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胶束毛细管电泳在线扫集技术同时分离测定穿心莲内酯和脱水穿心莲内酯的研究 总被引:1,自引:0,他引:1
采用胶束毛细管电泳在线扫集技术分离测定了中药穿心莲中脱水穿心莲内酯和穿心莲内酯.电泳条件:以20 mmol/L H3BO310 mmol/L NaH2PO4-50mmol/L SDS(含体积分数20%甲醇,pH 2.4)为电泳运行缓冲溶液,未涂层石英毛细管(58 cm×50 μm i.d.,有效长度为41.2 cm)为分离通道,重力进样,进样高度为11 cm,-20 kV恒压,检测波长为246 nm.富集倍数可以达到200倍以上.在5.70~91.20 mg/L,和3.96~31.68 mg/L范围内呈良好的线性关系,对两种内酯分别进行了定量分析.加标平均回收率脱水穿心莲内酯为100.80%,穿心莲内酯为98.06%. 相似文献
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建立了人尿中马尿酸和甲基马尿酸的毛细管电泳同时测定方法。尿样经乙酸乙酯提取,N2流挥干,硼砂-乙腈缓冲液溶解后毛细管电泳法分析。熔融石英毛细管(50 cm×50μm,有效长度41 cm,未涂层)为分离柱;20 mmol/L的硼砂+20%乙腈(pH 9.3)为运行缓冲液,紫外检测波长为230 nm,电泳分离温度为20℃,分离电压为20kV,重力进样高度20 cm,进样时间为10s。在优化的条件下,马尿酸和甲基马尿酸质量浓度在2~50 mg/L范围内具有良好的线性关系,线性相关系数分别为0.9998和0.9994,检出限分别为0.26和0.20 mg/L,加标回收率分别为100.7%~115.5%及93.3%~116.7%。本法适合于尿中马尿酸和甲基马尿酸的同时快速测定。 相似文献
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以手性冠醚为胶束毛细管电泳手性分离选择剂,对吉米沙星对映体药物的在线富集分离进行了研究.考察了阳离子表面活性剂十二烷基三甲基溴化铵浓度、运行缓冲溶液中有机添加剂含量和进样方式对对映体的富集和分离度的影响.使用未涂层毛细管柱(37 cm×51 μm,有效柱长30 cm),45 mmol/L Bis-Tris缓冲液+10 mmol/L十二烷基三甲基溴化铵(DTAB)+1 mmol/L手性冠醚+11%乙腈为运行缓冲溶液(pH=4.0),在紫外检测波长280 nm、运行电压-10 kV、电动进样条件下,对吉米沙星对映体进行在线推扫(sweeping)富集分离,在基线分离的前提下,富集倍数可达600~700倍.吉米沙星浓度为0.3 μmol/L时,两对映体峰高的相对标准偏差<4.0%(n=7).本方法为毛细管电泳在痕量对映体药物分析等方面的应用提供了新方法. 相似文献
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为建立一种快速分离白花丹参水溶性有效成分的毛细管区带电泳体系,分别考察了缓冲液浓度、缓冲液pH、运行电压、检测波长对样品的分离度、迁移时间等因素的影响。最终优化的分离条件为:5 mmol/L硼砂缓冲液(pH 7.5);毛细管柱75 μm×60.2 cm,有效长度50 cm,压力进样(3.45 kPa×4 s),27.5 kV恒压分离,210 nm波长下检测,柱温25 ℃。在优化的条件下,8 min内使白花丹参样品中的原儿茶醛、丹参素、原儿茶酸组分达到完全基线分离。 相似文献
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胶束扫集毛细管电泳分离测定绿原酸和咖啡酸 总被引:1,自引:0,他引:1
采用胶束扫集毛细管电泳分离测定双黄连口服液中的绿原酸和咖啡酸.试验条件为:重力进样时间40 s;以20 mmol/L NaH_2PO_4,100 mmol/L 十二烷基磺酸钠(SDS)为电泳缓冲液(含体积分数15%甲醇,pH 2.20),分离电压-20 kV,检测波长214 nm,讨论了pH、SDS浓度、样品溶剂等对分离效果的影响.在优化条件下,绿原酸和咖啡酸的检出限分别达到1.02和0.168 μg/mL,线性范围分别为5.86~51.5 μg/mL和1.27~14.5 μg/mL. 相似文献
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毛细管区带电泳法快速测定消毒剂中苯扎溴铵的含量 总被引:4,自引:0,他引:4
采用毛细管区带电泳法(CZE)测定了复方消毒剂中苯扎溴铵的含量。以乙腈-50 mmol/L磷酸二氢钠(pH 2.24)(体积比为50∶50)为背景电解质,以46.4 cm×75 μm i.d.未涂敷的毛细管为色谱分离柱,于214 nm波长检测。详细研究了影响苯扎溴铵准确定量的因素,如缓冲溶液的浓度、pH值、毛细管清洗方式等。样品仅需简单的稀释即可直接进样。采用峰面积外标法定量。方法的检出限为0.2 mg/L(S/N=3),线性范围为20-400 mg/L,苯扎溴铵峰迁移时间的相对标准偏差(RSD)为0.6 相似文献
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高效毛细管电泳安培法测定芦荟中芦荟苷的含量 总被引:1,自引:0,他引:1
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. 相似文献
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Separation of nucleosides using capillary electrochromatography 总被引:1,自引:0,他引:1
The analysis of nucleosides and nucleotides have in most cases been performed by HPLC using either reversed-phase HPLC with gradient elution or using reversed-phase ion-pair chromatography. In this paper we have explored the possibility of using capillary electrochromatography (CEC) in order to avoid the use of gradients or ion-pairing reagents. CEC is in many ways comparable to HPLC, but CEC is theoretically able to provide better separations due to the higher efficiency caused by the flowfront being more plug-like as also is the case in CE, which is to be compared to the more parabolic flow observed in HPLC. The separation of six nucleosides (adenosine, cytidine, guanosine, inosine, thymidine and uridine) was investigated with respect to concentration of buffers, pH, amount of acetonitrile, temperature and voltage in order to optimise the separation. Baseline separation was achieved for the six nucleosides in less than 13 min using a background electrolyte consisting of (5 mM acetic acid, 3 mM triethylamine, pH 5.0)-acetonitrile (92:8, v/v). 相似文献
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Determination of nucleosides in natural Cordyceps sinensis and cultured Cordyceps mycelia by capillary electrophoresis 总被引:7,自引:0,他引:7
