阴离子交换色谱-积分脉冲安培法测定鱼粉和玉米粉水解液中氨基酸

将高效阴离子交换色谱．积分脉冲安培直接检测法应用于鱼粉和玉米粉水解液中的氨基酸的分析测定。该方法使用Dionex AminoPac PA10阴离子交换柱为分析柱，控制柱温为35℃，以NaOH和NaAc的强碱性溶液为淋洗液，在合适的梯度条件下，可以实现对17种常见氨基酸的高效分离。在强碱性条件下，获得良好分离的各个氨基酸可在配有金工作电极的电化学检测器上以积分脉冲安培法获得高灵敏度的检测。在优化的测定条件下，该方法对这17种氨基酸的检出限在0．21—3．38pmol之间；峰面积校正曲线的线性范围为2—3个数量级；5次平行测定的峰面积的相对标准偏差RSD在0．32％—4．7％之间。该方法应用于玉米粉和鱼粉水解液中氨基酸含量的测定，结果良好。对玉米粉和鱼粉水解液标准加入的回收率分别在81．9％—108．0％和90．0％～108．0％之间。     

阴离子交换色谱-积分脉冲安培检测法测定寿胎丸中游离氨基酸

建立了阴离子交换色谱-积分脉冲安培检测法测定寿胎丸煎煮液中游离氨基酸的分析方法。实验考察了18种氨基酸的梯度洗脱条件,优化了固相萃取条件,最终选用SSDBX型固相萃取小柱净化煎煮液。在优化实验条件下,进行了加标回收实验,回收率在71.2%~120.9%之间,相对标准偏差为0.8%~10.4%。18种氨基酸的检测限为0.07~5.00μg/L。方法能满足寿胎丸煎煮液中氨基酸的检测要求。     

高效阴离子交换色谱积分脉冲安培检测法分析注射液中的氨基酸

建立了高效阴离子交换色谱积分脉冲安培检测器同时分离并测定注射液中18种常见氨基酸、氨基己酸和牛磺酸含量的方法. 注射液用20 mg/L的NaN3溶液稀释1000倍, 经0.22 μm尼龙膜过滤后直接进样分析. 以一定浓度的NaOH和NaAc溶液为淋洗液, 选择合适的梯度淋洗条件, 20种氨基酸在AminoPac PA10阴离子交换色谱柱上在30min内很好地分离, 并用脉冲安培检测器进行了测定. 氨基酸的检出限在0.14～3.81 pmol (25 μL进样, 峰面积定量).     

固相萃取-离子色谱-积分脉冲安培法测定人血清中游离氨基酸

比较了磺基水杨酸和无水甲醇沉淀人血清中蛋白质的效果,优化了国产732型阳离子交换树脂进行固相萃取净化的条件和Dionex-600离子色谱分析系统的梯度淋洗条件。用该离子色谱仪检测了谷氨酰胺等14种氨基酸,结果表明,峰面积-浓度的校正曲线的相关系数为0.9900~0.9995,检出限为0.02~0.59mg/L;峰面积的相对标准偏差为1.9%~10.4%;回收率为80.6%~114.8%。     

人血浆中游离氨基酸的离子色谱/积分脉冲安培法分析

采用离子色谱积分脉冲安培法,在AminoPae PA10色谱柱上,用250 mmol/L的NaOH溶液和1.00 mol/L的乙酸钠溶液为淋洗液分离血浆中的游离氨基酸,以Au为工作电极,pH-Ag/AgCl电极为参比电极,检测了血浆中的16种游离氨基酸,无需衍生,检出限为0.11～3.3μg/L,样品加标回收率在87%～117%范围内.     

