稀土离子及胺和氨基酸的高效毛细管区带电泳电导检测

用自制高效毛细管电泳装置研究毛细管电泳电导检测，由用阴离子交换膜管制作的导电接口连接电泳毛细管和电导池，高电压被有效隔离，实现柱后电导检测，用长６０ｃｍ、内径５０μｍ石英毛细管，以ｐＨ４．０的７×１０￣（－３）ｍｏｌ／ＬＮａＡｃ￣（－２）×１０￣（－３）ｍｏｌ／ＬＨＩＢＡ－ＨＡＣ溶液为载体，在１８ｋＶ电压下，轻重三种稀土Ｎｄ、Ｇｄ、Ｙｂ的混合物８ｍｉｎ内完成分离检测。用上述毛细管，以ｐＨ为５．８的５×１０￣（－３）ｍｏｌ／ＬＮａＡｃ－ＨＡＣ溶液为载体，在２０ｋＶ电压下乙二胺、三乙胺、组氨酸、谷氨酸混合有机物７．５ｍｉｎ内完成分离检测。     

高效细内径毛细管电色谱填充柱的制备

发展了一套毛细管填充柱制备方法,在１００μｍ内径毛细管柱中填充３μｍＯＤＳ固定相,以毛细管电色谱法（ＣＥＣ）分离模式对芳香胺类样品进行分离,柱效高达２５．９万理论塔板数／米,折合塔板高度达１．３。类似研究在国内尚未见报道。     

5-氨基水杨酸锌及相关物质的高效液相色谱分析研究

对５－氨基水杨酸锌及相关物质５－氨基水杨酸、水杨酸、对氨基苯酚和５－苯偶氮基水杨酸的高效液相色谱法（ＨＰＬＣ）的分离条件进行了优化研究,结果表明,采用ＣＬＣ－ＯＤＳ（１５０ｍｍ×６．０ｍｍｉ．ｄ．,１０μｍ）作为分离柱,１％（Ｖ／Ｖ）ＨＡｃ－ＭｅＯＨ（４∶６）作为流动相,在流速为１ｍＬ／ｍｉｎ的情况下,上述５种物质在１０ｍｉｎ内可以达到基线分离,保留时间的日内和日间的变异系数分别小于２％和５％,在一定浓度范围内,浓度与峰面积的线性关系良好。     

毛细管电泳的原理及应用（第三讲）毛细管电泳的柱技术

毛细管电泳的原理及应用（第三讲）毛细管电泳的柱技术王义明,罗国安（清华大学化学系,清华大学生命科学与工程研究院北京１０００８４）关键词毛细管电泳,柱技术１概述毛细管电泳（ＣＥ）的分离和检测过程均在毛细管内完成,所以说毛细管是ＣＥ的核心部件之一。早期对毛细管的研究集中在毛细管直径、长度、形状和材料方面。采用细柱可减少电流及自热,而且能加快散热,以保持高效分离;但会造成进样、检测及清洗上的困难,也不利于对吸附的抑制,故现在一般采用２５～１００μｍ内径的毛细管。     

毛细管电泳在拮抗药物对氨基苯甲酸，对羟基苯甲酸和磺胺分析测…

本报道了一种用毛细管区带电泳法分离与测定对氨基苯甲酸、对羟基苯甲酸及磺胺类药物的新方法。电泳条件为：用２０ｍｍｏｌ／Ｌ硼砂－２０ｍｍｏｌ／ＬＨ３ＰＯ４－２０ｍｍｏｌ／Ｌβ－环糊精－４％乙醇作电泳液，Ｌ－抗坏血酸为内标，２８０ｎｍ为检测波长，样品由电进样方式１０ｋＶ／１０ｓ）引入毛细管（５１．２ｃｍ×５０μｍｉ．ｄ．，有效分离长度为３８．５ｃｍ）．在２４．５℃下，６ｍｉｎ内三可达基线分离（电泳电     

