐Syringe Electrokinetic Protein Removal from Biological Samples prior to Electrospray Ionization Mass Spectrometry

In‐Syringe Electrokinetic Protein Removal from Biological Samples prior to Electrospray Ionization Mass Spectrometry

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