阴离子交换-积分脉冲安培检测法分离测定氨基酸注射液中的氨基酸和葡萄糖

 用阴离子交换 积分脉冲安培检测法测定了氨基酸注射液中 1 7种氨基酸和葡萄糖。研究了氨基酸和葡萄糖在阴离子交换中的保留行为。采用了优化的水、NaOH和NaAc三元梯度淋洗条件。在优化的梯度淋洗条件和积分脉冲安培检测条件下 ,氨基酸和葡萄糖的检出限为 0 3pmol～ 1 0 3pmol,线性范围约为 2个数量级。样品加标回收率为 88 3 %～ 1 0 4 6 %。方法简单、灵敏、准确。     

离子排斥色谱-脉冲安培法测定电镀液中的游离CN-

建立了离子排斥色谱-脉冲安培法测定游离CN-的检测方法。方法使用IonPac ICE-AS1离子排斥柱为分析柱,以120 mmol/L HClO4为淋洗液,安培法检测（工作电极为Pt电极）。CN-的检出限为0.42μg/L（50μL进样,三倍基线噪音）;在1-1000μg/L范围内具有良好的线性（r=0.9996）。0.01 mg/L和0.1mg/LCN-分别连续进样9次,峰面积相对标准偏差（RSD）分别为4.0%和3.0%。用该方法检出了电镀液样品中大量的游离CN^-。对实际样品进行加标,其回收率在83%-117%之间。     

阴离子交换色谱-积分脉冲安培检测法测定赣南脐橙中的氨基酸

建立了阴离子交换色谱-积分脉冲安培法测定脐橙中17种氨基酸的分析方法。样品用无水乙醇提取,经聚苯乙烯-二乙烯基苯型阳离子交换树脂(PS-DVB)003x7去除碳水化合物,采用AminoPac PA10保护柱(50×2mm)和AminoPac PA10分析柱(250×2mm)分离,积分脉冲安培检测器检测。所测17种氨基酸在一定浓度范围内与峰面积呈良好的线性关系,相关系数均大于0.995,检出限为0.01~0.19mg/L。在2.0mg/L和8.0mg/L两个添加水平的平均回收率在72.5%~130.5%之间,相对标准偏差在0.5%~10.1%范围。该法具有较好的准确度和精密度,基本能满足实际样品分析的要求。     

缬氨酸产品中微量氨基酸杂质的高效阴离子交换色谱-积分脉冲安培测定

在优化实验条件下,建立了高效阴离子交换色谱-积分脉冲安培检测法分离测定缬氨酸产品中微量氨基酸杂质的方法。研究了氨基酸的阴离子交换色谱分离和积分脉冲安培检测。采用优化的水、0.25 mol/LNaOH、1.0 mol/L NaAc三元梯度淋洗条件及35℃柱温实现了19种氨基酸的分离。在最佳条件下,氨基酸的检出限(S/N=3)为3.1~67.1 nmol/L,线性范围约为3个数量级。样品加标回收率为90%~96%。方法可以推广至其它氨基酸产品中微量氨基酸杂质的测定。     

液相色谱-电喷雾电离/离子阱质谱法分析金线莲中3-吡啶甲醇

应用现代提取技术超声-微波协同萃取金线莲中的3-吡啶甲醇,采用固相萃取技术对样品进行前处理,高效液相色谱法-电喷雾电离/离子阱质谱法(HPLC-ESI/MS)对提取物中3-吡啶甲醇进行测定和鉴别.色谱条件:Agilent TC-C₁₈色谱柱(5 μm,4.6×250 mm),流动相:甲醇-0.02 mol/L乙酸铵(5∶95,V/V),流速:1 mL/min,检测波长:260 nm.结果表明峰面积与3-吡啶甲醇在浓度1~10 μg/mL范围内呈良好线性关系.回收率在92.0%~96.2%之间,相对标准偏差为2.36%.该法简便、准确、快速.     

