高效液相色谱–波长切换法同时测定独一味软胶囊中6种成分

建立高效液相色谱–波长切换法同时测定独一味软胶囊中山栀苷甲酯、绿原酸、8-O-乙酰山栀苷甲酯、连翘酯苷B、毛蕊花糖苷和木犀草苷的方法。以Symmetry Shield RP18柱(250 mm×4.6 mm,5 μm)为色谱柱,乙腈–0.3%磷酸水为流动相,检测波长分别为235 nm(山栀苷甲酯、8-O-乙酰山栀苷甲酯)、330 nm(绿原酸、连翘酯苷B、毛蕊花糖苷)、360 nm(木犀草苷),流量为1 mL/min。山栀苷甲酯、绿原酸、8-O-乙酰山栀苷甲酯、连翘酯苷B、毛蕊花糖苷和木犀草苷的进样量在各自的范围内与色谱峰面积线性关系良好,相关系数不小于0.999 0,测定结果的相对标准偏差为0.21%～0.69%(n=6),平均加标回收率为94.0%～101.1%。该方法简单、准确、重现性好,适用于独一味软胶囊的质量评价。     

高效液相色谱法测定新雪颗粒中栀子苷的含量

建立了新雪颗粒中栀子苷含量的高效液相色谱测定方法。色谱柱为Diamonsil C18(200 mm×4.6 mm i.d., 5 μm), 流动相为乙腈-水(体积比为15∶85),流速1.0 mL/min,检测波长238 nm,进样量20 μL。栀子苷在25~400 mg/L时其浓度与峰面积呈良好的线性关系,方法平均回收率为101.2%,相对标准偏差(RSD)为1.6％。     

基于超高效合相色谱对黄芪中5种主要黄酮类化合物的快速检测

建立了利用超高效合相色谱法(Ultra performance convergence chromatography,UPC2)快速分离和测定黄芪中5种主要黄酮类化合物(毛蕊异黄酮、毛蕊异黄酮苷、美的紫檀素、芒柄花苷、芒柄花素)的方法.黄芪样品采用80％乙醇提取后,以超临界CO2-0.2％ H3PO4-甲醇溶液为流动相,梯度洗脱,色谱柱为Waters ACQUITY UPC2 CSH柱(100 mm×3.0 mm,1.8 μm),柱温为40℃,流速为0.4 mL/min,进样量为1μL,检测波长为280 nm.整个分析过程仅需15 min,分析速度是传统液相色谱的3倍以上.结果表明:毛蕊异黄酮、毛蕊异黄酮苷、美的紫檀素、芒柄花苷与芒柄花素的检出限及定量限范围分别在0.3 ～0.5 mg/kg和1.0～2.0 mg/kg之间,5种黄酮类成分的加标平均回收率均高于99.7％,相对标准偏差(RSD)小于2.2％(n=6);在最优条件下,对13批不同产地的黄芪进行检测,毛蕊异黄酮、毛蕊异黄酮苷、美的紫檀素、芒柄花苷与芒柄花素的含量范围分别在4.8 ～ 102 mg/kg、14 ～ 277 mg/kg、0 ～ 135 mg/kg、5.3 ～ 119 mg/kg及2.8 ～ 41 mg/kg之间;本方法简便快速,重复性良好,结果准确可靠,可用于黄芪药材中5种主要黄酮类成分的含量测定.     

苹果叶和花在花开放过程中根皮苷含量动态变化研究

对同时期苹果叶和花在花开放过程中根皮苷含量动态变化进行了研究。以根皮苷含量为指标,采用HPLC法测定苹果叶和花中根皮苷含量,色谱条件:采用PUXIANG C18色谱柱(4.6 mm×5 mm,5μm),以甲醇-0.1%磷酸水溶液为流动相,梯度洗脱,进样量为20μL,流速为0.8 mL/min,检测波长270 nm,柱温30℃.根皮苷进样量在0.40～16.00μg(r=0.999 1)范围内与峰面积呈良好的线性关系;苹果叶和苹果花中根皮苷的含量大体上呈现出先增加后降低又上升的趋势,二者变化趋势基本一致,在第6天含量达到最高,最高含量分别为263.92和143.00 mg/g.在花开放过程中,对比同时期的苹果叶和苹果花中根皮苷含量,苹果叶中根皮苷含量明显高于苹果花中根皮苷含量.     