硅胶填充柱反相洗脱毛细管电色谱研究

在７５μｍ（ｉ．ｄ．）×２７／２０ｃｍ的硅胶（３μｍ）填充柱上，以乙腈（９５：５）－Ｔｒｉｓ／ＨＣｌ缓冲液（ｐＨ８．３）为流动相，实施毛细管电色谱并对其保留机理进行了研究。研究表明，当采用反相洗脱时，硅胶填充柱显示出阳离子交换和正相分配双重保留机理。同时还对电渗流和热效应进行了研究。     

钛层柱粘土的合成 Ⅰ．四氯化钛作钛源

由ＴｉＣｌ４／ＨＣｌ配制的含钛柱化剂与粘土进行阳离子交换后得到大孔钛层柱粘土（Ｔｉ－ＰＩＬＣ），详细研究了各种合成条件，诸如Ｔｉ（Ⅳ）及ＨＣｌ浓度，柱化剂老化时间，粘土初始浓度，交换温度及配料比等对层柱粘土的大孔及比表面积的影响．优化条件合成的Ｔｉ－ＰＩＬＣ存在两种晶面间距（ｄ００１），其中之一（２．５６ｎｍ）对应大孔结构．Ｔｉ－ＰＩＬＣ比表面积为３２８ｍ２／ｇ，５００℃焙烧后ｄ００１保持２．３２ｎｍ，６５０℃焙烧后比表面积仍达３０１．４ｍ２／ｇ．Ｔｉ－ＰＩＬＣ的大孔结构主要取决于交换时混合液中Ｔｉ（Ⅳ）和ＨＣｌ浓度，并与柱化剂老化时间、交换温度等因素有关；与原柱化剂中Ｔｉ（Ⅳ）和ＨＣｌ浓度无关．混合液中ＣＨＣｌ提高，Ｔｉ－ＰＩＬＣ的比表面积下降；当ＣＨＣｌ增至７０ｍｍｏｌ／Ｌ时，产物中大晶面间距消失，仅留下小晶面间距（～１．４ｎｍ）．随着混合液中ＣＴｉＣｌ４的提高，Ｔｉ－ＰＩＬＣ的比表面积先上升而后下降。当ＣＴｉＣｌ４增至１４６ｍｍｏｌ／Ｌ时，产物也仅有小晶面间距（１．４ｎｍ）．     

复方新诺明片剂中有效成分的毛细管区带电泳快速测定法

研究了用毛细管区带电泳法快速测定复方新诺明片中磺胺甲恶唑（ＳＭＺ）和甲氧苄氨嘧啶（ＴＭＰ）的含量。使用长２７ｃｍ（有效长度２０ｃｍ）内径５０μｍ的石英毛细管,２５ｋＶ分离电压,在０．０５ｍｏｌ／Ｌ的乙酸盐缓冲液（ｐＨ５．５）中,上述两组分可在１．５ｍｉｎ内完全分离。用紫外检测器在２１４ｎｍ处检测,外标法定量。１０次检测含有１４１．７ｍｇ／ＬＳＭＺ和２５．６ｍｇ／ＬＴＭＰ的试样溶液,相对标准偏差为１     

毛细管区带电泳在氧氟沙星含量分析中的应用

氧氟沙星（ＯＦ）是第三代喹诺酮类药物中效果最好的广谱抗菌素之一。由于它在ｐＨ２～１１范围内难溶于水与醇，给用ＨＰＬＣ法检测其含量带来一定困难。本文报告了用毛细管区带电泳（ＣＺＦ）分离检测该药的方法。由于使用ｐＨ调制样品引入技术，克服了其溶解性不好给ＨＰＬＣ法所带来的困难。其实验条件为：５０ｍｍｏｌ／Ｌ硼砂（ｐＨ１．５）为电泳缓冲液，２８０ｎｍ为紫外检测波长，２５ｋＶ为电泳电压。样品由高差进样方式引入分离毛细管（５．１２ｃｍ×５０μｍｉ．ｄ．，有效分离长度为３８．５ｃｍ）。用磺胺作内标，ＯＦ在４８～５３０ｍｇ／Ｌ及５８０～９７０ｍｇ／Ｌ范围内可进行定量分析。保留时间（ｔｒ）及相对紫外吸收（Ａ（样品）／Ａ（内标））的日内－ＲＳＤ值分别小于１．０％和２．４％（ｎ＝６）。     

