高效液相色谱法快速测定鸭肉和鸭蛋中苏丹红染料

建立了一种快速测定鸭肉和鸭蛋中苏丹红染料的高效液相色谱分析方法。样品经乙腈提取后浓缩至干,最后用乙腈定容;采用ZorbaxSB-C18柱,以乙腈-水为流动相等度洗脱,进行高效液相色谱分离,二极管阵列检测器检测,外标法定量。6种苏丹红染料标准曲线的线性回归系数均在0.999以上;线性范围为30～1000μg/L;检出限在4～13μg/kg之间。同时在40、80和200μg/kg3个添加浓度水平下添加回收率为85.3%～96.6%;相对标准偏差在1.8%～5.2%之间。本方法具有快速、灵敏的特点。     

离子液体中卤素离子杂质的离子色谱-直接电导检测法分析

研究了离子色谱-直接电导检测法分离测定离子液体中的卤素离子(F~-、Cl~-、Br~-)杂质.采用Shim-pack IC-A3阴离子交换色谱柱,考察了淋洗液种类及浓度、流速和色谱柱温度对分离测定的影响.最佳色谱条件为:以1.25 mmol/L邻苯二甲酸氢钾为淋洗液,流速1.5 mL/min,色谱柱温45 ℃.在此条件下可以基线分离卤素离子,且NO~-_3、BF~-_4、SO~(2-)_4不干扰测定.该法测定卤素离子的检出限(S/N=3)为0.02 ～0.11 mg/L,峰面积的相对标准偏差(n=5)不大于0.7%,F~-、Cl~- 和Br~- 的标准曲线的线性范围分别为0.1 ～50、0.1 ～50、0.5 ～100 mg/L.将方法用于烷基咪唑四氟硼酸盐离子液体中卤素离子杂质的测定,加标回收率为98% ～102%.     

UPLC-MS-MS法快速测定含乳冷冻饮品中氯霉素残留量

建立了UPLC-MS-MS法测定含乳冷冻饮品中氯霉素的含量。样品经高氯酸沉淀蛋白,乙酸乙酯提取,浓缩干燥,流动相溶解,正己烷脱脂后,采用ACQUITYUPLCBHEC18色谱柱分离,以1％甲酸水溶液一乙腈为流动相进行梯度洗脱,利用电喷雾质谱负离子监测模式对氯霉素进行检测。氯霉素浓度在0．1～100．0ng／mL范围内与色谱峰面积呈良好的线性,线性相关系数r=0．9986。加标回收率为81．5％～103．4％,测定结果的相对标准偏差为1．72％-3,18％（n=5）,以3倍信噪比计算方法的检出限为0．1μg／kg。     

凝胶渗透色谱-气相色谱质谱法测定：花生中6种除草剂农药残留

建立了凝胶渗透色谱一气相色谱质谱（GPC～GC=MS）法测定花生中6种除草剂（氟乐灵、异恶草酮、甲草胺、二甲戊乐灵、乙氧氟草醚、喹禾灵）农药残留的方法。样品经乙腈提取,氨基固相萃取柱和凝胶渗透色谱净化,在选择离子扫描（SIM）模式下进行气相色谱质谱法测定,外标法定量。6种除草剂浓度在0．02-1．00mg／L范围内与色谱峰面积呈良好的线性,线性相关系数为O．9949～0．9998,添加回收率为77．8％-101．6％,测定结果的相对标准偏差为4．4％～11．4％（月=5）,方法的检出限为0．1～1．3μg／kg。     

反相高效液相色谱法同时测定新生儿尿液中4种苯丙酮尿症特征酸的含量

提出了反相高效液相色谱同时测定新生儿尿液中4-羟基苯乙酸、2-羟基苯乙酸、苯乙酸和苯丙酮酸等4种苯丙酮尿症特征酸的方法。取尿液样品5.00mL,乙腈5mL,混合振荡1min,离心10min,取上清液进行液相色谱分离。用Waters Symmetry C18色谱柱作为固定相,用不同比例的乙腈和0.15%(体积分数)磷酸溶液进行梯度洗脱,检测波长为210,289nm。在上述条件下,4种特征酸分离完全,并且不受尿液中内源性物质的干扰。4种特征酸的质量浓度在一定范围内呈线性,检出限(3S/N)分别为0.43,0.22,0.62,0.42mg·L-1。按标准加入法在3个浓度水平上进行加标回收试验,测得回收率在89.1%~108%之间,测定值的相对标准偏差(n=6)小于4%。     

