气相色谱-质谱联用法分析全氟酰氟

采用气相色谱-质谱联用技术(GC/MS)对电化学氟化法生产的全氟环己烷酰氟产品中主要产物全氟酰氟进行了检测。在60℃下,采用甲醇对全氟环己烷酰氟产品进行甲酯化处理。考察了不同长度,极性及膜厚的毛细管色谱柱的分离效果。以KB-1MS毛细管色谱柱(90 m×0.25 mm×1.0μm)为分离柱,采用GC/MS法对全氟酰氟组成进行了定性与定量分析;结合有机质谱学裂解规律,分别对环状全氟羧酸甲酯、饱和直链全氟羧酸甲酯和单不饱和脂肪酸甲酯的裂解方式和质谱特征进行了分析归纳。通过质谱数据库检索、标准品对照及已知全氟化合物的质谱信息分析,共鉴定出5种全氟酰氟,其中包括两种异构体;测得全氟环己烷酰氟约占总全氟酰氟含量的65%。     

GC,GC/MS法定性定量分析鱼油中的脂肪酸

本文介绍了一种用色谱-质谱联用仪(GC/MS),气相色谱仪(GC),定性、定量地分析测定鱼油脂中各种主要脂肪酸百分含量的方法。此法的分析过程比较直观和简单。样品在分析之前需要进行甲酯化衍生制备。鱼油脂中从11碳到22碳范围内的20几种主要脂肪酸均可准确地定性并获得定量结果。     

液相色谱/质谱大气压化学电离源鉴定深海鱼油中长链不饱和脂肪酸

以1,2-苯并-3,4-二氢咔唑-9-乙基苯磺酸酯为衍生化试剂,在充氮的气氛下对鱼油进行皂化处理,所得皂化产物经正己烷萃取处理后进行柱前衍生化,再以HPLC/MS分离和鉴定。通过对长链脂肪酸分子的标记处理,其衍生物分子在质谱分析中呈现出双键位置的规范信息。通过建立模型计算式,借助不饱和脂肪酸的分子离子峰和特征碎片离子峰的质量数,计算不饱和的碳碳双键位置。共鉴定出23种脂肪酸。结果表明深海鱼油主要由C12-C22的脂肪酸组成,多不饱和脂肪酸含量占67.08%(峰面积百分比,下同),其中C16∶19-十六碳烯酸(11.7%);C16∶44,7,10,13-十六碳四烯酸(2.91%);C18∶112-十八碳烯酸(11.1%);C18∶46,9,12,15-十八碳四烯酸(3.62%);C20∶113-二十碳烯酸(1.21%);C20∶55,8,11,14,17-二十碳五烯酸(16.71%);C22∶62,5,8,11,14,17-二十二碳六烯酸(10.53%)。所建立的方法为不饱和脂肪酸碳链中双键位置的确定提供了新的技术手段。     

2-氨基-2-甲基丙醇衍生气相色谱/质谱分析深海鱼油脂肪酸

以2-氨基-2-甲基丙醇为衍生化试剂,皂化和衍生化充氮气保护,柱前衍生气相色谱／EI质谱分析深海鱼油脂肪酸。通过修改官能团抑制了脂肪链中碳碳双键的移位,并使质谱呈现显示双键位置的规范信息。解析隐藏羧基的脂肪酸衍生物2-烯基-4,4-二甲基噁唑的质谱图,确定了深海鱼油多不饱和脂肪酸中双键的位置。共鉴定出23种脂肪酸。结果表明：深海鱼油由C12～C22脂肪酸组成,多不饱和脂肪酸含量占56．82％(峰面积百分比,下同),其中以9,12,15-十八碳三烯酸(6．96%),9,12-十八碳二烯酸(7．15％),5,8,11,14,17-二十碳五烯酸(20．83％),5,8,11,14-二十碳四烯酸(2．15％),4,7,10,13,16,19-二十二碳六烯酸(12．7％)和4,7,10,13,16-二十二碳五烯酸(2．59％)为主。为多不饱和脂肪酸中双键的定位提供了新的技术手段。     

小茴香超临界CO_2萃取产物脂肪酸成分分析

通过脂肪酸的衍生化处理，再利用色谱（GC）和色谱一质谱（GC－MS）等分析手段，对小茴香超临界CO2萃取产物的脂肪酸成分进行了剖析，共鉴定出九种脂肪酸，其中，十八碳一烯酸、十八碳二烯酸和棕榈酸是其主要成分，分别占脂肪酸总量的75．12％、15．18％和5．34％．     