碱性药物与人血清白蛋白结合参数的毛细管区带电泳/前沿分析

将毛细管区带电泳／前沿分析技术用于测定碱性药物ｖｅｒａｐａｍｉｌ（ＶＥＲ）和ｐｒｏｐｒａｎｏｌｏｌ（ＰＲＯ）与人血清白蛋白（ＨＳＡ）平衡体系中结合参数的研究。通过压力进样将药物白蛋白混合液引入石英毛细管电泳柱（３２ｃｍ×５０μｍｉ．ｄ．,聚丙烯酰胺涂渍柱）,在ｐＨ值为７．４、离子强度为０．１７的磷酸缓冲液及运行电压为１０ｋＶ的条件下,未结合的碱性药物的浓度可以通过电泳平台峰的高度定量,并且具有良好的线性关系（相关系数ｒ＝０．９９９）。     

毛细管电泳-限制性片段长度多态性分析检测胃癌H-ras基因点突变

建立一种毛细管电泳快速高效检测限制性内切酶酶切产物的方法, 使其更好地用于基因诊断. 以甲基纤维素(Methyl cellulose, MC)为筛分介质, 用pUC19 DNA/Msp I (Hpa II) Marker标准DNA片段为实验对象, 通过考察筛分介质的浓度、pH值、毛细管的温度和运行电压优化出分离小于600 bp的双链DNA片段的最适条件, 并将此方法应用于临床59例胃癌患者肿瘤组织H-ras基因12位密码子点突变情况的检测. MC是一种良好的筛分介质, 运用其进行毛细管电泳对于遗传性疾病的诊断将更加快速、准确、简便、灵敏.     

Further Study on Separation of DNA Fragments by Capillary Electrophoresis by Quasi-interpenetrating Network of Polyacryamide and Polyvinylpyrrolidone with UV Detection

Quasi-interpenetrating network of polyacrylamide （PAA） and polyvinylpyrrolidone （PVP） had been successfully used for single-base resolution of double-stranded DNA （0.76 for 123 bp/124 bp） and single-stranded DNA fragments （0.97 for 123 b/124 b） with UV detection. This quasi-IPN （interpenetrating network） sieving matrix showed low viscosity （23.5 mPa·s at 25 ℃） and decreased with increasing temperature. This polymer also exhibited dynamically coating capacity and could be used in the uncoated capillary. The effects of temperature and electric field strength on the DNA separation of quasi-IPN matrix were also investigated and found that the temperature and electric field strength could markedly affected the mobility behavior of DNA fragments. This polymer matrix has also applied to separate the bigger DNA fragments by capillary electrophoresis with UV detection. Under the denaturing conditions, this matrix separated the samples with last fragment of 1353 base in 40 rain, in which the doublet of 309/310 base was partial separated and the resolution was 0.88.     

High-speed DNA sequencing by tube-based capillary electrophoresis

We assessed the feasibility of high-speed DNA sequencing by tube-based capillary electrophoresis (TCE) with electrokinetic sample injections. We developed a water-circulated TCE system to control the capillary temperature precisely. Using this system and a ready-made sieving matrix at 50 degrees C, single-stranded DNA size marker fragments were separated at various pairs of the electric field strength, E, of 128-480 V/cm and the capillary effective length, L, of 100-360 mm. Assuming the read length (RL) is the fragment size at which the peak width equals the peak interval per base in obtained electropherograms, we estimated the values of RL (E, L), the RL at the pair (E, L). The points in ELz-space, (E, L, RL(E, L)), form a curved surface expressed by z = RL(E, L). Analyzing the contour lines of this curved surface, we determined the pairs of E and L providing target RLs of 300-500 bases within a minimum time. At a pair optimized for a 500-base RL (330 V/cm, 200 mm), one-color sequencing fragments were successfully separated up to 529 bases within 9.6 min. These results demonstrate that high-speed DNA sequencing comparable with that obtained by microfabricated chip-based capillary electrophoresis (MCE) can be achieved with TCE, which is more suitable in automation than MCE.     