梯度淋洗离子对色谱法测定咪唑离子液体中的阳离子

采用梯度淋洗离子对色谱-紫外检测(IPC-UV)法分离测定5种咪唑离子液体中的阳离子。实验采用ZORBAX Eclipse XDB C18色谱柱,以离子对试剂与乙腈为流动相,首先考察了离子对试剂种类和浓度、乙腈浓度和色谱柱温度对咪唑阳离子保留的影响,然后确定了最适宜分离的色谱条件。在此条件下可同时基线分离5种咪唑阳离子。所测阳离子的检出限(S/N=3)为0.05～0.30 mg/L,峰面积的相对标准偏差(RSD, n=5)在0.1%以下。将此方法用于分析实验室合成的2种1-烷基-3-甲基咪唑离子液体中的阳离子,加标回收率在98.6%～102.1%之间。本方法准确、可靠,具有较好的实用性。     

反相硅胶整体柱离子对色谱法快速测定吡啶离子液体阳离子

建立了整体柱离子对色谱-紫外检测法梯度淋洗快速分离测定4种吡啶离子液体阳离子的方法。分离采用C18反相硅胶整体柱,以离子对试剂(用柠檬酸调节pH值)-乙腈为淋洗液,并采用多级梯度洗脱程序。实验考察了色谱柱、离子对试剂、乙腈浓度、色谱柱温度及流速对吡啶阳离子保留的影响,并讨论了其保留规律。咪唑阳离子的保留符合碳数规律。最佳色谱条件是:在流速3.0 mL/min,柱温30℃下,以1.0 mmol/L庚烷磺酸钠(pH 4.0)(A)+乙腈(B)为淋洗液进行梯度洗脱。淋洗梯度为0～2.0 min,10%B;2.0～2.5 min,10%～15%B;2.5～4.0 min,15%B;4.0～4.5 min,15%～20%B;4.5～10.0 min,20%B。在此条件下,4种吡啶阳离子可在7 min内基线分离。所测阳离子的检出限(S/N=3)为0.05～0.17 mg/L;峰面积的相对标准偏差(n=5)小于0.6%。将本方法用于实验室合成的离子液体样品和污水样品的分析,加标回收率在95.7%～99.0%之间。本方法准确、快速,具有较好的实用性。     

有机酸的非抑制型离子排斥色谱法测定

研究了非抑制型离子排斥色谱分离测定7种有机酸(柠檬酸、酒石酸、苹果酸、琥珀酸、乳酸、甲酸、乙酸)的方法.以Shim-pack SCR-102H柱为分离柱,选用对甲苯磺酸-乙腈为淋洗液,考察了淋洗液浓度、流速、pH、色谱柱温度及淋洗液中乙腈含量等条件对分离和测定的影响.通过实验确定最佳的色谱条件:2.0 mmol/LP-甲苯磺酸-乙腈(体积比91:9)为淋洗液,流速1.0 mL/min,柱温50℃,pH 2.8.该法对所测有机酸的检出限在0.06～1.05.mg/L之间,相对标准偏差在3.3%以下(n=5),加标回收率在96%-101%之间,整个分析过程在11 min内完成.     

直接进样气相色谱法测定密闭环境中有机硫化合物

建立了直接进样气相色谱-硫化学发光法测定密闭环境空气中微痕量有机硫化合物的方法。密闭环境空气通过直接进样、DB-SULFUR毛细管色谱柱分离、硫化学发光检测器进行检测，实现了对密闭环境空气中二硫化碳、甲硫醇等8种有机硫化物完全分离并准确测定。以目标组分的色谱峰面积响应值对相应质量浓度进行线性回归，计算线性方程和相关系数。建立的8种有机硫化物标准曲线线性良好，相关系数达0.999，加标回收率为96.4%～111.2%，测定结果的相对标准偏差不大于3%(n=6)，方法检出限为0.003～0.008 mg/m³，部分有机硫化物的检出限低于人体嗅觉阈值。     

高效液相色谱法分离测定牦牛乳中的8种蛋白质

建立了同时分离和测定牦牛乳中4种酪蛋白和4种乳清蛋白的反相高效液相色谱方法。脱脂牦牛乳经分散剂处理后,采用C4色谱柱(250 mm×4.6 mm,300,5μm i.d.)进行分离,以0.1%的三氟乙酸水溶液和0.1%的三氟乙酸乙腈溶液为流动相,流速为0.8 mL/min,梯度洗脱,二极管阵列检测器(DAD)在220nm波长下检测,外标法定量。结果表明,牦牛乳中8种主要蛋白质在40 min内完全分离,在各自的线性范围内呈良好线性,除α-乳白蛋白外,其余7种蛋白的相关系数均大于0.99。8种蛋白质的回收率为86%～103%,相对标准偏差(RSDs)为1.7%～8.7%;检出限(LODs)为10.7～39.2 mg/L,定量下限(LOQs)为35.7～130.7 mg/L。该方法的准确度和精密度均较高,能够满足实际检测的要求。     

