多肽的反相梯度加压毛细管电色谱分离

以C18为固定相，采用电压和压力联合驱动流动相，研究反相加压毛细管电色谱分离多肽；考察了加压电色谱中，电压对带电和中性物质迁移的影响，实现了梯度加压毛细管电色谱分离6种多肽；结果表明，加压电色谱可以很好地抑制气泡形成，实验结果准确，重复性好；梯度加压毛细管电色谱在复杂样品的分离分析中，具有很大的潜力。     

强阳离子交换毛细管液相色谱-反相加压毛细管电色谱二维系统的构建及其在中药黄柏提取物分离中的应用

加压毛细管电色谱(pCEC)具有电泳和液相色谱的双重分离机理,其柱效高、选择性强、分辨率高和分离速度快并可进行梯度洗脱。我们在此基础上加入离子交换色谱模式,构建了强阳离子交换-反相加压毛细管液相色谱(micro strong cation exchange liquid chromatography/reversed phase pressurized capillary electrochromatography, μ-SCXLC/RP-pCEC)二维系统,并对中药黄柏的提取物进行了优化分离。第一维μ-SCXLC采用线性盐梯度分离,样品被切割成11个馏分洗脱收集后进入第二维,第二维脱盐后,采用RP-pCEC进行分离分析,梯度洗脱。以中药黄柏提取物为样品,此二维系统的分辨率和峰容量都较一维系统有很大提高,理论峰容量可达900左右,证明构建的二维体系非常适合复杂样品的分离分析。     

梯度加压毛细管电色谱分离蛋白质

 以1.5 μm无孔硅胶颗粒(non-porous silica,NPS)为固定相,采用电压和压力联合驱动流动相,用反相梯度加压毛细管电色谱(p-CEC)在7.5 min内实现了核糖核酸酶A、细胞色素C、溶菌酶和肌红蛋白等4种蛋白质的快速、高效的分离。比较了梯度加压毛细管电色谱和微柱液相色谱(μ-HPLC)分离蛋白质的结果,同时考察了固定相、离子对试剂三氟醋酸(TFA)浓度和电压等条件对梯度加压毛细管电色谱分离蛋白质的影响。结果表明,梯度p-CEC可以通过调节电压精细调节带电溶质的保留,提高分离选择性,缩短分离时间,得到较高的柱效。该方法在蛋白质分离分析及蛋白质组学的研究中具有很大的应用潜力，为高效快速地分离蛋白质开辟了新的途径。     

吉培福林对映体的毛细管电色谱分离

在碱性条件下合成了单(六-氧-甲基丙烯酸酯)-β-环糊精(CD),以甲基丙烯酸甘油酯(GMA)和单(六-氧-甲基丙烯酸酯)-β-CD为单体,乙二醇二甲基丙烯酸酯(EDMA)为交联剂,2-丙烯酰胺基-2-甲基-1-丙磺酸(AMPS)用来产生电渗流,正丙醇和1,4-丁二醇为制孔剂,偶氮二异丁腈(AIBN)为引发剂,在内径100 μm的毛细管内原位聚合制得了手性毛细管电色谱整体柱.采用制得的手性整体柱,在加压毛细管电色谱(pCEC)模式下,对吉培福林对映体进行手性分离,考察了流动相配比、背景电解质pH值、柱温和分离电压等对分离的影响.在缓冲溶液为5 mmol/L NaH2PO4-Na2HPO4(pH 2.5)、运行电压20 kV、毛细管温度15 ℃条件下,16 min内成功分离了吉培福林对映体,其分离度为1.53.     

毛细管电色谱硅胶整体柱的制备与性能研究

以甲基丙烯酸丙酯基三甲氧基硅烷(MPTMS)为单体,甲苯为致孔剂,偶氮二异丁腈(AIBN)为引发剂,盐酸为催化剂,采用热引发法制备毛细管电色谱硅胶整体柱.在反相毛细管电色谱条件下,对中性化合物硫脲,苯,萘,芴,蒽实现了基线分离了.柱效超过100,000 plates/m.探讨了该柱的制备条件如单体比例,毛细管内径,制柱反应时间对分离的影响,并且在电色谱条件下考察了有机溶剂比例,pH值,电压和温度对分离的影响.     

开管毛细管电色谱进展

开管毛细管电色谱是近年发展起来的一种高效、快速的新型微柱分离方法。它是在毛细管管壁涂布或键合固定相,以电渗流驱动流动相的一种色谱分离模式。该文对开管毛细管电色谱的发展、柱制备、理论进行了较为详细的综述,引用文献４７篇     

连续二维开管离子交换/反相整体柱毛细管电色谱的构建与评价

在毛细管中原位合成反相整体色谱柱,并在同一根毛细管柱中的其余部分通过在内表面涂覆N-[3-(三甲氧基硅烷)-丙基)]-乙二胺(PEDA)使其具有离子交换功能,制备成连续二维开管离子交换/反相整体柱毛细管电色谱柱.通过对7种有机酸的分离探讨了开管柱中离子交换对分离的影响,进一步以天麻提取物为样品,对二维分离系统加以评价,...     

