高效液相色谱梯度洗脱同时测定化妆品中防腐剂、抗氧化剂和杀菌剂

建立了一种灵敏、快速的高效液相色谱梯度洗脱同时测定化妆品中防腐剂、抗氧化剂和杀菌剂的方法。采用C8柱,以甲醇和水为流动相梯度洗脱。在检测波长273nm用二极管阵列检测器,17min内可将4种防腐剂、2种抗氧化剂和2种杀菌剂分离测定。方法快速准确,用于实际样品的测定。     

HPLC与UPLC色谱条件转换方法研究

以分离分析化妆品中对羟基苯甲酸酯类防腐剂为内容,对HPLC和UPLC的色谱条件转换方法进行了研究。比较了采取不同方法转换得到的色谱条件参数的分离状况,选出了UPLC法最佳色谱条件。同时,用HPLC法和UPLC法对4种化妆品中的4种对羟基苯甲酸酯类防腐剂进行了定量测定,两种方法的测定结果吻合较好,相互印证了方法的准确性。     

高效液相色谱-电感耦合等离子体质谱法同时测定化妆品中5种含溴防腐剂

建立了同时测定化妆品中苯扎溴铵、2-溴-2-硝基-1,3-丙二醇、5-溴-5-硝基-1,3-二■烷、甲基二溴戊二腈、溴氯芬5种含溴防腐剂的高效液相色谱-电感耦合等离子体质谱法(HPLC-ICP-MS)。样品经含0.1%甲酸的甲醇溶液超声提取后,采用Agilent Eclipse-C_(18)(150 mm×4.6 mm,5μm)色谱柱分离,以0.1%甲酸-甲醇为流动相进行梯度洗脱,ICP-MS测定组分中的~(79)Br,以保留时间定性,外标法定量。5种含溴防腐剂均在0.5～100 mg/L范围内线性关系良好(r0.999),检出限为1.5～3.0μg/g,不同基质化妆品中的回收率为91.2%～108%,相对标准偏差(n=6)为1.3%～4.2%。该方法快速、准确、灵敏、专属性强,适用于化妆品中5种含溴防腐剂的定性定量分析。     

反相高效液相色谱法测定化妆品中的24种防腐剂

建立了同时检测化妆品中24种防腐剂含量的反相高效液相色谱法(RP-HPLC).采用Kromasil C18 (4.6 mm×250 mm,5 μm)色谱柱,以磷酸盐缓冲溶液(pH=4.26)为流动相,梯度洗脱.样品经甲醇超声提取,然后采用RP-HPLC-二极管阵列检测法测定,对样品前处理和色谱条件进行研究和优化.方法的相对标准偏差为1.3%～3.3%;回收率为90.6%～97.8%;各种防腐剂的线性相关系数≥0.9997,具有较高的准确度和精密度,可用于化妆品中24种防腐剂含量的分析.     

气相色谱-质谱法测定化妆品中多种防腐剂

采用超声抽提法对化妆品中的苯甲醇、3-甲基-4-异丙基苯酚、对羟基苯甲酸丁酯和2-苄基-4-氯酚等18种防腐剂进行了气相色谱-质谱法(GC-MS)测定的研究。建立了一种简单、快速、准确测定化妆品中各种防腐剂的测定方法。进行了样品提取溶剂和超声提取时间选择以及线性、回收率、精密度试验。结果表明,该方法能够有效地提取化妆品(口红和香波)中的18种防腐剂,并可对其进行GC-MS分离和鉴定。18种防腐剂的平均回收率为91.66%-100.6%(n=7),相对标准偏差为0.46%-6.23%(n=7),最低检测限为     

气相色谱-质谱法测定化妆品中10种防腐剂

采用气相色谱-质谱法(GC-MS)同时测定化妆品中10种防腐剂含量。样品经甲醇超声提取,无水硫酸钠脱水后过滤进样检测。采用Agilent HP-5MS毛细管色谱柱(30m×0.25mm,0.25μm)分离,程序升温,分流进样进行测定。结果表明:17min内即可完成10种防腐剂的测定,各防腐剂的质量浓度均在5.00~100mg·L-1范围内与峰面积呈线性关系,方法的检出限(3S/N)为0.30~0.70ng。方法用于化妆品测定,加标回收率在96.5%~105%之间,测定值的相对标准偏差(n=6)在0.66%~3.2%之间。     