高效液相法测定芦荟胶囊中的芦荟甙

 建立了高效液相法测定芦荟胶囊中芦荟甙含量的方法。实验采用ODS柱 ,以甲醇 水 (体积比为 5 0∶5 0 )溶液为流动相 ,用紫外检测器于 2 98nm处检测。结果表明 ,芦荟甙的进样量为 0 0 2 μg～ 1 5 μg时 ,进样量与峰面积呈良好的线性关系 (r =0 9999) ;样品的加标回收率为 99 0 %～ 10 1 9% ;方法的精密度好 ,相对标准偏差(RSD)为 1 37% (n =6 )。方法快速、简便、准确 ,所测结果稳定、重现性好 ,可作为胶囊类保健食品质量检验的一个定量方法。     

HPLC同时测定毛蕊花糖苷、咖啡酸和羟基酪醇

根据毛蕊花糖苷、羟基酪醇、咖啡酸的紫外吸收性质,建立了同时检测3种物质的高效液相色谱法。采用Waters e2695型高效液相色谱仪,色谱柱为Waters Symmetry C18柱(5μm,250 mm×4.6 mm);流动相为甲醇(A)和体积分数0.1%甲酸水溶液(B),比例为40:60(V/V);流速0.7 m L/min;2998PDA二极管阵列检测器,检测波长280 nm,柱温35℃;进样量10μL。毛蕊花糖苷标准曲线的线性回归方程为y=4.474ρ+5.224,R2=0.9999;加样回收率为100.2%。咖啡酸标准曲线的线性回归方程为y=20.687ρ-3.392,R2=0.9995;加样回收率为100.0%;羟基酪醇标准曲线的线性回归方程为y=4.716ρ-17.901,R2=0.9999;加样回收率为102.0%;毛蕊花苷的检测限为5 ng,咖啡酸的检测限为0.8 ng,羟基酪醇的检测限为0.25 ng。     

反相高效液相色谱法测定康肾颗粒中的葛根素

建立了反相高效液相色谱分离、质谱定性、紫外检测定量测定康肾颗粒中葛根素含量的方法。采用YMC-ODS色谱柱(4.6 mm i.d.×100 mm,10 μm),选用甲醇(含0.1%三氟醋酸)和水(含0.1%三氟醋酸)体系为流动相,非线性梯度洗脱分离,流速1.0 mL/min,检测波长250 nm;用基质辅助激光解吸离子化飞行时间质谱(MALDI-TOF MS)分析鉴定对照品和样品的馏分,在确定目标峰后进行紫外检测定量测定。结果表明,葛根素在0.132 ~1.32 μg范围内其峰面积与进样量呈良好的线性关系（r=0.9997）,平均加标回收率高于103%,相对标准偏差低于2.0%(n=6)。应用该方法测定康肾颗粒中葛根素,其平均含量为3.09 mg/g。该方法简单、快速、重现性好。     

高效液相色谱-蒸发光散射检测法测定玉屏风胶囊中黄芪甲苷的含量

建立高效液相色谱-蒸发光散射检测法测定玉屏风胶囊中黄芪甲苷的含量.采用Phenomenex C18(4. 6mm×250 mm i. d. ,5μm)色谱柱,柱温为35℃,以乙腈-水(35∶65)为流动相,以蒸发光散射检测器进行检测.以峰面积的常用对数(Y)对进样量的常用对数(X)进行线性回归,回归方程为Y=1. 6709 X+14. 2699(r=0. 9998),线性范围为1～19μg.加标回收率为86. 7%～96. 2%,测定结果的RSD为0. 22%(n=7).方法准确、可靠、重复性好,可有效控制玉屏风胶囊的质量.     

