共查询到19条相似文献,搜索用时 173 毫秒
1.
采用动态pH联接-扫集毛细管电泳法对化妆品中的迷迭香酸进行检测。用重力进样的方式,进样高度为15 cm的情况下,研究了硼砂浓度、pH、十二烷基硫酸钠(SDS)浓度、甲醇浓度、样品基体、进样时间、分离电压对富集与分离的影响。优化后的实验条件:15 mmol/L硼砂-45 mmol/L SDS(pH8.8)-15%甲醇为缓冲液,进样时间60s,分离电压16kV,样品中磷酸盐浓度10 mmol/L,样品基质pH 4.7。在上述条件下,迷迭香酸(RA)的线性回归方程式为y=539200ρ+53588(r=0.9985),线性范围为0.144~3.6μg/mL,检出限0.036μg/mL,迷迭香酸的回收率为92.5%~103%,相对标准偏差为2.5%。 相似文献
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建立了胶束毛细管电动色谱在线富集技术测定药品中痕量的泼尼松的方法。在胶束扫集的基础上联用场放大进样,使泼尼松的富集倍数提高了136倍;检出限由原来的2.7mg/L降至20μg/L。胶束扫集毛细管电泳缓冲体系为120mmol/LSDS、10mmol/LNaH2PO4(pH2.5)10%乙腈(V/V)。分离电压-20kV,进样电压-20kV,进样时间70s,进水时间180s,检测波长250nm。同时讨论了SDS浓度、样品基质pH、进样电压、进水时间和进样时间对分离效果的影响。实验结果显示:在优化实验条件下,样品的检测仅需8min,泼尼松在0.05~10mg/L的范围内线性关系良好(r=0.998)。回收率在89.4%~106%之间,相对标准偏差在2.1%~2.6%之间,可用于各种中药制剂中泼尼松的含量测定。 相似文献
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联用阴离子选择性耗尽进样和胶束扫集两种在线富集技术,建立了胶束毛细管电泳方法测定化妆品中醋酸氢化可的松的方法。讨论了SDS浓度、样品基体、进样电压、进水时间和进样时间对富集和分离的影响。优化的实验条件:以120 mmol/L SDS-20 mmol/L NaH2PO4(pH2.2)-10%(体积分数)甲醇为缓冲体系,分离电压-20 kV,进样电压-20 kV,进样时间80 s,进水时间200 s,测量波长250 nm。在该实验条件下,醋酸氢化可的松的富集倍数比普通毛细管电泳法提高了约173倍。方法的线性范围为0.05~5.0 mg/L,检出限为12.6μg/L。该方法用于化妆品中醋酸氢化可的松含量的测定,回收率为98%~105%,相对标准偏差均小于4.0%(n=4)。 相似文献
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毛细管电泳分离莽草酸及其对映体 总被引:1,自引:0,他引:1
采用毛细管电泳分离莽草酸及其对映体.试验了缓冲溶液的种类、浓度、pH值、分离电压、进样时间、添加剂对分离的影响.结果表明:以30 mmol·L-1三(羟甲基)氨基甲烷-30 mmol·L-1 H3BO3(pH 8.6)为缓冲体系,在波长214 nm,分离电压为15 kV,进样时间为10 s的条件下,实现了对莽草酸及其对映体的分离. 相似文献
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建立了以三联吡啶钌为发光体系的毛细管电泳电化学发光(CE-ECL)检测系统,并应用于分离和测定西咪替丁片剂中西咪替丁的含量。考察了检测电位,三联吡啶钌(Ru(bpy)32+)的溶液浓度,缓冲液的pH和溶液浓度,分离电压、进样电压与进样时间等因素对分离检测的影响。结果表明:在检测电位1.18V,Ru(bpy)32+溶液浓度为5 mmol/L,磷酸盐缓冲液(PBS)25 mmol/L(pH 7.8),进样时间10 s,进样电位10 kV,运行电位15 kV下,测得西咪替丁线性范围为2.8×10-6~4.0×10-4mol/L,检出限为1.2×10-7mol/L(S/N=3)。对1.0×10-5mol/L的西咪替丁标准溶液连续测定5次,电化学发光强度和迁移时间的RSD分别为3.9%和1.5%。方法已应用于西咪替丁片剂中西咪替丁含量的测定。 相似文献
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毛细管电泳电致化学发光法同时测定氯丙嗪、异丙嗪及其主要代谢物 总被引:3,自引:0,他引:3
建立了同时检测氯丙嗪、异丙嗪及其主要代谢物的毛细管电泳电致化学发光新方法。最佳实验条件为: 检测电位1.20 V,钌联吡啶浓度5 mmol/L,检测池磷酸缓冲溶液40 mmol/L (pH 6.5),分离磷酸缓冲溶液18 mmol/L (pH 4.8),进样电压11 kV,进样时间8 s,分离电压13.5 kV。方法的检出限(3σ)分别为氯丙嗪8.3×10~7 g/L、异丙嗪7.2×10~6 g/L、氯丙嗪亚砜1.9×10~5g/L和异丙嗪亚砜3.7×10~6g/L,各组分的电化学发光强度和迁移时间的相对标准偏差(RSD)分别不超过3%和1%。本方法具有简便、快速、灵敏、进样量少和不受共存物干扰等特点,可在不必预分离的情况下直接同时连续测定家犬尿样中的氯丙嗪、异丙嗪、氯丙嗪亚砜和异丙嗪亚砜。 相似文献
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托吡卡胺对映体的毛细管电泳-方波安培分离检测 总被引:2,自引:0,他引:2
采用毛细管电泳-方波安培检测法,在熔融石英毛细管(75 μm i.d.×50 cm)中,以7 mmol/L 三羟甲基氨基甲烷(Tris)-10 mmol/L柠檬酸-2 mmol/L硼酸-15mmol/L β-环糊精 (β-CD) (pH 3.0)为电泳介质,采用重力进样,高度差为20 cm,进样时间为10 s,在分离电压为15 kV,方波平衡电位+0.8 V的条件下,实现了托吡卡胺对映体的分离检测。线性范围为5~750 μmol/L,检出限为2 μmol/L。对影响分离度的因素β-CD浓度、硼酸浓度及p 相似文献