Effect of steric exclusion on the separation of proteins by hydrophilic size-exclusion chromatography

On the basis of studying the retention and band broadening of proteins on the TSK SW column, diffusion coefficients (Ds) of solute in stationary phase were obtained which elucidate the hydrodynamic process of chromatographic resolution of proteins by hydrophilic size-exclusion chromatography (SEC). After calculating the correlation between Ds and the molecular weight of the solute, the molecular dimensions of proteins in the process of chromatographic separation can be predicted. Deviations in diffusion coefficient of a protein from the calculated value reflect differences of measured molecular dimensions from molecular volumes predicted from the calibration curve of the SEC column. This study illustrates a convenient method for estimating the purity of proteins by SEC. Deviations from 2 lambda dp (where dp is the particle diameter) in the intercept of the theoretical plate height (H) versus flow-rate (U) curve from the band broadening equation H = CsU + 2 lambda dp + f(alpha M)T (where CsU represents mass transfer resistance caused by solute diffusion in the stationary phase and f(alpha M)T an added term for polydisperse solutes as proposed by Knox and McLennan [Chromatographia, 10 (1977) 75]) reflect impurities in the proteins.     

Application of off-line size-exclusion chromatographic fractionation-matrix assisted laser desorption ionization time of flight mass spectrometry for proanthocyanidin characterization

In this work, we wanted to devise a reliable method to characterize polymerized forms of tannins, their structural information and mass distribution. Size-exclusion chromatography (SEC) is a chromatographic technique used to determine molecular mass (weight) distributions of polymers. One important step in the data treatment is the modeling of the calibration curves. Polystyrenes (PS) are standards usually used because no commercial procyanidin (PC) standards are available. An off-line coupling of SEC and MALDI was carried out to measure differences between polystyrenes and procyanidins. Thus, a new calibration curve was established; from 1000 to 8000 Da, there is a good correlation between the MALDI and PS calibration curves, in this field the PS calibration is correct and enables true mass determination. For masses above 8000 Da, PS calibration overestimates the real molecular weight of PC, overestimation of 53%. And for masses below 1000 Da, PS calibration underestimates their real molecular weight (10-15%). This means that to truly characterize PC, calibration based on PC standards is required.     

Size Exclusion Chromatography of Poly(vinylpyrrolidone)

Abstract

Poly(vinylpyrrolidone) and poly(ethylene oxide) separate by hydrodynamic volume on Toyo Soda TSK-PW columns in a mixed solvent mobile phase of 50:50 (v/v) MeOH/H₂O containing 0.1M LiNO₃. From this separation a single universal calibration curve based on hydrodynamic volume [η]M can be obtained. Accurate weight average molecular weights of PVP were obtained by both SEC/LALLS and universal calibration showing good agreement between the two methods. SEC/LALLS overestimates the number average molecular weight for broad distribution polymers due largely to the lack of sensitivity of the LALLS detector to the low molecular weight portion of the polymers, while the universal calibration method slightly underestimates the number average molecular weight as compared to osmometric values.     

Size Exclusion Chromatography Calibration Assessment Utilizing Coupled Molecular Weight Detectors

Abstract

This paper shows that the usual method of representing an SEC calibration curve by a single polynomial curve may often be inadequate with new high resolution columns. Data points wind about the fitted line. The significant magnitude and systematic nature of these deviations clearly appear when a plot of residuals is derived from the conventional calibration curve and expressed in terms of the percent error in molecular weight. The deviation of the calibration data from the fitted line was approximately 10% for the conventional molecular weight and intrinsic viscosity calibration curves. It became 20% for the universal calibration curve. LALLS and DV detectors were used together with the DRI detector to provide evidence that the calibration curve deviations were due to the column packings and not due to some other cause (e.g., vendor values of molecular weight). Use of a polynomial fit to a portion of the curve corresponding to the retention volume range of an unknown was used to show the significant improvement in results which occurred when the calibration variations were taken into account. At present, use of many individual narrow standards is necessary to elucidate the effect.     