脂肪酸的色谱保留时间规律与质谱特征研究及其在食品分析中的应用

用石油醚提取食品中的脂肪,经甲酯化反应后,采用HP-88(100m×0.25mm,0.33μm)弹性石英毛细管柱分离脂肪酸甲酯的同系物及异构体,GC/MS法测定。研究了不同链长脂肪酸的同系物及异构体的气相色谱出峰顺序,得到其保留时间规律;研究了不同脂肪酸的质谱断裂规律,选择3个特征离子来鉴定脂肪酸成分。建立了3个特征离子确定脂肪酸碳数及双键数目,色谱保留时间规律确定脂肪酸顺反异构体及双键位置异构体的方法。本法无需标准品即可快速测定脂肪酸同系物及异构体的含量,适用于脂肪酸组成的研究;及油脂、食品中脂肪酸,特别是反式脂肪酸的测定。     

超临界萃取蝼蛄脂肪酸成分及其气相色谱-质谱分析

采用超临界CO2萃取蝼蛄总脂肪酸,对影响萃取效果的各个因素应用正交设计试验,优化了各萃取参数.各个因素的影响顺序为压力＞温度＞时间＞流量.萃取的优化条件为压力35 MPa,温度50℃,时间1 h,流量45 kg/h.运用该萃取条件改善了萃取物的物理性状,脂肪酸的纯度提高,总脂肪酸的含量可达83.29%;而采用常规的有机溶剂提取法,脂肪酸的纯度仅为60%左右.甲酯化采用气相色谱-质谱分析技术对其中的16个成分进行了鉴定,并测定了相对含量,其中主要有油酸甲酯(30.40%)、十六烷酸甲酯(14.19%)、9,12-十八碳二烯酸甲酯(11.99%)、油酸乙酯(11.75%)、9-十六碳烯酸甲酯(7.77%)、十六烷酸乙酯(5.97%)、9,12-十八碳二烯酸乙酯(4.53%)及9-十六碳烯酸乙酯(2.87%)等.     

高效液相色谱法分离纯化微生物油脂中的花生四烯酸

为满足花生四烯酸样品制备的需要,将微生物油脂中制得的脂肪酸先经尿素包合(脲包法)和甲酯化后,再利用反相高效液相色谱法分离纯化其中的花生四烯酸。在C18反相柱上,以甲醇-水(体积比为95∶5)为流动相,采用示差折光检测器检测,流速为5 mL/min时,目标产物的分离度较佳。用气相色谱/质谱法(GC/MS)进行分析的结果表明,花生四烯酸甲酯在纯化后的样品中的质量分数由38%提高到99%以上,基本达到标准物质的质量要求。     

质谱特征结合等效链长定性分析植物油中的脂肪酸

建立了质谱特征结合等效链长快速定性植物油中脂肪酸的方法。首先根据质谱特征判断脂肪酸的类型并鉴定出其中的饱和脂肪酸甲酯,然后利用它们的保留时间信息计算得到不饱和脂肪酸甲酯的等效链长值,与已建立的脂肪酸甲酯数据库对照实现不饱和脂肪酸甲酯的结构鉴定。用NaOH-甲醇对5种常见植物油(花生调和油、茶籽调和油、菜籽油、葵花籽油、大豆油)中的脂肪酸进行衍生和提取,采用DB-23石英毛细管柱(30m×0.25mm×0.25μm)分离脂肪酸甲酯的同系物和异构体,气相色谱质谱法(GC/MS)测定,结果表明,5种样品油中所含不饱和脂肪酸的组成和含量上均存在明显差异。本方法无需标准品即可快速定性检测脂肪酸同系物及异构体,适用于油脂、食品中脂肪酸的成分分析。     

油松籽油脂的提取及其脂肪酸组成与含量的评价

采用索氏提取法提取油松籽中的油脂,得油率为42.9%;对油脂进行甲酯化处理后用气相色谱-质谱联用仪检测其中的脂肪酸组成及含量。实验结果表明,油松籽油中含有7种脂肪酸,分别为肉豆蔻酸10.38%、硬脂酸3.05%、油酸21.98%、亚油酸(13,16-十八碳二烯酸)3.53%、亚油酸(9,12-十八碳二烯酸)38.38%、亚麻酸20.06%和二十碳三烯酸2.62%,其中饱和脂肪酸含量为13%,不饱和脂肪酸含量为87%。     

Analysis of Polyunsaturated Fatty Acids Using High Performance Liquid Chromatography – Atmospheric Pressure Chemical Ionization Mass Spectrometry

Analysis of polyunsaturated fatty acids using high performance liquid chromatography–atmospheric pressure chemical ionization mass spectrometry is described. The standard fatty acid methyl esters from 16 to 22 carbons were analyzed by LC‐MS with APCI. The effect of orifice voltage and total carbon atoms versus number of double bonds in each homologue on the mass spectra is discussed. The correction coefficients for homologues from saturated fatty acids to hexaenoic acid are also mentioned.     