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基于微流控芯片-激光诱导荧光分析技术,探讨了奶酪中两种β-酪啡肽(β-CM-5和β-CM-7)的场放大进样富集和检测。采用10 mmol/L硼酸-硼砂溶液(pH8.7)作为衍生缓冲液,5 mmol/L硼砂溶液(pH8.9)作为样品缓冲液,进样10s,60 mmol/L硼砂溶液(pH8.9)作为运行缓冲液,分离电压1500V,在120s内成功分离检测了两种β-酪啡肽。实验结果表明,β-CM-5和β-CM-7的富集倍数是16倍和21倍,检出限分别是8.2 nmol/L和3.6 nmol/L,线性范围分别是0.05~2μmol/L和0.02~1μmol/L,加标回收率在86.9%~107.5%,该方法可应用于奶制品中β-CM-5和β-CM-7的含量测定。 相似文献
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建立了毛细管区带电泳(CZE)在线富集3种肌肽类活性肽(肌肽、鹅肌肽和高肌肽)的两种简便有效的方法。一种是大体积进样反向压力排除基体富集(LVSRP)技术,即通过流体动力学进样,在不改变电源极性的条件下,利用反向压力排除样品基体,电堆积富集后进行CZE分离;另一种是大体积进样电渗流排除基体富集(LVSEP)技术,即通过流体动力学进样,于运行缓冲液中加入溴化十六烷基三甲基铵(CTAB)动态修饰毛细管表面,通过电渗流排除样品基体,改变电源极性后进行CZE分离。与常规CZE相比,LVSRP技术和LVSEP技术使检测灵敏度提高了40~60倍。对影响两种富集过程的一些因素进行了研究,在最优富集条件下考察本方法的线性范围为0.080~5.0 μmol/L。对3种生物活性肽的检测限(S/N=3)分别为LVSRP 41~58 nmol/L,LVSEP 35~43 nmol/L。 相似文献
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采用建立在移动反应界面理论上的体系进行尿样中氧化苦参碱的富集与定量检测。与传统的毛细管电泳相比,体系中引入了富集缓冲溶液(富集相)和分离缓冲溶液(分离相)。优化的条件如下:样品缓冲溶液为20 mmol/L 甲酸钠(用氨水调节pH至10.70),富集缓冲溶液为40 mmol/L 甲酸-甲酸钠(pH 2.60),分离缓冲溶液为100 mmol/L 甲酸-甲酸钠(pH 4.80);样品相压力进样1.4 kPa×3 min,富集相压力进样1.4 kPa×7 min,紫外检测波长210 nm,电压21 kV。氧化苦参碱在2.2~65 mg/L的质量浓度范围内呈良好的线性关系(r=0.9991),检出限为0.74 mg/L,灵敏度比常规毛细管电泳方法提高约70倍,重现性良好。该方法已经成功地应用于尿样中氧化苦参碱的检测。 相似文献
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利用胶束电动色谱测定胡黄连中的香草酸、肉桂酸和阿魏酸;在联用场放大进样后,富集倍数提高30倍以上,检出限降至3.6μg/L,线性范围向下延伸到14μg/L。胶束扫集电动色谱缓冲体系为100mmol/L十二烷基磺酸钠(SDS)+20mmol/L磷酸钠(pH=2.20)+15%甲醇,分离电压-20kV。进样电压-8kV,进样时间20s,进水时间160s(H=20.0cm),测量波长214nm。考察了SDS浓度、进样长度、进样电压等对分离效果的影响。在优化条件下,3种有机酸在10min内出峰,峰面积相对标准偏差(RSD)≤5.9%。方法检出限、线性范围、相关系数分别为:香草酸3.6μg/L、14~460μg/L、0.9996;肉桂酸9.8μg/L、20~310μg/L、0.9994;阿魏酸11μg/L、22~180μg/L、0.9996。回收率为95.4%~107%。 相似文献
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Hai-Yan Feng Shu-Rong Hou Na Zheng Xiang-Jun Li Zhong-Bo Hu Zhuo-Bin Yuan 《Chromatographia》2008,68(5-6):431-435
A rapid capillary electrophoresis method based on online acid barrage stacking has been successfully established for analysis of trace amounts of genistein in human plasma. Genistein was analyzed within 8 min, with 200 mmol L?1 citric acid (pH 1.7) as acid barrage, and injection times of 180 and 30 s for sample and acid, respectively. Good linearity was obtained in the range 0.05–5 mg L?1 and the limit of detection was 0.03 mg L?1. Compared with normal sample injection, this method resulted in more than a fiftyfold improvement in detection sensitivity. The technique has potential for use in studies of genistein metabolism and of exposure levels in humans. 相似文献