Cordyceps sinensis is a well-known traditional Chinese medicine, and some of the active components are nucleosides. The analysis of nucleosides in Cordyceps material has been performed by reversed-phase high-performance liquid chromatography (HPLC) with gradient elution or by spectrometry. Here, we have explored the possibility of using capillary electrophoresis to determine the content of three major nucleosides (adenosine, guanosine and uridine) in Cordyceps. Capillary electrophoresis needs no gradients, and it provides a better separation due to its higher efficiency. In order to optimize the resolution, the separation of adenosine, guanosine and uridine was determined in Cordyceps with respect to the variation of buffer concentration, pH, temperature, and voltage. By using the calibrated electrophoresis system, the separation was achieved for the three nucleosides in less than 10 min with a background electrolyte consisting of 0.2 M boric acid-sodium hydroxide buffer, pH 8.5. The nucleoside contents of various types of natural Cordyceps and cultured Cordyceps mycelia were determined and compared. There was a great variation of nucleoside content in different sources of Cordyceps; the cultured Cordyceps mycelia, however, contains a much higher concentration than the natural Cordyceps. 相似文献
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The electrochromatographic separations of 2'-, 3'- and 5'-monophosphates of adenosine, guanosine, cytidine, and uridine were carried out with an open-tubular capillary column which was wall-coated with a highly selective reagent, 28-membered macrocyclic polyamine, 4, 8, 12, 18, 22, 26-hexaaza-1,15-dioxacyclooctaeicosane ([28]ane-N6O2). The effects of pH, composition and concentration of background electrolyte (BGE), applied voltage, column length, and the additive of the BGE, such as metal ions, borate, beta-cyclodextrin and organic solvent on the separation of these monophosphorylated nucleotide isomers were investigated. The results suggested that the interactions between analytes and the bonded groups on the wall predominantly comprise anion coordination and anion exchange in addition to the electrophoresis. A well-resolved electrochromatogram was obtained with the capillary column of 100 cm (75 cm effective length) x 75 microm inside diameter (ID), citrate buffer (20 mM, pH 3.99), applied voltage of -22 kV and detection at 254 nm. Column efficiency was found with the average theoretical plate numbers of 119,500/m and a low detection limit of 0.01 microM level could be achieved for the separation of these isomers. 相似文献
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建立了消毒剂中活性成分醋酸氯己定(又名:醋酸洗必泰)的毛细管电泳快速检测法。采用15 mmol/L磷酸盐-乙腈(
体积比为60∶40)缓冲体系,将醋酸氯己定在50 cm×75 μm i.d.的石英毛细管柱中进行电泳分离,电泳电压为15 kV,检
测波长为254 nm。同时,对毛细管电泳分析醋酸氯己定的条件(如缓冲液的种类、pH值、浓度及电泳电压等)进行了优化
。用该方法对消毒剂样品进行测定,在4 min内可完成分析。醋酸氯己定在质量浓度为0.01~0.10 g/L时线性良好,检测
限为0.004
mg/L,吸光度值的相对标准偏差为3.97%,迁移时间的相对标准偏差为2.99%,样品加标回收率为91.4%~116.6%。将该方法
与高效液相色谱法进行比较,两种方法测定结果的相对误差≤4%。所建立的检测醋酸氯己定含量的毛细管区带电泳法简单
、快速,适用于消毒剂样品的测定。 相似文献
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An open-tubular wall-coated macrocyclic polyamine capillary column (70 cm x 75 microm ID) with 50 cm effective length for the separation of nucleoside monophosphates is described. Some parameters with respect to concentration, pH, composition of the buffer, and voltage in order to optimize the separation were studied. The coated capillary showed reversed electroosmotic flow (EOF), allowing anions to be separated in the co-EOF mode. Baseline separations were achieved for the eight nucleotides in less than 26 min using a background electrolyte consisting of H(3)PO(4)-NaH(2)PO(4) (30 mM, pH 3.10), an applied voltage of -15 kV, and detection at 254 nm. The macrocyclic polyamine on the capillary wall introduced anion coordination for the interaction with the analytes, the strength of which could be moderated by the type and concentration of the competing ion used in the background electrolyte (BGE). With a low concentration of the competing ion (phosphate ion), the migration behavior followed that obtained in the electrophoretic system. Increasing the concentration of the competing ion resulted in a faster migration and more complete elution of the analyte. The method established was also employed for the analysis of nucleotides in mushrooms. Aqueous extracts of mushrooms from different species and various extraction methods were injected directly for the analysis. Uridine 5'-monophosphate, guanosine 5'-monophosphate, adenosine 5'-monophosphate, and cytidine 5'-monophosphate, were found in the sample tested. 相似文献
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Determination of scopolamine, atropine and anisodamine in Flos daturae by capillary electrophoresis.