气相色谱质谱法测定植物油中脂肪酸

建立了气相色谱质谱法测定食用植物性油中脂肪酸检测的方法。植物油中的脂肪酸甘油酯在碱性条件下被水解为游离脂肪酸,随后采用三氟化硼将其转化为脂肪酸甲酯。采用同位素标记脂肪酸进行加标回收试验,回收率在94%以上。通过质谱的选择离子检测模式对硬脂酸、油酸、亚油酸等10种目标脂肪酸进行了检测,结果显示,该方法可用于油品的质量检测和日常分析。     

Determination of lipids in infant formula powder by direct extraction methylation of lipids and fatty acid methyl esters (FAME) analysis by gas chromatography.

Fatty acid methyl esters (FAMEs) of pure triglyceride standards, oils, and fat from dry matrixes were formed by transesterification using sodium methoxide in methanol-hexane. FAMEs were produced by direct addition of sodium methoxide-hexane to samples and heating to simultaneously extract and transesterify acyl lipids. FAMEs were quantitated by capillary gas chromatography (GC) over a fatty acid concentration range of 0 to 1.7 mg/mL (r > or = 0.9997). Total fat was calculated as the sum of individual fatty acids expressed as triglyceride equivalents, in accordance with nutrition labeling guidelines. Saturated, polyunsaturated, and monounsaturated fats were calculated as sums of individual free fatty acids. Absolute recoveries determined from individual fatty acids in test samples ranged from 69.7 to 106%. Recoveries (relative to the C13:0 internal standard) for individual fatty acids in test samples ranged from 95 to 106%. Reproducibility was constant at each fatty acid level in the reaction mixture (n = 5, coefficient of variation [CV] < 2%). Absolute recovery determined from the sum of total fatty acids in standard reference material (SRM) 1846 (powdered infant formula) was 96.4%. Analysis of SRM 1846 gave results that agreed closely with the certified fat and fatty acid values. Analysis of commercial infant formula gave results that were comparable to those obtained with AOAC Method 996.01. The direct extraction methylation procedure is rapid, and the transesterification of acyl lipids to form FAMEs is complete within 15 min. Classical saponification and refluxing are not required. This method provides FAMEs free of interferences and easily quantitated by GC or confirmed by GC/mass spectrometry (MS). Unambiguous MS identification of individual FAMEs derived from pure standards, SRM 1846, and powdered infant formula product was obtained.     

Characterization and purification of polyunsaturated fatty acids from microalgae by gas chromatography-mass spectrometry and countercurrent chromatography

Summary The present study was undertaken in order to characterize then to purify fatty acids from marine phytoplankton. From a crude mixture of fatty acid methyl esters it was possible to isolate by countercurrent chromatography a mixture of four polyunsaturated fatty acid methyl ester identified as being hexadecatrienoic acid methyl ester, octadecatetraenoic acid methyl ester, eicosapentaenoic acid methyl ester and docosahexaenoic acid methyl ester by gas chromatography coupled with mass spectrometry in electron impact and in positive-ion chemical ionization mode. The four polyunsaturated fatty acids are in different ratios in mixtures from the two microorganisms:Skeletonema costatum andIsochrysis galbana.     

Identification of chlorinated fatty acids in fish by gas chromatography/mass spectrometry with negative ion chemical ionization of pentafluorobenzyl esters

This paper reports the development of a technique for identifying and confirming chlorinated fatty acids previously detected in fish by gas chromatography (GC) with halogen-specific detection (XSD). Fatty acid methyl esters (FAMEs) including chlorinated FAMEs within fractions of reversed-phase high-performance liquid chromatography of transesterified fish extracts were derivatized to pentafluorobenzyl esters, which were subjected to GC/mass spectrometry (MS) with negative ion chemical ionization (NICI). Pentafluorobenzyl esters displayed reasonably good GC characteristics, a very high ionization efficiency and a low degree of fragmentation. Chloride ion chromatograms extracted at m/z 35 and 37 from full scans were utilized for locating traces of chlorinated unknowns in the GC elution profile so that their mass spectra could be readily displayed. Significant ions displayed in the mass spectrum scanned in a narrow range of retention time where a chlorinated unknown was located were evaluated using ion chromatograms extracted at the m/z of these ions. The chromatographic peaks of those ions derived from the analyte were expected to center at that specific retention time, whereas those originating from matrix compounds were not. The isotopic patterns of chlorinated ions were also examined against their theoretical relative abundances. Using this approach, three metabolism-related dichloro fatty acids previously identified by GC/XSD in filet extracts of white sucker sampled downstream from a bleached kraft pulp mill were confirmed: dichlorooctadecanoic, dichlorohexadecanoic and dichlorotetradecanoic acids. In addition, an isomer of dichlorotetradecanoic acid was found in a reference fish sample. As sample preparation is critical in this application, improved conditions for hydrolysis and pentafluorobenzyl esterification are also discussed.     