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利用高压电容耦合非接触电导检测器(HV-C4D),结合毛细管电泳场放大进样(FASS),以2-N-吗啡啉乙磺酸(MES)/组氨酸(His)为缓冲溶液,电泳分离测定了Zn2+.考察了样品溶液中MES/His的浓度及电动进样时间对场放大浓缩因子及缓冲溶液浓度对检测灵敏度的影响.在10mmol/LMES/His(pH=4.9)的分离缓冲溶液中,FASS对Zn2+的浓缩因子为1.3×103.Zn2+的浓度在10~1000nmol/L范围内与峰面积有良好线性关系(R=0.9995),检测限为5nmol/L(S/N=3).该方法可用于痕量Zn2+的测定. 相似文献
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Yuanqi Lu Hong Bai Chunyan Kong Hao Zhong Michael C. Breadmore 《Electrophoresis》2013,34(24):3326-3332
A method was developed to determine brazilin and protosappanin B in natural products by CE after acid barrage stacking. The optimum conditions were as follows: a BGE of 20 mM sodium tetraborate (pH 9.2) containing 6% v/v of methanol, hydrodynamic injection (0.5 psi, 65 s) followed by hydrodynamic injection of 150 mM citric acid (pH 2.3; 0.5 psi, 22 s), and separated with +25 kV. Under these conditions, brazilin and protosappanin B were separated with a sample‐to‐sample time less than 13 min and detection limits of 0.28 μg/mL and 0.15 μg/mL, respectively. The applicability of the developed method was demonstrated by the detection of brazilin and protosappanin in methanol extract of sappan lignum. 相似文献
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A highly sensitive method for enantioseparation of trace fenoprofen and amino acid derivatives by capillary electrophoresis (CE) with vancomycin as the chiral selector was developed. Several CE techniques, such as the partial filling, large-volume sample stacking with EOF as pump plus anion-selective exhaustive injection (LVSEP-ASEI) were involved in the present method to improve the detection sensitivity. With on-column concentration, enantioseparation of racemic fenoprofen and six 9-fluorenylmethyl chloroformate (FMOC)-amino acid derivatives (at the concentration level of ng/mL) with the background electrolyte composed of 100 mmol/L Tris-H(3)PO(4) (pH 6.0) and 2 mmol/L vancomycin was detected readily with the UV detection at 214 nm. Successfully performing LVSEP-ASEI needs a very low EOF that could be depressed by coating the capillary with poly(dimethylacrylamide) solution. The coating also played a role to minimize the adsorption of vancomycin onto the capillary wall. Effect of the injected sample volume and the electrokinetic injection time on the peak area of the enantiomers and their resolution factor were investigated and optimized. Under the optimized conditions, more than 1000-fold enhancement in detection sensitivity compared with the normal injection was achieved. 相似文献