南海短足软珊瑚Cladiella sp.中两个新孕甾醇苷的分离

从短足软珊瑚Cladiella sp．中,分离得到3个甾类化合物：孕甾-5,20-二烯-3β-醇-3-O-α-L-吡喃岩藻糖苷(1)、孕甾-5,20-二烯-3β-醇-3-O-β-D-吡喃木糖苷(2)和(22E,24R)-麦角甾-7,22-二烯-3β,5α,6β-三醇(3),其中1和2为新化合物．孕甾醇苷具有抗早孕和抑制肿瘤细胞生长活性．     

高效毛细管电泳安培法测定芦荟中芦荟苷的含量

建立了芦荟中芦荟苷含量的高效毛细管电泳安培检测方法. 探讨了缓冲溶液种类、浓度、酸碱度,工作电位,有机改性剂及其操作电压、进样时间等对检测的影响. Na2B4O7-NaOH(Na2B4O7浓度为30 mmol/L)为缓冲液,工作电位为-0.8 V,体积分数为2.5%甲醇为有机添加剂,进样时间为10 s,在15 kV分离高压,pH=9.5的碱性条件下柱端安培法检测了芦荟苷的含量. 该法的线性范围为50～0.05 mg/L,线性方程Y=856.2+123.3c,相关系数r=0.999 4,检出限为0.01 mg/L.     

Separation of acteoside and linarin from Buddlejae Flos by high‐speed countercurrent chromatography and their anti‐inflammatory activities

Buddleja officinalis Maxim., a deciduous, flowering shrub, is used as a traditional Chinese medicine; the bioactivity of B. officinalis is primarily due to flavonoids and phenylethanoid glycosides. In the study, acteoside and linarin were successfully isolated from B. officinalis by high‐speed countercurrent chromatography with a two‐phase solvent system composed of ethyl acetate: n‐butanol: water (5:0.8:5, v/v/v). The purities of acteoside and linarin were determined to be 97.3 and 98.2%, respectively, using one‐step high‐speed countercurrent chromatography separation. The chemical structures of the two compounds were identified by electrospray ionization‐mass spectrometry and nuclear magnetic resonance. After separation, the anti‐inflammatory effects of the two compounds were evaluated using lipopolysaccharide‐induced human umbilical vein endothelial cells. Acteoside and linarin inhibited the expression of nitric oxide, tumor necrosis factor α and interleukin 1β, which demonstrated that acteoside and linarin possessed anti‐inflammatory activity.     

Comparative pharmacokinetics of acteoside from total glycoside extracted from leaves of Rehmannia and Dihuangye total glycoside capsule in normal and diabetic nephropathy rats

Rehmannia glutinosa Libosch (RG), is officially listed in the Chinese Pharmacopoeia and is widely used in China. In this paper, a sensitive and rapid ultra‐performance liquid chromatography–mass spectrometry method including multiple‐reaction monitoring mode was developed and applied to study the pharmacokinetic effect of acteoside from total glycoside extracted from the leaves of Rehmannia (TLR) and Dihuangye total glycoside capsule (DTG) in normal and diabetic nephropathy rats. The diabetic nephropathy rat model was induced by intraperitoneal injection of a small dose of streptozotocin and high‐fat diet and plus 5% glucose drinking water. Samples of plasma of rats were obtained at different times after rats were administered TLR (7.2 g/kg) and DTG (360 mg/kg). After deproteinization by acetonitrile, the concentrations of acteoside in rats at different time points were detected by UPLC‐TQ‐MS method and pharmacokinetics parameters were calculated using DAS 3.2.8 software. A good linearity of acteoside was shown in the range of 8.51–3404.8 ng/m L (r ² = 0.9987). The mean extraction recovery of analyte was in the range of 63.55–79.49%, and the intra‐ and inter‐day RSD values were <8.8%. Compared with the normal group, the maximum plasma concentration, AUC_0–t , AUC_0–∞ and apparent plasma clearance corresponding dose in model group rats decreased significantly. After rats were administered TLR and DTG, the acteoside reached the maximum plasma concentration at about 15 min. The method proved to be simple, rapid and specific, and to be suitable for the determination of acteoside in plasma of diabetic nephropathy rats and pharmacokinetic study.     