A capillary electrophoresis method was developed for the separation and determination of tropane alkaloids in Flos daturae plants. Separation was performed on a fused silica capillary(42.1 cm x 50 microm i.d.) at an applied voltage of 20 kV. Scopolamine, atropine and anisodamine were well separated in the buffer of 50 mmol/L phosphate buffer (pH 5.0) containing 20% (v/v) tetrahydrofuran (THF). Beer's law was obeyed in the range of concentration of 2.4-21.8 microg/mL for scopolamine, 4.0-36.0 microg/mL for atropine and 2.6-23.7 microg/mL for anisodamine, respectively, and the correlation coefficients were over 0.999 (n = 6). The developed method was applied for the analysis of herb samples. 相似文献
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应用毛细管区带电泳法测定分别以冬虫夏草菌丝体粉和鹿茸血为主要原料制品中的多种核苷和碱基成分。对实验条件进行了优化,结果表明,以20mmol/L硼砂-15mmol/Lβ-环糊精为缓冲溶液(pH=9.4),分离电压22kV,检测波长254nm,电动进样为10kV、5s时,在10min内同时分离测定了虫草素、腺嘌呤、鸟嘌呤、尿嘧啶、腺苷、次黄嘌呤、尿苷、鸟苷和肌苷。各组分在0.2~200μg/mL范围内呈线性关系,检出限的范围是0.07~1.67μg/mL。5个批次的冬虫夏草菌丝粉保健品中腺嘌呤、尿嘧啶、腺苷、鸟苷、尿苷5组分的定量结果分别在0.15~0.19mg/g、0.72~0.92mg/g、1.44~1.59mg/g、1.51~2.32mg/g和1.77~2.56mg/g范围内,加标回收率的范围是82.83%~109.21%;2个批次的鹿茸血保健品中次黄嘌呤、尿苷的定量结果在36.55~49.97μg/mL和86.08~108.97μg/mL范围内,加标回收率的范围分别是89.68%~96.79%和99.05%~102.81%。 相似文献
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A practical NACE method was developed for simultaneous determination of three adenosine monophosphate (AMP) isomers. Separation of three AMP isomers was achieved using 200 mM Tris/H(3)BO(3) in acetontrile/water (2:1 v/v) at pH* 10.0 as the running buffer and +25 kV as the applied voltage over a bare fused-silica capillary of 50 microm id x 375 microm od x 54.5 cm (46 cm to the detector window). At 260 nm, the calibration curves were linear in the range of 1-100 microg/mL. The detection limits were less than 0.70 microg/mL. The recovery ranged from 94.5 to 106.4%. The intraday RSDs of the migration times were between 2.1 and 3.0%. The developed NACE method has been successfully applied for the determination of three AMP isomers in the real samples of biomimicking prebiotic synthesis reaction between N-(O,O-diisopropyl) phosphoryl amino acid and adenosine. 相似文献
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Franco Cataldo 《Journal of Radioanalytical and Nuclear Chemistry》2018,318(3):1649-1661
The RNA nucleosides, namely adenosine, cytidine, guanosine and uridine were γ-radioyzed in solid state and in vacuo at room temperature to a total dose of 3.2 MGy. Through electronic absorption spectroscopy, differential scanning calorimetry and through polarimetry and optical rotatory dispersion spectroscopy, it was found that the purine-based nucleosides (adenosine and guanosine) show a much higher radiolysis resistance than the pyrimidine-based nucleosides (cytidine and uridine). In an astrochemical/astrobiological context, these results may explain why purine nucleobases are found in practically all carbonaceous chondrite meteorites while the pyrimidine nucleobases are absent or below the detection limits of the current analytical techniques. In the hypothesis that both purines and pyrimidines nucleobases were present in certain bodies at the beginning of the solar system 4.6?×?109 years ago, the radiolysis due to radionuclides decay has destroyed more easily and completely the pyrimidine bases due to their much lower radiolysis resistance than the purine bases. 相似文献