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A capillary electrophoresis-acid barrage stacking online enrichment method has been established to detect the four isoflavones which are Daidzein, Genistein, Formononetin, and Biochanin A. The proposed method was optimized using a single factor alternative method, and the optimal conditions obtained from the optimization were: the BGE was 25 mM borax and 2 mM β-cyclodextrin, the applied separation voltage was 20 kV, and the detection wavelength was 260 nm. The time ratio of the injection of sample and the injection of acid was 150 s:20 s, and the acid used was 250 mM acetic acid. The sample solvent used was 60% v/v acetonitrile. The established method had the enrichment factor of these four isoflavones at 24.5, 32.0, 29.2, and 33.7, respectively, LOD and LOQ are as low as nanograms per milliliter. Finally, the CE-acid barrage stacking method was successfully applied to the determination of four isoflavones in rat plasma and red clover extract, verifying the applicability and feasibility of the method. 相似文献
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The separation of three common anabolic steroids (methyltestosterone, methandrostenolone and testosterone) was performed for the first time by capillary EKC. Different charged CD derivatives and bile salts were tested as dispersed phases in order to achieve the separation. A mixture of 10 mmol/L succinylated-beta-CD with 1 mmol/L beta-CD in a 50 mmol/L borate buffer (pH 9) enabled the separation of the three anabolic steroids in less than 9 min. Concentration LODs, obtained for these compounds with low absorption of UV light, were approximately 5 x 10(-5) mol/L. The use of online reverse migrating sample stacking with large-volume injection (the effective length of the capillary) enabled to improve the detection sensitivity. Sensitivity enhancement factors (SEFs) ranging from 95 (for testosterone) to 149 (for methyltestosterone) were achieved by single stacking preconcentration. Then, the possibilities of multistep stacking to improve the sensitivity for these analytes were investigated. SEFs obtained by double stacking preconcentration ranged from 138 to 185, enabling concentration LODs of 2.79 x 10(-7) mol/L (for methyltestosterone), 3.47 x 10(-7) mol/L (for testosterone) and 3.56 x 10(-7) mol/L (for methandrostenolone). Although online triple stacking preconcentration was achieved, its repeatability was very poor and SEFs for the studied analytes were not calculated. 相似文献