Gas chromatographic/mass spectrometric analysis of the essential oil of Houttuynia cordata Thunb by using on-column methylation with tetramethylammonium acetate

This paper describes a simple and novel on-column derivatization procedure used with gas chromatography/mass spectrometry (GC/MS) for the analysis of essential oil of Houttuynia cordata Thunb (HCT), a traditional Chinese medicine. In the procedure, the essential oil was obtained by hydrodistillation, and the fatty acid components were derivatized with tetramethylammonium acetate (TMAA) at 250 degrees C and identified by GC/MS. Methylation improved the determination of both the fatty acids and the other components in the essential oil of HCT. To obtain optimum methylation conditions, several important factors were investigated with pentadecane as the internal standard and a GC inlet temperature of 250 degres C. Tetramethylammonium hydroxide (TMAH) and TMAA were compared as the derivatization agent, and a 2:1 ratio of TMAA to capric acid was evaluated. Fatty acid methyl esters produced good chromatographic peak shapes and did not interfere with the determination of dodecanal and caryophyllene. TMAA is a neutral methylation reagent, and it yielded no side reactions during derivatization. It was found that the fatty acid content of the essential oil was about 81%; among the methylated fatty acids found were capric acid, methyl (43.66%), methyl laurate (16.15%), methyl hexadecanoate (9.27%), undecanoic acid, methyl (5.62%), methyl oleate (1.98%), and methyl linoleate (1.40%). Other major constituents were (-)-beta-pinene (1.02%), beta-myrcene (1.62%), 1-terpinen-4-ol (1.59%), decanal (1.49%), and 2-undecanone (1.47%). The results obtained demonstrated good efficiency for the procedure. Pure chromatograms allowed quantitation, which was obtained by total volume integration. The on-column derivatization procedure was simple to perform, and it improved the sensitivity, the peak resolution, and the selectivity of the GC/MS determination.     

Identification of intact long-chain p-hydroxycinnamate esters in leaf fibers of abaca (Musa textilis) using gas chromatography/mass spectrometry

The study of acetone-extractable components from the leaf fibers of the non-wood plant abaca (Musa textilis) resulted in the isolation and identification of series of intact hydroxycinnamate esters consisting of ferulic and p-coumaric acids esterified to long-chain fatty alcohols (C20 to C28) and omega-hydroxyfatty acids (C22 to C28). These series of compounds were characterized by high-temperature gas chromatography/mass spectrometry (GC/MS) using capillary columns (12 m length) with thin films that allowed the analysis of intact (i.e., without prior saponification) hydroxycinnamate esters. Characterization of intact individual compounds was achieved based on the mass spectra obtained by GC/MS of the underivatized compounds and their methyl and/or trimethylsilyl ether derivatives.     

Creating a fatty acid methyl ester database for lipid profiling in a single drop of human blood using high resolution capillary gas chromatography and mass spectrometry

Capillary gas chromatography (CGC) in combination with mass spectrometry (MS) was optimized for the separation and detection of the fatty acids occurring in the lipid fraction of blood. A fingertip blood sample (ca. 50 microL) was transesterified into the methyl esters and analyzed on a 100 m x 0.25 mm ID column coated with a biscyanopropyl polysiloxane (HP-88) stationary phase. The method was retention time locked. Programmed temperature vaporization injection (PTV) in the solvent venting mode was applied to minimize the sample size, while maintaining high sensitivity. The total analysis time was ca. 60 min. Retention times and both electron impact (EI) and positive chemical ionization (PCI) mass spectrometry were combined to elucidate the fatty acids according to alkyl chain, degree of unsaturation and position of the double bonds. Using extracted ion chromatograms about 100 fatty acids and related compounds were detected in blood samples and most of them were identified. This work resulted in a very large fatty acid methyl esters database, containing retention time and mass spectral information that will be applied to metabolomic studies.     

Analysis of bacterial fatty acids by flow modulated comprehensive two-dimensional gas chromatography with parallel flame ionization detector/mass spectrometry

Comprehensive two-dimensional gas chromatography (GC × GC) offers an interesting tool for profiling bacterial fatty acids. Flow modulated GC × GC using a commercially available system was evaluated, different parameters such as column flows and modulation time were optimized. The method was tested on bacterial fatty acid methyl esters (BAMEs) from Stenotrophomonas maltophilia LMG 958^T by using parallel flame ionization detector (FID)/mass spectrometry (MS). The results are compared to data obtained using a thermal modulated GC × GC system. The data show that flow modulated GC × GC-FID/MS method can be applied in a routine environment and offers interesting perspectives for chemotaxonomy of bacteria.