Determination of cholesterol in fat and muscle of pig by HPLC and capillary gas chromatography with solvent venting injection

Two methods for determination of cholesterol in fat and muscle of pig were evaluated: extraction with chloroform:methanol (2:1, v/v) followed by saponification (method 1) and direct saponification (method 2). HPLC and GC were used to determine cholesterol concentrations. GC analysis was performed with a capillary column of 100 μm using a PTV injector in the modes of cold split and solvent venting. Cholesterol was analyzed without derivatization. Both methods of extraction did not present significant differences (p > 0.01). Sample analysis by GC with solvent venting injection and HPLC showed the lowest % r.s.d. but GC in the cold split mode allowed to obtain a shorter analysis time. Cholesterol concentrations obtained by HPLC were not statistically different from the results obtained by GC with solvent venting injection and were slightly lower than those previously reported. Cholesterol concentrations in fat and muscle tissues respectively ranged from 52 to 77 mg/100 g and from 55 to 65 mg/100 g.     

Analysis of nonylphenol polyethoxycarboxylates and their related metabolites by on-line derivatization and ion-trap gas chromatography-mass spectrometry

This study presents a modified method to analyze nonylphenol polyethoxycarboxylates (NPEC) and their related metabolites (carboxyalkylphenol ethoxycarboxylates (CNPEC)) in water samples. The method involves extraction of samples by a graphitized carbon black (GCB) cartridge, and direct derivatization in the GC injection-port using a large-volume (10-20 microl) direct sample introduction (DSI) device with tetraalkylammonium (TAA) salts. The analytes are identified and quantitated by ion-trap GC-MS. The large-volume DSI injection-port derivatization technique provides sensitivity, fast and reproducible results for NPEC and their metabolites, to quantitation at 0.1 microg/l in 200 ml of water samples. The retention effect of TAA salts in the injection-port is not detected. In addition, the significant [M-29]+ ions and molecular ions of butylated NPEC and CNPEC residues are observed. Recovery of NP1EC in spiked water samples ranges from 90 to 108%. Moreover, relative standard deviations of replicate analyses ranges from 1 to 9%. However, unsatisfactory on-line derivatization of CNPEC residues is observed. This finding maybe owing to their lesser dissociation with the ion-pair reagent in chloroform.     

Sample preparation for organic acids in biological fluids

A review of sample preparation methods for organic acids in biological fluids, in particular serum and urine, is presented. It covers techniques on organic acid determination without sample preparation, release of organic acids from binding locations, removal of proteins by protein precipitation and ultrafiltration, isolation of the organic acids by liquid-liquid and liquid-solid extraction, purification of the extract, derivatization and pre-fractionation. The various alternative sample preparation steps are compared and critically discussed. Examples of applications including profile analysis of organic acids by gas chromatography (GC), determination of particular organic acids by GC or liquid chromatography and determination of fatty acids as a distinct chemical class of acids demonstrate that the kind of sample preparation chosen depends strongly on the analytical aims.     

气相色谱/电子捕获检测法测定键合态糖苷的研究

该文建立了GC/ECD法测定键合态糖苷的分析方法,采用N-甲基-双(三氟乙酰胺)(MBTFA)对目标物进行衍生,并优化了反应温度和时间.结果表明在60℃下反应50 min时,衍生效果最好.该衍生反应在产物中引入氟元素,可用GC/JECD法进行测定.以苯氧基葡萄糖苷为典型目标物进行线性研究,方法在0.05～200 mg/...     

Experimental design for the study of two derivatization procedures for simultaneous GC analysis of acidic herbicides and water chlorination by-products