色谱柱分类数据库用于指导天然药物化学对照品色谱纯度测定时色谱柱理性选择

由于中药化学对照品多数来源于动植物药材,很容易混有结构类似物,故有机杂质测定是可能影响其化学对照品赋值准确性的关键风险因素。中药化学对照品的有机杂质测定通常采用药典收载或文献报道的高效液相色谱法,这些方法通常仅规定“以十八烷基硅烷键合硅胶为填充剂”,无适宜色谱柱的品牌信息,或者实验室无文献所用的色谱柱品牌,而目前市场上已有800多种品牌的C₁₈柱,生产工艺的不同导致不同品牌C₁₈柱的选择性有差异,甚至差异显著。这很容易出现由于色谱柱选择不适宜而导致测定结果不准确的风险。该文采用国外色谱柱分类数据库指导对照品纯度考察时色谱柱的理性选择,尽可能减少色谱柱盲选可能导致的纯度结果不准确的风险。首先,用数据库挑选2根选择性差异显著的色谱柱（选择性因子F≥6）进行平行实验,以尽可能反映采用不同品牌色谱柱可能出现的分离效果差异。如果这2根色谱柱的分离效果及纯度测定结果无显著性差异,则可以交叉验证该对照品纯度测定的准确性。否则需要从数据库中选择另外1根与之前试验中分离效果更好、选择性相似的色谱柱进行纯度结果验证。在N-反式-p-对香豆酰基酪胺和表儿茶素没食子酸酯首批对照品的纯度考察中,使用了上述策略并验证了其有效性和科学性,计划推广应用至更多的中药化学对照品,特别当其可能含碱性或弱酸性化合物时,更应该尝试采用本文推荐的色谱柱选择策略交叉验证其纯度测定结果的准确性。     

高效液相色谱法测定三嗪类防腐剂中苯乙醇

苯乙醇常作为防腐剂的添加剂使用,它既具有香料的作用又有协同杀菌作用。为了进行防腐剂的配方研究和稳定性研究,我们建立了苯乙醇的高效液相色谱(HPLC)测定方法。关于苯乙醇的HPLC分离已有一些报道,但是三嗪类防腐剂中苯乙醇的HPLC分离和测定都还没有报道。 由于三嗪类防腐剂中组分复杂,苯乙醇的含量仅在万分之几,而且在反相色谱中又在主峰的后边,给分离带来了一定困难。本工作通过选择灵敏的检测波长和最佳的流动相组成,并在流动相中加入少量磷酸解决了大峰拖尾问题,使苯乙醇获得了较好的分离和测定。     

液相色谱法同步测定化妆品中6种邻苯二甲酸酯

采用甲醇超声提取,高效液相色谱-二极管阵列检测器(HPLC-DAD)同步测定化妆品中6种邻苯二甲酸酯类环境激素;探讨了流动相和色谱柱对6种邻苯二甲酸酯分离的影响,以及二极管阵列检测器对定性分析的重要性和检测波长的选择,并对实际样品进行了测定.结果表明:方法的线性相关系数R>0.999 8,检出限在4.0～10.0mg/kg,加标回收率为90%～98%,相对标准偏差为0.11%～1.13%.该方法灵敏、快速、高通量,可用于检测国际关注的6种邻苯二甲酸酯,为化妆品中邻苯二甲酸酯的测定提供参考依据.     

色谱-质谱联用技术测定化妆品中25种邻苯二甲酸酯

建立了乳液、霜、水以及油类化妆品中25种邻苯二甲酸酯类化合物的气相色谱-质谱和液相色谱-质谱测定方法。不同基质样品经不同方法净化处理后,采用气相色谱-质谱或液相色谱-质谱进行测定。气相色谱-质谱法采用DB-5MS毛细管色谱柱(30 m,250 mm×0.25μm),程序升温,选择离子模式同时测定21种邻苯二甲酸酯类化合物。液相色谱-质谱采用MN EC-C18色谱柱(4.6×100 mm,2.7μm),以甲醇和0.1%甲酸为流动相,梯度洗脱,流速0.7 mL/min,采用电喷雾电离(ESI+),多反应监测(MRM)模式同时测定24种邻苯二甲酸酯类化合物。25种邻苯二甲酸酯类化合物的线性关系良好,相关系数均大于0.999,回收率实验结果为89.3%~105.6%,RSD为0.4%~4.0%,检出限均小于0.3 mg/kg。方法适用于化妆品中邻苯二甲酸酯类化合物的全面筛查。     