毛细管等电聚焦-毛细管区带电泳二维蛋白质分离平台的构建及其性能

通常采用二维聚丙烯酰胺凝胶电泳 ( 2 D- PAGE)分析组织或细胞的全蛋白质 [1] ,但难与质谱 ( MS)直接联用 .用高效液相色谱 ( HPLC)和毛细管电泳 ( CE)分离分析蛋白质和多肽的一维分离模式的分辨率和峰容量有限 .多维柱联用技术比一维分离有更高的分辨率和峰容量 [2 ] ,便于和 MS直接联用 [3,4 ] ,易于实现自动化 .目前 ,有关 2 D- CE的报道相对较少 [5～ 7] ,我们初步实现了将 2 D- PAGE由平板转移到毛细管中[6 ,7] ,但凝胶柱的制作烦琐 ,存在交叉污染 ,不能与 MS直接联用 .本文用微透析中空纤维膜为接口构建了毛细管等电聚焦 ( …     

填充毛细管电色谱手性分离

采用两种毛细管填充电色谱手性分离模式 ,在短时间内对 3种手性化合物进行成功拆分 :( 1 )用匀浆法制成 75 μm内径的 β CD固定相填充电色谱柱 ,考察了电压、缓冲溶液pH值和有机添加剂浓度对该柱电渗流 (EOF)和两种手性物质分离的影响 .手性化合物安息香 (benzoin)和手性药物美芬妥因 (mephenytoin)在有效长度为6 2cm的β CD填充柱中获得快速、高效的分离 .安息香的最高柱效达 3.2万理论塔板数 /m ,最大分离度Rs 为 1 42 ,美芬妥因的最高柱效达 4 5万理论塔板数 /m ,最大分离度Rs 为 3 40 ,特别是美芬妥因在 1 5kV电压下 3 4min内获得Rs=2 .6 0和N1=2 .1万理论塔板数 /m的分离结果 . ( 2 )用匀浆法制成 75 μm内径的ODS填充电色谱柱 ,在该柱上用二甲基 β CD (DM β CD)作流动相手性添加剂 ,施加 1 0kV电压在1 2min内使手性药物心得安 (propranolol)得到基线分离 ,柱效达 8 1万理论塔板数 /m .     

毛细管电色谱应用研究进展

对近年来毛细管电色谱(CEC)的研究现状以及实际应用进行归纳总结。以查阅国内外有关文献资料的方法,综述毛细管电色谱的研究现状以及在药物、食品、农残、化妆品、氨基酸以及环境检测等分析中的应用。毛细管电色谱在上述分析领域中获得了广泛的应用,同时对毛细管电色谱的未来发展方向(加压毛细管电色谱)进行了展望。毛细管电色谱拥有广阔的发展应用前景。     

Capillary electrophoresis of hemoglobins and globin chains.

Capillary isoelectric focusing (cIEF) and free zone capillary electrophoresis were evaluated for separation of native hemoglobins and globin chains. High-resolution separations of adult human hemoglobin A, fetal human hemoglobin F, and hemoglobin variants S and C were obtained using cIEF with cathodic mobilization. Absorbance detection in the UV and visible regions were compared, and on-line fast UV or visible-wavelength scanning detection was used to obtain spectral information on separated components. Globin chain analysis was performed on the same hemoglobin species by free zone capillary electrophoresis following precipitation of the protein with acidic acetone. Free zone separations were carried out at low pH in the presence of 7 M urea.     

Capillary electrophoretic separations of proteins using carrier ampholytes

Capillary separations of proteins using carrier ampholytes are performed between an anolyte and a catholyte of same pH (pH 3). Depending upon the concentration of carrier ampholytes used, two different separation processes take place. At a 10% concentration, the high-resolution separation of six model proteins is achieved, which can be described as a transient capillary isoelectric focusing (cIEF) system moving isotachophoretically. The isotachophoretic (ITP) behaviour of the system is evidenced by the influence of the catholyte concentration on the separation. The separation is neither pure cIEF nor pure cITP and the migration order of the proteins results from the influence of both their isolelectric points and their mobilities.     

Capillary isoelectric focusing of erythropoietin glycoforms and its comparison with flat-bed isoelectric focusing and capillary zone electrophoresis

The influence of several operation conditions on separation of recombinant human erythropoietin glycoforms by capillary isoelectric focusing (cIEF) is explored. From this study it is deduced that in order to separate several glycoforms of erythropoietin, urea has to be added to sample, which should not be completely depleted of the excipients used in its formulation. On-line desalting does not provide separation enhancement for samples with high content of salt. Better resolution is obtained using a mixture of a broad and a narrow pH-range carrier ampholytes than with either one used separately. Under the experimental conditions, focusing voltages of 25 kV improve separation compared to lower and higher electric fields. Focusing times shorter than the time necessary for electric current to reach a minimum provide similar separations than longer focusing times at which a minimum value of the current has already been achieved. The optimized method allows the separation and quantitation in 12 min of at least seven bands containing glycoforms of recombinant erythropoietin with apparent isoelectric points in the range 3.78–4.69. Compared to flat-bed isoelectric focusing, cIEF provides better separation of bands of glycoforms in a shorter time, and allows quantitative determination. Capillary zone electrophoresis (CZE) gives rise to resolution of erythropoietin glycoforms similar to that obtained by cIEF. Although CZE requires a longer analysis time, its reproducibility in terms of peak area of glycoforms is better than in cIEF.     