Two well known derivatization procedures, pentafluorobenzylation and BF(3)/methanol esterification, were compared for their applications to GC analysis of acidic water micropollutants (chloroacetic and phenoxyalkanoic acids). A two-level factorial design was used to determine the influence of different parameters and their interactions on each derivatization process. The studied parameters are the reaction time, the amount of reagent (PFBBr) or catalyst (BF(3)) and the temperature. Considering pentafluorobenzylation, the most influential factors are the concentration of PFBBr and the interaction ;temperature-time', which improve the derivatization efficiency. However, a PFBBr concentration of 250 mg l(-1) in the reaction medium cannot be exceeded because of the increase in interfering by-products in GC/ECD. Moreover, chloroacetic acid derivatives are co-eluted with these compounds. This disadvantage was not observed in the operating conditions of GC/MS. The improved pentafluorobenzylation procedure allows the direct determination of the derivatives in GC/ECD without any purification step. The average detection limits are 1.6 and 80 mug l(-1), respectively in GC/ECD and in GC/MS. The reproducibility is 13%. For the BF(3)/methanol esterification, the interactions ;BF(3) concentration-temperature' and ;BF(3) concentration-reaction time' are significant and have a negative effect on the derivatization yield. A linear model was therefore proposed and validated in the experimental area under study. All the compounds studied were detected in GC/MS, and the average detection limit is 2 mug l(-1). The reproducibility is around 7%. Therefore, after optimization, BF(3)/methanol esterification followed by GC/MS is as sensitive as pentafluorobenzylation used with GC/ECD, and more reproducible.     

Analysis of linear alkylbenzenesulfonates in water samples by large-volume injection-port derivatization and gas chromatography-mass spectrometry.

This work presents a modified method to analyze linear alkylbenzenesulfonates (LASs) in water samples. The method involves extraction of samples by a graphitized carbon black (GCB) cartridge, and direct derivatization in the GC injection port using a large-volume (10-20 microl) direct sample introduction (DSI) device with tetraalkylammonium (TAA) salts. The analytes were then identified and quantitated by ion-trap GC-MS. The large-volume DSI injection-port derivatization technique provides sensitivity, fast and reproducible results for LAS residues, to quantitation at 0.1 microg/l in 200 ml of water samples. The retention effect of TAA salts in the injection port was not detected. Enhanced selected mass chromatograms of [M-55]+ ions of butylated C10-C13 LASs by electron impact ionization MS allows one to determine LAS residues at trace levels in environmental samples. Recovery of total LASs in spiked variety water samples ranged from 89 to 112% while RSDs ranged from 2 to 13%.     

基于考古情境的化学综合实践活动设计——“考古”陶片中残留油脂的检测

针对实际考古问题进行分析,提炼实践活动主题,围绕"考古陶片中残留油脂的分析检测"这一主题设计化学综合实践活动。通过陶片中残留油脂的分析检测,引导学生了解化学技术手段在考古中的跨学科应用。学生通过实验操作提取"考古"陶片中的脂肪酸残留,并将其交换为脂肪酸甲酯,通过气相色谱进行表征,最后结合陶片及其考古背景分析陶片的使用情况。该实验可向化学、生物化学、人类学以及考古等专业学生开放,可帮助学生了解并掌握样品分离和制备、衍生化、气相色谱和多组分样品分析等方面的基本概念和实践操作。     

Sample preparation and gas chromatography of primary fatty acid amides

A method for the isolation of bio-active primary fatty acid amides (PFAM's) from total lipid extract by solid-phase extraction (SPE) was developed and validated. The lowest mass of amide to be loaded and recovered by this method was detected as 0.5 microg using 500 mg of normal phase adsorbent. The isolated PFAM's were separated and quantified by GC/MS and percent recoveries were calculated. An HP-5MS column was able to provide base line separation between the saturated and unsaturated PFAM's whereas clear resolution between geometric and positional isomers having the same number of carbons was obtained using a BPX70 column. The separated amides were all 18 carbon analogs of cis-9-octadecenoamide (oleamide). Detection limits in the single ion monitoring mode were found to be on the order of 10 pg in a 1 microl injection. Solid phase extraction of amides from total lipid extract before GC/MS analysis provides clean detection and interference free analysis.     

Application of Single Drop Extraction (SDE) Gas Chromatography Method for the Determination of Carbonyl Compounds in Spirits and Vodkas

Abstract

The application of single drop extraction (SDE) for isolation and enrichment of carbonyl compounds after derivatization with O‐(2,3,4,5,6‐pentafluorobenzyl)hydroxylamine in spirits and vodkas is discussed. The optimal parameters (extraction volume, drop volume, content of ethyl alcohol, sample volume, temperature and time of extraction) for isolation and preconcentration of C₁–C₆ aldehydes from alcoholic matrices were established. The developed SDE‐gas chromatography (GC)‐electron capture detection (ECD), an extraction method, allows the determination of low molecular aldehydes at level lower than 1 µg dm^?3. The overall analysis time without derivatization is 35 minutes. The procedure was applied for the determination of aldehydes in real alcoholic beverages (vodkas). The simplicity and cost‐effectiveness of the proposed procedure makes it a good alternative to solid phase microextraction (SPME) and other more labor‐intensive methods.     