蛋白质高效分离两维色谱柱的选择优化

为了构建高效的离子交换/反相二维液相色谱(IEC/RPLC)分离平台系统,提高复杂蛋白质样品的分离效率,对色谱柱进行了评价与筛选。通过对实际人肝蛋白质样品的分离效果的比较,选择确定了TSKgel DEAE-5PW弱阴离子交换色谱柱(WAX)作为第一维色谱分离柱;考察了同一规格的10支代表性反相色谱柱(250 mm×4.6 mm, 5 μm, 30 nm, C4、C8或C18),通过评价其对尿嘧啶、硝基苯、萘和芴的分离性能以及对3种标准蛋白质样品的非特异性吸附、对人肝蛋白质样品的WAX馏分的分离效果,最终确定以Jupiter 300 C4反相色谱柱作为第二维色谱分离柱。对两维色谱柱的选择优化为蛋白质高效分离二维液相色谱平台的搭建提供了可靠基础。     

高效液相色谱法同时测定阿达帕林凝胶剂中的主药阿达帕林和两种防腐剂

建立了同时测定阿达帕林凝胶剂中主药阿达帕林和防腐剂(苯氧乙醇、对羟基苯甲酸甲酯)含量的反相高效液相色谱法(HPLC)。采用Tigerkin C18柱(150 mm×4.6 mm,5 μm),以pH 3.0的0.02 mol/L醋酸盐缓冲液-四氢呋喃-乙腈为流动相进行梯度洗脱,在270 nm波长条件下检测。线性范围:苯氧乙醇,10～100 mg/L(r=0.9999);对羟基苯甲酸甲酯,4～40 mg/L(r=0.9999);阿达帕林,4～40 mg/L(r=0.9999)。3种组分的平均回收率为98.0%～98.6%。该方法简便、可靠,可用于阿达帕林凝胶剂中阿达帕林、苯氧乙醇和对羟基苯甲酸甲酯的同时测定。     

Properties of two amide‐based hydrophilic interaction liquid chromatography columns

Hydrophilic interaction liquid chromatography is a separation technique suitable for the separation of moderately and highly polar compounds. Various stationary phases (SPs) for hydrophilic interaction liquid chromatography are commercially available. While the SPs based on the same type of ligand are available from different providers, they can display a distinct retention characteristics and separation selectivity. The current work is focused on characterization and comparison of the separation systems of two amide‐based HPLC columns from two producers, i.e. XBridge Amide column and TSK gel Amide‐80 column. Several characterization procedures (tests) were used to investigate the differences between these columns. The chromatographic behavior of selected analytes indicates that multimodal interactions are responsible for retention and separation on these columns. Multiple testing approaches were used in order to reveal subtle differences between the SPs. Both amide‐based columns showed certain differences in retention, selectivity, and plate counts. Based on the tests used in this study, we conclude that the investigated columns provide a different degree of H‐bonding interactions.     

(3,5-二甲基苯基氨基甲酸酯)衍生的纤维素手性固定相

纤维素三（3,5-二甲基苯基氨基甲酸酯）是液相色谱中使用最广泛的手性柱。该文详细地研究了不同程度衍生的纤维素（3,5-二甲基苯基氨基甲酸酯）以及不同硅胶（粗制硅胶、氨丙基粗制硅胶、精制硅胶、氨丙基精制硅胶、大孔硅胶、氨丙基大孔硅胶）作为支撑体对该柱手性分离能力的影响。自制了13根手性色谱柱,分别考察了其对16种外消旋体的拆分,分离结果显示：三取代纤维素柱 > 二取代纤维素柱 > 纤维素柱;精制硅胶和大孔硅胶优于粗制硅胶,大孔硅胶的柱压更低;硅胶的氨丙基化对手性选择性有一定的影响;这些手性柱之间具有一定的互补性,尤其是纤维素柱。该文有助于人们更深刻地理解和更好地把握高效液相色谱手性柱的制备。     

Comparison of different types of stationary phases for the analysis of soy isoflavones by HPLC

Nowadays, there are new technologies in high-performance liquid chromatography columns available enabling faster and more efficient separations. In this work, we compared three different types of columns for the analysis of main soy isoflavones. The evaluated columns were a conventional reverse phase particle column, a fused-core particle column, and a monolithic column. The comparison was in terms of chromatographic parameters such as resolution, asymmetry, number of theoretical plates, variability of retention time, and peak width. The lower column pressure was provided by the monolithic column, although lower chromatographic performance was achieved. Conventional and fused-core particle columns presented similar pressure. Results also indicate that direct transfer between particle and monolithic columns is not possible requiring adjustment of conditions and a different method optimization strategy. The best chromatographic performance and separation speed were observed for the fused-core particle column. Also, the effect of sample solvent on the separation and peak shape was evaluated and indicated that monolithic column is the most affected especially when using higher concentrations of acetonitrile or ethanol. Sample solvent that showed the lowest effect on the chromatographic performance of the columns was methanol. Overall evaluation of methanol and acetonitrile as mobile phase for the separation of isoflavones indicated higher chromatographic performance of acetonitrile, although methanol may be an attractive alternative. Using acetonitrile as mobile phase resulted in faster, higher resolution, narrower, and more symmetric peaks than methanol with all columns. It also generated the lower column pressure and flatter pressure profile due to mobile phase changes, and therefore, it presents a higher potential to be explored for the development of faster separation methods.     