Ultra-slim laminated capillary array for high-speed DNA separation

We developed a new kind of capillary array for electrophoresis by using the numerical-control (NC) wiring technique conventionally used to produce printed-circuit boards. Laminating two polyimide sheets after laying cylindrical capillaries between them according to designed geometries, we fabricated a 16-lane laminated capillary array (LCA) 9.9 cm long, 7.2 cm wide, and 0.5 mm thick in which the effective length of all capillaries was only 10.9 cm. This compact LCA thus had separation columns as short as those in capillary array electrophoresis chips fabricated by lithography techniques. Like conventional capillary arrays, it also enabled pipetting-less direct injection of analytes from sample preparation plates. Using the LCA with LIF detection and a replaceable fluid sieving matrix, we demonstrated high-speed ssDNA fragment separations. At an electric field strength of 316 V/cm, 15 fragments ranging from 50 to 500 bases were completely separated within 5.8 min in all lanes. The lane-to-lane CV of migration time was only 0.38%, and the fragment size for which the resolution per base was 0.59 was 258 +/- 15 bases (average +/-SD).     

Separation of double-stranded DNA fragments in plastic capillary electrophoresis chips by using E99P69E99 as separation medium.

The separation of double-stranded DNA (dsDNA) fragments in polymethylmethacrylate (PMMA) capillary electrophoresis (CE) chips by using E99P69E99 as a separation medium has been demonstrated. The PMMA CE chips were simply manufactured by micromachining and adhesive tape sealing. To make the separation channel compatible with the separation medium, a dynamic nonionic surfactant coating procedure was developed, which made the plastic separation channel sufficiently hydrophilic to allow the separation medium to fill the channel by capillary action. Subsequent separation of DNA fragments was successful with a separation efficiency of the order of 10(4) theoretical plates over an effective separation distance of 1.5 cm. By using an applied electric field strength of 200 V/cm, the separation of low DNA mass ladder was completed within 5 min. The simple coating procedure, together with the self-assembled viscosity-adjustable separation medium, should be useful to meet some of the essential requirements for developing single-use disposable CE chips. Coating the channels with polymer blends of PMMA and the separation medium also showed promise.     

Divergent dispersion behavior of ssDNA fragments during microchip electrophoresis in pDMA and LPA entangled polymer networks

Resolution of DNA fragments separated by electrophoresis in polymer solutions ("matrices") is determined by both the spacing between peaks and the width of the peaks. Prior research on the development of high-performance separation matrices has been focused primarily on optimizing DNA mobility and matrix selectivity, and gave less attention to peak broadening. Quantitative data are rare for peak broadening in systems in which high electric field strengths are used (>150 V/cm), which is surprising since capillary and microchip-based systems commonly run at these field strengths. Here, we report results for a study of band broadening behavior for ssDNA fragments on a glass microfluidic chip, for electric field strengths up to 320 V/cm. We compare dispersion coefficients obtained in a poly(N,N-dimethylacrylamide) (pDMA) separation matrix that was developed for chip-based DNA sequencing with a commercially available linear polyacrylamide (LPA) matrix commonly used in capillaries. Much larger DNA dispersion coefficients were measured in the LPA matrix as compared to the pDMA matrix, and the dependence of dispersion coefficient on DNA size and electric field strength were found to differ quite starkly in the two matrices. These observations lead us to propose that DNA migration mechanisms differ substantially in our custom pDMA matrix compared to the commercially available LPA matrix. We discuss the implications of these results in terms of developing optimal matrices for specific separation (microchip or capillary) platforms.     