气相色谱-质谱法测定富硒酵母中的硒蛋氨酸

建立了气相色谱-质谱（GC-MS）测定富硒酵母中硒蛋氨酸含量的方法。比较了3种从样品中提取硒蛋氨酸方法的效果。样品在三羟甲基氨基甲烷（Tris）缓冲液中酶解24 h后,以丁醇及三氟乙酸酐为衍生化试剂对硒蛋氨酸进行衍生化,采用选择离子模式对衍生物进行GC-MS测定。硒蛋氨酸的回收率为98.5%~103.7%,相对标准偏差为0.9%~2.4%,检出限为0.5 mg/L（S/N=3）。对实际样品进行测定,得到样品中硒蛋氨酸的含量结果。该法简便快速,准确可靠,灵敏度高。     

大孔树脂-高速逆流色谱法分离纯化地黄中毛蕊花糖苷

该文建立了大孔树脂-高速逆流色谱分离中药材地黄中有效成分毛蕊花糖苷的方法。考察了4种大孔树脂对地黄粗提物中毛蕊花糖苷的静态吸附与解吸情况,其中D101大孔树脂对目标成分的吸附率与解吸率最理想,实验结果表明体积分数为10%的乙醇洗脱得到的毛蕊花糖苷含量最高,目标成分含量从4.9%提高到32.6%。最后,部分纯化的样品（165 mg）采用高速逆流色谱进一步纯化,两相溶剂系统由乙酸乙酯-正丁醇-水（1：4：5,v/v/v）组成,分离得到45 mg纯度为96%的毛蕊花糖苷。     

Isolation and purification of acteoside and isoacteoside from Plantago psyllium L. by high-speed counter-current chromatography

Two isomeric phenylethanoid glycosides, acteoside and isoacteoside were isolated and purified from the seeds of Plantago psyllium L. for the first time by high-speed counter-current chromatography (HSCCC) using a solvent system consisting of ethyl acetate-water (1:1, v:v). By injecting 200 mg of the n-butanol extract of P. psyllium for five consecutive times, the two-step HSCCC procedure yielded a total of 165 mg of acteoside and 17.5 mg of isoacteoside from 978 mg extract. The recovery rates for acteoside and isoacteoside were 90 and 84%, respectively, and the purities were 98 and 94%, respectively. The HSCCC fractions were analyzed by HPLC and the structures were identified by UV, LC-APCI-MS in negative ion mode, and confirmed by NMR experiments.     

Separation of 2-naphthol atropisomers on cyclofructan-based chiral stationary phases

A set of fifteen 2-naphthol-derived atropisomers were evaluated on three different cyclofructan-based chiral stationary phases (CSP). The cyclofructan CSPs were a dimethylphenyl-derivatized cyclofructan 7 (CF7-DMP), a isopropyl (CF6-P) and a R-naphthylethyl cyclofructan 6 (CF6-RN) derivative, all bonded to 5-µm spherical fully porous silica particles packed into three 25?cm?×?4.6?mm columns (commercially available as Larihc columns). The 15 atropisomers were analyzed in the normal-phase mode with heptane/alcohol mobile phases. The CF7-DMP column was the most effective partially or fully separating 14 of the 15 compounds (93%). All 15 compounds could be separated by at least one cyclofructan column. Five compounds could be partially or fully separated by all three CSPs. The effect of ethanol, 2-propanol and butanol as 5 and 10% v/v polar modifiers in heptane was studied. A prototype 15?cm?×?4.6?mm column packed with superficially porous 2.7?µm CF6-P bonded particles was tested with the same set of compounds and a standard HPLC system. The increased efficiency and solvent saving were significant.     