C18柱串联冠醚手性柱高效分离3种芳香族氨基酸对映体

将C18柱与手性冠醚柱串联,建立了一种反相高效液相色谱法用于3种芳香族氨基酸对映体同时拆分的方法.考察了反相色谱流动相的组成、pH值、柱温、流速对对映体拆分的影响.实验结果表明,当流动相为HClO4-乙睛溶液(86:14,V/V,pH 2.0)、柱温20℃、流速0.4 mL/min时,3种氨基酸对映体可获得基线分离.进一步对比了C18柱、冠醚手性柱和串联顺序不同的4种分离模式,结果表明,C18柱不能拆分氨基酸对映体,仅能分离不同种类氨基酸;冠醚手性柱可分离氨基酸映体,但不同种类氨基酸色谱峰出现重叠;串联模式能实现3种氨基酸对映体的基线分离,实现双柱优势互补,而串联顺序对分离影响不大,仅影响色谱峰的峰形.     

Comparison of ultra high performance supercritical fluid chromatography,ultra high performance liquid chromatography,and gas chromatography for the separation of synthetic cathinones

A comparison of ultra high performance supercritical fluid chromatography, ultra high performance liquid chromatography, and gas chromatography for the separation of synthetic cathinones has been conducted. Nine different mixtures of bath salts were analyzed in this study. The three different chromatographic techniques were examined using a general set of controlled synthetic cathinones as well as a variety of other synthetic cathinones that exist as positional isomers. Overall 35 different synthetic cathinones were analyzed. A variety of column types and chromatographic modes were examined for developing each separation. For the ultra high performance supercritical fluid chromatography separations, analyses were performed using a series of Torus and Trefoil columns with either ammonium formate or ammonium hydroxide as additives, and methanol, ethanol or isopropanol organic solvents as modifiers. Ultra high performance liquid chromatographic separations were performed in both reversed phase and hydrophilic interaction chromatographic modes using SPP C18 and SPP HILIC columns. Gas chromatography separations were performed using an Elite‐5MS capillary column. The orthogonality of ultra high performance supercritical fluid chromatography, ultra high performance liquid chromatography, and gas chromatography was examined using principal component analysis. For the best overall separation of synthetic cathinones, the use of ultra high performance supercritical fluid chromatography in combination with gas chromatography is recommended.     

Development and validation of an improved liquid chromatographic method for the analysis of dirithromycin

The official method for the determination of dirithromycin and related substances in the European Pharmacopoeia (Ph. Eur.) and in the United States Pharmacopeia (USP) is an isocratic liquid chromatographic (LC) method using an ODS column. With this method, the separation of the main component dirithromycin from its epimer is not complete. Moreover, this method suffers sometimes from drift of the baseline and from subsequent quantitation problems. The required resolution is not easy to obtain.

Using an adapted method derived from the one prescribed in the pharmacopoeias, the selectivity of a set of more than 40 reversed-phase columns towards dirithromycin components was investigated. The selection of the most suitable column was achieved by the chromatographic response function (CRF) approach. Several changes were introduced to the method in order to improve the separation and to overcome the baseline drift problem. The resulting method uses a Zorbax Extend column maintained at 30 °C and a mobile phase containing acetonitrile, methanol, 2-propanol, water and a phosphate buffer at pH 7.5. The method allows a good separation of dirithromycin components, which is much better than that obtained with the existing methods. Several impurities of unknown identity are also separated. The method shows good repeatability, linearity and sensitivity, and it is robust. In addition, it proved to be applicable to a wide number of C18 reversed-phase columns.     

Comparison of separation power of ultra performance liquid chromatography and comprehensive two-dimensional liquid chromatography in the separation of phenolic compounds in beverages

In this study, 1-D and 2-D liquid chromatographic systems, namely, conventional HPLC, UPLC, HPLC x HPLC and HPLC x UPLC systems were developed and evaluated for the separation of phenolic acids in wine and juices. In the LC x LC studies, the first dimension separation was based on RPLC and the second dimension was performed with ion-pair chromatography. Three different columns, namely two short columns packed with either 2.5 or 1.7 microm particles and a monolithic column, were tested for the fast second dimension separation. The best results were obtained when the monolithic column was applied for the second dimension separation. The peak capacities for comprehensive 2-D systems varied from 330 to 616.