Fatty acids not only form phospholipids that contribute to the formation of cell membranes but also participate in many metabolic activities, such as energy storage and cell signal transduction. The liver plays a key role in the synthesis and metabolism of fatty acids. The composition and contents of fatty acids in the liver are closely related to body health. Most fatty acid-detection methods require a large sample size and can detect only a small number of fatty acids. Therefore, a sensitive and efficient method to determine fatty acids in the liver is urgently required. Herein, a method based on gas chromatography-mass spectrometry (GC-MS) was established for the simultaneous determination of 39 fatty acids in 1.1 mg of liver tissue. Different extraction methods and derivatization conditions were compared to develop an optimal sample-treatment method. The performance of two different columns in separating the target fatty acids were also compared. A total of 10 mg of liver was added to 450 μL of normal saline and ground at -35 ℃ to obtain a homogenate. Next, 50 μL of the homogenate (equivalent to 1.1 mg of liver) was added with 750 μL of chloroform-methanol (1∶2, v/v) to extract total fatty acids. The fatty acid extracts were dried under nitrogen, and then derivatized at 100 ℃ for 90 min after being added with methanol containing 5% sulfuric acid. The fatty acid methyl esters were extracted with hexane and then separated on an SP-2560 capillary column (100 m×0.25 mm×0.2 μm; Supelco, USA) via GC-MS. The results revealed that all 39 fatty acid methyl esters detected had good linearities in the certain mass concentration ranges with correlation coefficients (R2) greater than 0.9940. The limits of detection (LOD) and quantification (LOQ) of these methyl esters in the liver were 2-272 ng/mg and 7-906 ng/mg, respectively. The accuracy and precision of the method were evaluated by spiking the liver homogenate with tridecylic acid and eicosanoic acid at low (0.09 μg/mg), moderate (0.90 μg/mg), and high (5.40 μg/mg) concentration levels. The recoveries ranged from 82.4% to 101.0% with an intraday relative standard deviations (RSDs) (n=5) of 3.2%-12.0% and interday RSDs (n=3) of 5.4%-13.4%. The method was successfully applied to detect fatty acids in the livers of four healthy male Sprague-Dawley (SD) rats and four male SD rats with abnormal liver function induced by perfluorooctane sulfonate (PFOS). PFOS is a persistent organic pollutant. Twenty-six fatty acids were detected in the livers of both groups. Among the fatty acids investigated, pentadecanoic acid (C15∶0), γ-linolenic acid (C18∶3n6), and elaidic acid (C18∶1n9t) cannot be detected by the methods reported in the literature. By contrast, the method developed in this study could separate the isomers of oleic acid (elaidic acid, C18∶1n9t; oleic acid, C18∶1n9c) and linolenic acid (linolelaidic acid, C18∶2n6t; linoleic acid, C18∶2n6c). In conclusion, the developed method is simple and can detect a large number of fatty acids using small sample amounts and few reagents. More importantly, it could successfully separate fatty acid isomers. These findings indicate that the developed method is suitable for the detection of fatty acid composition and contents in the liver in clinical and experimental research.
肝脏是脂肪酸代谢的主要场所,研究肝脏中脂肪酸组成和含量的变化可以监测机体的健康状态。现有的检测方法存在样本消耗量大、检测出的脂肪酸种类少等缺点。通过比较不同提取方法和衍生化条件,建立了仅用1.1 mg肝脏组织即可测定39种脂肪酸含量的气相色谱-质谱方法。肝脏组织经研磨匀浆,以氯仿-甲醇(1∶2, v/v)提取总脂肪酸后,氮气吹干,加入含5%硫酸的甲醇溶液,100 ℃反应90 min使脂肪酸甲酯化,经SP-2560色谱柱分离后进质谱仪分析。结果表明,39种脂肪酸甲酯在各自的浓度范围内线性关系良好,相关系数(R2)大于0.9940。将各脂肪酸甲酯的检出限(LOD)和定量限(LOQ)换算至肝脏中的含量,分别为2~272 ng/mg和7~906 ng/mg。以十三烷酸和二十三烷酸考察方法的加标回收率及精密度,在3个水平下的回收率为82.4%~101.0%,日内相对标准偏差(n=5)为3.2%~12.0%,日间相对标准偏差(n=3)为5.4%~13.4%。动物暴露于经典的持久性有机污染物全氟辛烷磺酸(PFOS)后,体内脂肪酸的代谢可能会出现异常。将该方法应用于健康和经口暴露PFOS的雄性SD大鼠肝脏中脂肪酸含量的检测,从两组大鼠中均检出了26种脂肪酸,其中C15∶0、C18∶3n6和C18∶1n9t为其他方法未检出的脂肪酸,C18∶1n9t和C18∶1n9c为其他方法未能分离的顺反式同分异构体脂肪酸。该方法操作简便,试剂及样品用量少,灵敏度高,能检测出种类更多的脂肪酸,并能有效分离顺反式同分异构体脂肪酸C18∶1n9t、C18∶1n9c和C18∶2n6t、C18∶2n6c,适用于临床诊断和动物研究中肝脏脂肪酸的组成和含量检测。
Keywords: fatty acids; gas chromatography-mass spectrometry (GC-MS); liver.