Simultaneous determination of three opiates in serum by micellar liquid chromatography using direct injection

A simple and reliable micellar liquid chromatographic method was developed for the simultaneous determination of 3 opiates (codeine, morphine, and thebaine) in serum, using direct injection and ultraviolet detection. The separation of the drugs was optimized on a C18 column, thermostatically controlled at 25 degrees C, by evaluating mobile phases containing sodium dodecyl sulfate (SDS) and various modifiers (propanol, butanol, or pentanol). Adequate resolution of the opiates was obtained with a chemometrics approach, in which retention was modeled as a first step by using the retention factors for several mobile phases. Next, an optimization criterion that takes into account the position and shape of the chromatographic peaks was applied. The 3 opiates were totally resolved and determined in 12 min with the mobile phase 0.15M SDS-7% (v/v) butanol buffered at pH 7. The limits of detection for codeine and morphine were greatly improved by using fluorimetric detection. Repeatability and intermediate precision were tested for 3 different concentrations of the drugs, and the relative standard deviations were <0.8% for most of the assays. Finally, the method was successfully applied to the determination of morphine and codeine in serum samples.     

A consecutive preparation method based upon accelerated solvent extraction and high‐speed counter‐current chromatography for isolation of aesculin from Cortex fraxinus

A consecutive preparation method based upon accelerated solvent extraction (ASE) coupled with high‐speed counter‐current chromatography (HSCCC) was presented and aesculin was obtained from Cortex fraxinus. The extraction condition of ASE was optimized with response surface methodology; some significant parameters such as the solvent system and its stability, the amount of loading sample in HSCCC were also investigated. The original sample was first extracted with methanol at 105°C and 104 bar for 7 min using ASE, then the extracts were consecutively introduced into the HSCCC system and separated and purified with the same ethyl acetate/n‐butanol/water (7:3:10, v/v/v) solvent system for five times without further exchange and equilibrium. About 3.1 ± 0.2 mg/g in each time and total of 15.4 mg/g aesculin with purity over 95% was isolated from Cortex fraxinus. The results demonstrated that the consecutive preparation method was time and solvent saving and high throughput, it was suitable for isolation of aesculin from Cortex fraxinus, and also has good potential on the separation and purification of effective compounds from natural product.     

Analysis of isoquinoline alkaloids using chitosan‐assisted liquid–solid extraction followed by microemulsion liquid chromatography employing a sub‐2‐micron particle stationary phase

A simple, efficient, and green chitosan‐assisted liquid–solid extraction method was developed for the sample preparation of isoquinoline derivative alkaloids followed by microemulsion LC. The optimized mobile phase consisted of 0.8% w/v of ethyl acetate, 1.0% w/v of SDS, 8.0% w/v of n‐butanol, 0.1% v/v acetic acid, and 10% v/v ACN. Compared to pharmacopoeia method and organic solvent extraction, this new approach avoided the use of volatile organic solvents, replacing them with relatively small amounts of chitosan. Under the optimum conditions, good linearity (r² > 0.9980) for all calibration curves and low detection limits between 0.05 and 0.10 μg/mL were achieved. The presented procedure was successfully applied to determine alkaloids in Rhizoma coptidis with satisfactory recoveries (81.3–106.4%).     

液相色谱-电喷雾串联质谱法测定生姜中的215种农药残留

建立了生姜中215种农药多残留测定的液相色谱-电喷雾串联质谱(LC-ESI-MS/MS)方法。样品用1%醋酸-乙腈溶液均质提取,经Sep-Pak Vac固相萃取柱净化,乙腈-甲苯(3:1, v/v)洗脱,旋转蒸发浓缩至约0.5 mL后,于室温氮气吹干,用乙腈-水(3:2, v/v)溶解,以电喷雾电离串联质谱在正离子多反应监测(MRM)模式下进行测定。在定量限水平进行添加回收率实验,方法的回收率范围为68.1%～132.6%,其中回收率在70%～120%的占94.4%,相对标准偏差(RSD)范围为0.4%～25.0%。方法的检出限(S/N=3)和定量限(S/N=10)范围分别为0.01～70.45 μg/L和0.04～234.84 μg/L。该方法操作简便,灵敏度、准确度和精密度均符合农药多残留检测技术要求,适用于生姜中215种农药多残留的快速测定。