聚环氧乙烷无胶筛分毛细管电泳分离宽分子量范围DNA片段

在无胶筛分毛细管电泳中,以聚环氧乙烷为筛分介质,用硅烷化处理的毛细管柱（31.2 cm×75 μm有效长度21.0 cm）分离DL5000 DNA Marker（DNA长度为100~5000 bp）,研究筛分介质浓度、缓冲液pH、分离电压和溴化乙锭浓度对分离双链DNA片段的影响,优化出分离100~5000 bp DNA片段的最佳条件。毛细管电泳的最佳条件为PEO浓度0.5%、缓冲液pH值8.0、电压12 kV、溴化乙锭浓度3.0 μg/mL。此条件下,对山梨醇脱氢酶基因（SDH）和乙烯受体基因（ETR1）的聚合酶链式反应（PCR）扩增产物同时检测,分离、鉴定效果良好。     

毛细管电泳中葡萄糖-羟丙基甲基纤维素体系分离脱氧核糖核酸

葡萄糖作为羟丙基甲基纤维素（Hydroxpropylmethyl cellulose,HPMC)筛分体系的添加剂,可以改善该体系在低浓度时分离脱氧核糖核酸（DNA）的能力。研究了硼酸浓度和pH值对葡萄糖－羟丙基甲基纤维素体系分离性能的影响;并将葡萄糖与其它添加剂如甘油、甘露醇对分离的影响作了比较,葡萄糖特有的环状结构使得其对羟丙基甲基纤维素体系分离能力的提高更为显著。     

Simultaneous detection of 19 K‐ras mutations by free‐solution conjugate electrophoresis of ligase detection reaction products on glass microchips

We demonstrate here the power and flexibility of free‐solution conjugate electrophoresis (FSCE) as a method of separating DNA fragments by electrophoresis with no sieving polymer network. Previous work introduced the coupling of FSCE with ligase detection reaction (LDR) to detect point mutations, even at low abundance compared to the wild‐type DNA. Here, four large drag‐tags are used to achieve free‐solution electrophoretic separation of 19 LDR products ranging in size from 42 to 66 nt that correspond to mutations in the K‐ras oncogene. LDR‐FSCE enabled electrophoretic resolution of these 19 LDR‐FSCE products by CE in 13.5 min (E = 310 V/cm) and by microchip electrophoresis in 140 s (E = 350 V/cm). The power of FSCE is demonstrated in the unique characteristic of free‐solution separations where the separation resolution is constant no matter the electric field strength. By microchip electrophoresis, the electric field was increased to the maximum of the power supply (E = 700 V/cm), and the 19 LDR‐FSCE products were separated in less than 70 s with almost identical resolution to the separation at E = 350 V/cm. These results will aid the goal of screening K‐ras mutations on integrated “sample‐in/answer‐out” devices with amplification, LDR, and detection all on one platform.     

Fast DNA sequencing up to 1,000 bases by capillary electrophoresis using poly(N,N-dimethylacrylamide) as a separation medium

Poly(N,N-dimethylacrylamide) (PDMA) with a molecular mass of 5.2 x 10(6) g/mol has been synthesized and used in DNA sequencing analysis by capillary electrophoresis (CE). A systematic investigation is presented on the effects of different separation conditions, such as injection amount, capillary inner diameter, polymer concentration, effective separation length, electric field and temperature, on the resolution. DNA sequencing up to 800 bases with a resolution (R) limit of 0.5 (and 1,000 bases with a resolution limit of 0.3) and a migration time of 96 min was achieved by using 2.5% w/v polymer, 150 V/cm separation electric field, and 60 cm effective separation length at room temperature on a DNA sample prepared with FAM-labeled--21M13 forward primer on pGEM3Zf(+) and terminated with ddCTP. Ultrafast and fast DNA sequencing up to 420 and 590 bases (R > or = 0.5) were also achieved by using 3% w/v polymer and 40 cm effective separation length with a separation electric field of 525 and 300 V/cm, and a migration time of 12.5 and 31.5 min, respectively. PDMA has low viscosity, long shelf life and dynamic coating ability to the glass surface. The unique properties of PDMA make it a very good candidate as a separation medium for large-scale DNA sequencing by capillary array electrophoresis (CAE).