Ultrasound‐assisted emulsification microextraction combined with injection‐port derivatization for the determination of some chlorophenoxyacetic acids in water samples

An efficient method based on ultrasound‐assisted emulsification microextraction followed by injection‐port derivatization GC analysis was developed to determine 2,4‐dichlorophenoxyacetic acid (2,4‐D) and 4‐chloro‐2‐methylphenoxyacetic acid (MCPA) in natural water samples. In this procedure, 12.5 μL of 1‐undecanol was injected slowly into a 12 mL home‐designed centrifuge glass vial containing an aqueous sample of the analytes located inside an ultrasonic water bath. The resulting emulsion was centrifuged, and 1 μL of the separated organic solvent together with 1 μL of the derivatization reagent were injected into a GC equipped with a flame ionization detector. Several factors that influence the derivatization and extraction were optimized. Under the optimal conditions, the LODs were 0.33 and 1.7 μg/L for MCPA and 2,4‐D, respectively. Preconcentration factors of 670 and 836 were obtained for MCPA and 2,4‐D, respectively. The precision of the proposed method was evaluated in terms of repeatability, which was <5.7% (n = 5). The applicability of the proposed method was evaluated by extraction and determination of chlorophenoxyacetic acids from some natural waters, which indicated that the matrices of natural waters have no significant effect on the extraction and derivatization efficiency of this method.     

High-performance gas chromatography of 1,4-naphthoquinones fromDroseraceae

Summary The analysis of natural 1,4-naphthoquinones from different species ofDroseraceae was performed by means of a direct GC method without derivatization. A simple and rapid extraction by toluene was used which did not need further purification. The sensitivity of the method allowed naphthoquinone estimation in one organ (leaf or root) only.The identity of plumbagin and 7-methyljuglone was confirmed by mass spectrometry.     

Alkyl methylphosphonic acids,the degradation products of organophosphorous CWA — preparation and direct quantitative GC-FID analysis

Seven alkyl methylphosphonic acids, products of hydrolytic degradation of organophosphorus chemical warfare agents, were obtained with a high purity (mostly above 98%), with the aim of being applyed as future certified reference materials. Ethyl (EMPA), isopropyl (IMPA), pinacolyl (PMPA), butyl (BUMPA), isobutyl (IBUMPA), cyclohexyl (CHMPA) and 2-ethylhexyl (EHMPA) monoesters of MPA were synthesized and characterized by MS EI, FTIR and NMR (¹H, ¹³C, ³¹P), TLC, as well as GC and GC-MS after derivatization. The conditions for a direct quantitative GC FID analysis on CP-FFAP CB column of non-derivatized alkyl methylphosphonic acids were developed. This is the first successful attempt of a directed GC analysis of free alkyl phosphonic acids. Their chemical purity was determined and limit of quantification (LOQ) values for some of them were evaluated for the GC-FID method.     

GC–MS Measurement of 13C-Enrichment of Lactic Acid in Sepsis Plasma

Sepsis is a systemic inflammatory response syndrome arising from infection. The plasma lactic acid level is a reliable marker of sepsis. A novel procedure based on microwave-assisted derivatization followed by gas chromatography–mass spectrometry (GC–MS) has been developed for the rapid measurement of ¹³C-isotope enrichment of lactic acid in plasma. The derivatization conditions and method validation were studied. The method was applied to the measurements of isotopic enrichment of lactic acid in the plasma of a rabbits which had received the tracer ([1,2,3-¹³C₃] lactic acid) by carotid infusion 2.5 h before blood sampling from the portal vein. These results show that the proposed method has excellent precision (RSD less than 4.57%), linearity (slope = 0.9936; r ² = 0.9998), accuracy and selectivity. The analytical results show that microwave-assisted derivatization coupled to GC–MS is a rapid method for the direct isotopic measurement of deproteinised plasma. The method could be of great interest for metabolic studies in animal models and human patients.     