一种新的标定体积排除色谱（SEC）的方法

基于体积排除色谱中测得的淋出体积和动态激光光散射中测得的平动扩散系数都直接依赖于高分子的流体力学体积这一事实，本文在理论上提出了一种把淋出体积分布和平动扩散系数分布二者结合起来标定体积排除色谱的新方法，并且在实验上通过对宽分布的聚苯乙烯标准样品的测试证实了该方法的可行性．     

Development and qualification of a size exclusion chromatography coupled with multiangle light scattering method for molecular weight determination of unfractionated heparin

The molecular weight of unfractionated heparin was determined by size exclusion chromatography (SEC) coupled with multiangle light scattering (MALS) detection. The SEC/MALS method determines absolute molecular weight directly from the angular dependence of scattered light intensity as a function of concentration and does not rely on molecular weight standards for column calibration. The SEC/MALS method developed at Scientific Protein Laboratories was qualified in terms of specificity, precision, robustness, and accuracy. By eliminating the requirement of well-characterized molecular weight standards derived from heparin, the present procedure represents a clear improvement over the column calibration methods used in molecular weight determination. The SEC/MALS method is suitable for routine quality control of unfractionated heparin.     

Simulation of size-exclusion chromatography distribution coefficients of comb-shaped molecules in spherical pores comparison of simulation and experiment

Simulations of the distribution coefficients of linear polymers and regular combs with various spacings between the arms have been performed. The distribution coefficients were plotted as a function of the number of segments in order to compare the size exclusion chromatography (SEC)-elution behavior of combs relative to linear molecules. By comparing the simulated SEC-calibration curves it is possible to predict the elution behavior of comb-shaped polymers relative to linear ones. In order to compare the results obtained by computer simulations with experimental data, a variety of comb-shaped polymers varying in side chain length, spacing between the side chains and molecular weights of the backbone were analyzed by SEC with light-scattering detection. It was found that the computer simulations could predict the molecular weights of linear molecules having the same retention volume with an accuracy of about 10%, i.e. the error in the molecular weight obtained by calculating the molecular weight of the comb-polymer based on a calibration curve constructed using linear standards and the results of the computer simulations are of the same magnitude as the experimental error of absolute molecular weight determination.     

Size-exclusion separation of proteins using a biocompatible polymeric monolithic capillary column with mesoporosity

Biocompatible poly(ethylene glycol methyl ether acrylate-co-polyethylene glycol diacrylate) monoliths were prepared for size exclusion chromatography (SEC) of proteins in the capillary format using Brij 58P in a mixture of hexanes and dodecanol as porogens. The monolithic columns provided size separation of four proteins in 20 mM sodium phosphate buffer (pH 7.0) containing 0.15 M NaCl, and there was a linear relationship between the retention times and the logarithmic values of the molecular weights. Compared to SEC monoliths previously synthesized using a triblock copolymer of polyethylene oxide and polypropylene oxide, an increase in mesoporosity was confirmed by inverse size exclusion chromatography. As a result, improved protein separation in the high molecular weight range and reduced column back-pressure were observed.     

A Method of Correcting for Flow-Rate Fluctuations in Size Exclusion Chromatography Calculations: Applications to Methylene Chloride/Hexafluoroisopropanol Solvent System

Abstract

The mixture of methylene chloride/hexafluoroisopropanol (70/30, v/v) is an excellent polyester solvent, but its low boiling point causes unstable flow when it is used for size exclusion chromatography (SEC). In high-performance SEC experiments, retention time is normally used to measure elution volume; however, unstable flow makes it difficult to calibrate an SEC column set or calculate molecular weight parameters from a chromatogram. We have devised a simple and inexpensive method to compensate for the effect of unstable flow in SEC calculations. A calibration marker injected along with each sample is used to indicate flow-rate variations. The ratio of the sample retention time to the marker retention time is invariant to flow-rate changes and is used in place of retention time as a measure of elution volume in the universal calibration technique. Calibrating a column set and analyzing chromatograms by this method result in a large improvement in the accuracy and precision of calculated molecular weight parameters.     

Characterization of Nonionic Polyacrylamides by Aqueous Size Exclusion Chromatography Using a DRI/LALLSP Detector System

Abstract

Herein is reported an experimental investigation of the molecular weight characterization of nonionic polyacrylamides by aqueous SEC with a DRI/LALLSP detector system. Methodology for the use of the DRI/LALLSP detector responses to determine the molecular weight calibration curve and the peak broadening parameter, [sgrave]² (variance of a Gaussian instrumental spreading function) over a wide molecular weight range has been developed. The method is based on the use of a broad MWD standard made by blending Polysciences broad MWD standards and a generalized analytical solution of Tung's integral equation for the detector response corrected for peak broadening. Molecular weight averages measured by SEC/DRI/LALLSP are in excellent agreement with those measured offline by LALLSP.