二维阀切换离子色谱法测定海带中游离氨基酸

建立一种测定海带中游离氨基酸的阀切换高效阴离子交换色谱耦合脉冲安培检测器法。采用一根阳离子交换柱对氨基酸进行富集,而后经阀切换至氨基酸分析柱Amino Pac~PA-10(250 mm×2 mm)上分离并进入安培检测器检测。在最佳分离条件下,20种氨基酸的质量浓度在0.1~20.0 mg/L范围内与其色谱峰面积线性关系良好,线性相关系数r~20.99,20种氨基酸的检出限为0.01 mg/L,加标回收率为83.12%~117.34%,测定结果的相对标准偏为1.02%~13.05%(n=8)。该方法样品前处理简单,无基底杂质干扰,适用于海带样品中游离氨基酸的测定。     

反相高效液相色谱法测定白肋烟烟叶中的游离氨基酸

建立了一种用于烟草中游离氨基酸测定的反相高效液相色谱法．实验采用超声波水解、邻苯二甲醛／3-巯基丙酸作为衍生剂进行柱前衍生．色谱柱为依利特C18柱（4．6mmi．d．×250mm,5μm）,流动相A为18mmol／L的醋酸钠溶液（pH7．2）含体积分数为0．002％的三乙胺和0．3％的四氢呋喃,流动相B组成为：100mmol／L的醋酸钠溶液（pH7．2）-乙腈-甲醇（体积比为1：2：2）,流速为1．0mL／min,柱温为40℃．荧光检测器,激发波长350nm,发射波长450nm．方法的回收率为95．3％～100．7％,RSD为2．32％～9．24％（n=6）．该方法简便、准确、重现性好．测定了不同肥料配比生产的白肋烟烟叶中17种游离氨基酸的含量．结果表明,不论有机肥与无机肥怎样配比,天冬氨酸的含量与各氨基酸相比都是最高的;随着饼肥的加入,大部分氨基酸的含量是先增加后逐渐降低的趋势,15％饼肥＋85％无机肥与30％饼肥＋70％无机肥配比时,大部分游离氨基酸的含量接近,30％饼肥＋70％无机肥配比时的游离氨基酸总量最高,综合考虑,30％饼肥＋70％无机肥配比时的烟叶质量最好．     

Determination of Free and Total Underivatized Amino Acids Including L-Canavanine in Bitter Vetch Seeds Using Hydrophilic Interaction Liquid Chromatography

A new hydrophilic interaction liquid chromatography method coupled with diode-array detector was developed for the determination of 17 underivatized amino acids including L-canavanine in bitter vetch [Vicia ervilia (L.) Willd.] seeds. Amino acids were extracted as free as well as total extracts after acid hydrolysis, followed by chromatographic separation on a Zorbax Rx-SIL column with a mobile phase of acetonitrile/potassium phosphate buffer (12.5?mM; pH 3.0) using gradient elution and detection at 190?nm. The method is characterized by a wide linear range (0.01–200?µg/mL, r?>?0.9987), sufficient accuracy (relative error 86.3–109.1%), and suitable precision for the results (relative standard deviation <4.9% in the case of intra-day and <9.8% in the case of inter-day precision). The limits of detection and quantification for free amino acids ranged from 0.01 to 0.24?mg/g and 0.03 to 0.72?mg/g, respectively, whereas the total amino acids ranged from 0.02 to 0.47?mg/g and 0.07 to 1.43?mg/g, respectively. The mean recoveries of free and total amino acids in spiked samples exceeded 70.3% for most amino acids. The mean total content of free and total amino acids in bitter vetch seeds was 1.71 and 14.88?g/100?g seed, whereas the corresponding values for canavanine were 0.07 and 0.19?g/100?g seed, respectively.     

Rapid Determination of Free Amino Acids in Milk by Microchip Electrophoresis Coupled with Laser‐induced Fluorescence Detection

A simple and sensitive method for determination of free amino acids in milk by microchip electrophoresis (MCE) coupled with laser‐induced fluorescence (LIF) detection was developed. Seven kinds of standard amino acids were derivated with sulfoindocyanine succinimidyl ester (Cy5) and then perfectly measured by MCE‐LIF within 150 s. The parameters of MCE separation were carefully investigated to obtain the optimal conditions: 100 mmol·L^?1 sodium borate solution (pH 10.0) as running buffer solution, 0.8 kV as injection voltage, 2.2 kV as separation voltage etc. The linear range of the detection of amino acids was from 0.01 µmol·L^?1 to 1.0 µmol·L^?1 and the detection limit was as low as about 1.0 nmol·L^?1. This MCE‐LIF method was applied to the measurements of free amino acids in actual milk samples and satisfactory experimental results were achieved.     