GC–MS analysis of organic acids in rat urine: A protocol of direct ultrasound-assisted derivatization

The aim of the present study was to develop a novel ultrasound-assisted derivatization method for analysis of urine that can be used for preliminary screening and monitoring of metabolic disorders. Here we describe an ultrasound-assisted derivatization method followed by GC–MS analysis to quantify 26 organic acids in urine. The optimum levels of the variables affecting the yield of derivatization were investigated, including urease doses, derivatization reagents and derivatization conditions (duration time, reaction temperature and sonic power). The method exhibited the best results with 80 μl urease. The optimal reaction conditions were 100 μl BSTFA, 80% ultrasound power, 70°C and 40 min. This method showed satisfactory linearity, good reproducibility and an acceptable limit of detection and accuracy. Therefore, it could potentially be used to as a standard method to enable comparisons between laboratories. Finally, we applied our method to urine samples from pregnant rats administered 2 or 10 mg/kg folic acid supplementation.     

Stereochemical analysis of 3,4-methylenedioxymethamphetamine and its main metabolites by gas chromatography/mass spectrometry

3,4-Methylenedioxymethamphetamine (MDMA, ecstasy) is consumed as the racemate but some metabolic steps are enantioselective. In addition, chiral properties are preserved during MDMA biotransformation. A quantitative analytical methodology using gas chromatography/mass spectrometry (GC/MS) to determine enantioselective disposition in the body of MDMA and its main metabolites including 3,4-methylenedioxyamphetamine (MDA), 4-hydroxy-3-methoxymethamphetamine (HMMA), and 4-hydroxy-3-methoxyamphetamine (HMA) was developed. Plasma and urine samples were collected from a male volunteer. The analysis of MDMA, MDA, and 4-hydroxy-3-methoxy metabolites by GC/MS required a two-step derivatization procedure. The first step consisted of derivatization of the amine with enantiomerically pure Mosher's reagent ((R)-MTPCl). Triethylamine was used as a base to neutralize hydrochloric acid formed during the reaction allowing quantitative derivatization, which resulted in a substantial improvement in the sensitivity of the method compared with other previously described techniques. Further treatment with ammonium hydroxide was required since both amine and hydroxyl groups underwent derivatization in the reaction. Ammonium hydroxide breaks bonds formed with hydroxyl groups without affecting amine derivatives. The second derivatization step using hexamethyldisilazane was needed for metabolites containing phenol residues. This derivatization method permitted the stereochemically specific study of MDMA and its main monohydroxylated metabolites by GC/MS. A detailed study of the chemical reactions involved in the derivatization steps was indispensable to develop a straightforward, sensitive, and reproducible method for the analysis of the parent drug compound and its metabolites.     

The use of trimethylsilyl cyanide derivatization for robust and broad-spectrum high-throughput gas chromatography–mass spectrometry based metabolomics

Reproducible and quantitative gas chromatography–mass spectrometry (GC-MS)-based metabolomics analysis of complex biological mixtures requires robust and broad-spectrum derivatization. We have evaluated derivatization of complex metabolite mixtures using trimethylsilyl cyanide (TMSCN) and the most commonly used silylation reagent N-methyl-N-(trimethylsilyl)trifluoroacetamide (MSTFA). For the comparative analysis, two metabolite mixtures, a standard complex mixture of 35 metabolites covering a range of amino acids, carbohydrates, small organic acids, phenolic acids, flavonoids and triterpenoids, and a phenolic extract of blueberry fruits were used. Four different derivatization methods, (1) direct silylation using TMSCN, (2) methoximation followed by TMSCN (M-TMSCN), (3) direct silylation using MSTFA, and (4) methoximation followed by MSTFA (M-MSTFA) were compared in terms of method sensitivity, repeatability, and derivatization reaction time. The derivatization methods were observed at 13 different derivatization times, 5 min to 60 h, for both metabolite mixtures. Fully automated sample derivatization and injection enabled excellent repeatability and precise method comparisons. At the optimal silylation times, peak intensities of 34 out of 35 metabolites of the standard mixture were up to five times higher using M-TMSCN compared with M-MSTFA. For direct silylation of the complex standard mixture, the TMSCN method was up to 54 times more sensitive than MSTFA. Similarly, all the metabolites detected from the blueberry extract showed up to 8.8 times higher intensities when derivatized using TMSCN than with MSTFA. Moreover, TMSCN-based silylation showed fewer artifact peaks, robust profiles, and higher reaction speed as compared with MSTFA. A method repeatability test revealed the following robustness of the four methods: TMSCN?>?M-TMSCN?>?M-MSTFA?>?MSTFA.