用聚丙烯酰胺交联涂层毛细管电泳柱分离无机阴离子

研究了用涂层柱分离Ｉ＾－，ＮＯ＾－２，ＮＯ＾－３，ＳＣＮ＾－，ＭｏＯ＾２－４等５种具有紫外吸收的阴离了的毛细管电泳方法。采用涂层柱可以有效地抑制电渗流，因此无需在载体电解质溶液中加入电流改性剂。其优越性在于改善了由于电渗流改性剂与体积较大的阴离子发生离子对相互作用所导致的峰形拖尾现象，有助于准确定理。     

毛细管电色谱手性分离进展

 :比较全面地评述了毛细管电色谱(CEC)在手性拆分领域中的应用和发展,包括CEC的不同操作模式、手性试剂和手性固定相。92篇。     

α-萘基缩水甘油醚对映体的毛细管区带电泳手性拆分

建立了毛细管区带电泳手性拆分α-萘基缩水甘油醚对映体的方法.考察了不同手性拆分试剂对手性选择性的影响,实验结果表明,20 mmol/L H3PO4-三乙醇胺(pH 2.5)、2%(w/V)HS-β-CD、毛细管温度20 ℃、运行电压-18 kV为最佳分离条件,在该分离条件下α-萘基缩水甘油醚对映体实现基线分离.方法简便、准确,可用于α-萘基缩水甘油醚的手性拆分和对映体过量值(ee,%)测定.     

毛细管电泳在手性分离中的应用及进展

本文评述了近年来毛细管电泳在手性分离中的应用及进展，介绍了毛细管电泳分离手性对映射的数学模型、五种不同的分离模式及机理、七种常用的手性选择性类型及其在药学、环境和生命科学中的应用、研究中需优化的操作参数及其发展方向。     

Extension of separation range in capillary isoelectric focusing for resolving highly basic biomolecules

The non-availability of commercial carrier ampholytes in the pH range greater than 11 has contributed to difficulties in focusing and resolving highly basic proteins/peptides using capillary isoelectric focusing (cIEF). Two different approaches, involving the use of N,N,N',N'-tetramethylethylenediamine (TEMED) and ampholyte 9-11, are investigated for their effects on the extension of separation range in cIEF. The addition of TEMED into pharmalyte 3-10 not only prevents the peptides/proteins from focusing in sections of the capillary beyond the detection point, but also extends the separation range to at least isoelectric point (pI) 12. The combination of ampholyte 9-11 with pharmalyte 3-10 surprisingly provides baseline resolution between bradykinin (pI 12) and cytochrome c (pI 10.3). The sample mixture, containing bradykinin, the high-pI protein calibration kit (pI 5.2-10.3), and cytochrome c digest, is employed to demonstrate the cIEF separation of proteins and peptides over a wide pH range of 3.7-12.     

Separation of Basic Drugs Using Pressurized Capillary Electrochromatography

A novel pressurized capillary electrochromatography(PCEC) was developed to separate baxic drugs on strong cation exchange(SCX) column.The separation result by using PCEC was better than that by using micro-HPLC.The effects of electrical field and pressure on plate height and resolution were investigated.Influences of organic modifier,ionic strength and pH value of buffer on retention behavior were evaluated,and the separation mechanism was also discussed.     

High-efficiency capillary isoelectric focusing of protein complexes from Escherichia coli cytosolic extracts

High-efficiency capillary isoelectric focusing (cIEF) separations of protein complexes obtained from soluble protein fractions are demonstrated. Size-exclusion chromatography was used as a first dimension separation to fractionate putative protein complexes with apparent molecular masses of up to 1,500,000 from an Escherichia coli cytosolic fraction. Non-denaturing cIEF separations using highly hydrophilic polymer-coated capillaries constituted the second dimension. The conditions developed produced reproducible and high-efficiency separations, corresponding to approximately 2 x 10(6) theoretical plates and peak capacities of approximately 10(3) for pH 3-10 cIEF separations in 65 cm long capillaries. Combination of the two non-denaturing separation dimensions permitted isolation and analysis of individual protein complexes from complicated biological samples. Studies indicated that many E. coli complexes were stable on the time scale of the cIEF separations, but were degraded upon more extended periods of storage on ice, necessitating rapid sample processing and fast analysis techniques.