Analysis of Free Amino Acids and Protein Contents of Mature Human Milk from Turkish Mothers

Abstract

This study was designed to evaluate free amino acid (FAA) composition and total protein in mature human milk from Turkish mothers. Free amino acid concentrations in mature human milk were determined in all subjects using a high‐performance liquid chromatography (HPLC) with postcolumn derivatization system, with a fluorescence detector. Total protein content was determined by the classical biuret method. Total protein concentration was found to be 1.3±0.4 mg/dl. Glutamic asid plus glutamine is the most abundant amino acid (1275 µmol/L), followed by taurine (353 µmol/L) and alanine (261 µmol/L). Glutamic acid plus glutamine accounts for the most free amino acids in mature human milk and their sum represents 40% of total FAA. On the other hand, some amino acid derivatives such as citrulline, ethanolamine, ammonium, ornithine, ortophosphoserine, and phosphoethanolamine, not usually a part of protein, are determined and this fraction represented ～21% of the total FAA in mature human milk in the present study.     

高效液相色谱法测定羊水中兴奋性氨基酸、抑制性氨基酸的含量

建立了反相高效液相色谱法测定羊水中兴奋性氨基酸天门冬氨酸、谷氨酸,抑制性氨基酸甘氨酸含量的方法,色谱柱为LUNAC18柱(4.6mm×250mm,5μm),流动相为乙腈水(V/V),按低压梯度洗脱,梯度系统0～4min,乙腈40%;4～20min,乙腈40%～52%;20～30min,乙腈52%～60%;30～40min,乙腈60%～40%。流速0.8mL/min,柱温40℃,紫外检测波长260nm;进样量10μL。结果显示,天门冬氨酸、谷氨酸和甘氨酸三者的线性范围均为2.5～85mg/L;标准加入的回收率为99.6%～102.6%。本方法灵敏度高、测定结果可靠。用本方法对201例不同孕期的羊水作兴奋性和抑制性氨基酸检测,发现羊水中3种氨基酸随妊娠进展而增加的趋势,胎儿畸形或宫内缺氧时羊水中这3种氨基酸水平明显升高。     

微分脉冲极谱同时测定三种碱性氨基酸的研究

应用微分脉冲极谱，在ｐＨ９．０ ＮａＢ４Ｏ７－ ＣＨ３ＣＨＯ－Ｃｏ２＋－ ＮａＯＨ组成的极谱底液，扫描电位－ ０．８０～－ １．６０ Ｖ、振幅 ２０ｍＶ、扫描速度５ｍＶ／ｓ、一滴汞周期２ｓ的条件下进行连续扫描测量三种碱性氨基酸，获得三个灵敏 度和分辨率均较高的极谱峰图。该法简便快速，稳定可靠，为测量各种蛋白质中的三种磁性氨基酸提供一种新途 径。     

The Determination of Protonation Constants of Some Amino Acids and Their Esters by Potentiometry in Different Media

In this study, stoichiometric protonation constants of L-tyrosine, L-cysteine, L-tryptophane, L-lysine, and L-histidine, and their methyl and ethyl esters in water and ethanol–water mixtures of 30, 50, and 70% ethanol (v/v), were determined potentiometrically using a combined pH electrode system calibrated as the concentration of hydrogen ion. Titrations were performed at 25^∘C and the ionic strength of the medium was maintained at 0.10 mol⋅L⁻¹ using sodium chloride. Protonation constants were calculated by using the BEST computer program. The effect of solvent composition on the protonation constants is discussed. The log₁₀ K₂ values of esters generally decreased with increasing ethanol content. However, the log₁₀ K₁ values of the esters of L-tyrosine, L-cysteine, and L-tryptophane were found to increase with increasing ethanol content in contrast those of L-lysine and L-histidine esters.