Capillary gas chromatography combined with high performance liquid chromatography for the structural analysis of olive oil triacylglycerols

The triacylglycerol composition of olive oil samples has been determined by stereospecific analysis after partial hydrolysis with ethyl magnesium bromide, derivatization, preparative chiral HPLC, transesterification, and GC quantitation of fatty acid methyl esters. The data obtained for position sn-2 were compared with those from capillary GC analysis of monoacyl sn-2-glycerols after enzymatic lipolysis of triacylglycerols. The determination of triacylglycerols collected by silver ion HPLC and quantified (as fatty acid methyl esters) by GC, together with direct GC analysis on a polar column, have then furnished a comprehensive picture of the triacylglycerol content of olive oil.     

Gas Chromatographic Method for Analysis of p-Synephrine in Citrus aurantium L. Products

A method has been developed and validated for the identification and quantification of p-synephrine in Citrus aurantium L. products. The approach comprises GC-FID analysis followed by GC-MS confirmation after clean-up by solid phase extraction with a strong cation-exchange phase and derivatization with cyclohexanone. Oxazolidine derivative of p-synephrine was subjected to analysis by nuclear magnetic resonance (¹H and ¹³C NMR), GC-FID and GC-MS. The GC method was validated and was found to be linear in the range of 125–500 mg%. Intra-day and inter-day precisions were 3.60 and 3.59%, respectively. Mean recovery from extract of C. aurantium was 78.1 ± 3.64%. The selectivity of the method was further improved by confirmation of oxazolidine derivative of p-synephrine by GC-MS.     

Effect of background derivatization on the signal enhancement of pesticide residues extracted from edible oils

The effect of background derivatization on the signal enhancement of pesticide residues extracted from edible oil samples was studied by GC with negative chemical ionization MS. The analytes were extracted by a solvent extraction process, and the extract was subjected to rapid low‐temperature fat precipitation. The residual fatty acids were silylated by derivatization with N,O‐bis(trimethylsilyl)trifluoroacetamide. The chromatograms obtained from the derivatized samples showed higher signal intensity and lower detection levels when compared to the direct analysis without derivatization. The sensitivity levels of the method are either better or comparable to that of previously reported methodologies. The LODs of the analyzed organochlorine, organophosphorus, and synthetic pyrethroid residues in sunflower, rice bran, and ground oil samples were in the range of 0.02–0.5 ng/g, and the LOQs were in the range of 0.1–2 ng/g. The intraday and interday accuracies were in the range of 81–116% with RSDs less than 14%. The recoveries obtained were in the range of 53–89% with the RSD values less than 13% for all the studied pesticide residues.     

Validation of a novel derivatization method for GC–ECD determination of acrylamide in food

This paper proposes a new method for quantitative analysis of acrylamide in cereal-based foods and potato chips. The method uses reaction with trifluoroacetic anhydride, and analyses the resulting derivative by use of gas chromatography with electron-capture detection (GC–ECD). The effects of derivatization conditions, including temperature, reaction time, and catalyst, on the acylation reaction were evaluated. Chromatographic analysis was performed on an SE-54 capillary column. Under the optimum conditions, good retention and peak response were achieved for the acrylamide derivative. The analytical method was fully validated by assessment of LODs and LOQs (1 ng g^?1 and 25 ng g^?1, with relative standard deviations (RSD) 2.1 and 3.6, respectively), linearity (R?=?0.9935 over the range 0.03–10 μg g^?1), and extraction recovery (>96 %, with RSD below 2.0, for acrylamide spiked at 1, 20, 50, and 100 ng g^?1; 99.8 % for acrylamide content >1000 ng g^?1). The method requires no clean-up of the acrylamide derivative before injection. The method has been successfully used to determine acrylamide levels in different commercial cereal-based foods, French fries, and potato chips.