基于硅溶胶-凝胶/褐藻酸钠复合膜包埋酪氨酸酶的苯酚传感器研制

将天然聚合物褐藻酸钠添加到无机硅溶胶-凝胶膜,获得一种新型的无机/有机杂化膜。用此杂化膜包埋酪氨酸酶,制备电化学苯酚传感器。研究表明:硅溶胶-凝胶/褐藻酸钠复合膜能有效克服纯无机溶胶-凝胶膜的脆性;避免膜的裂开;提供生物酶所适宜的微环境;有效保持所固定酶的生物活性。所制备的传感器测定苯酚的线性响应范围为3.4-93.1μmol/L,其线性回归方程i(μA)=0.0774C(μmol/L) 0.1616,r=0.9980。检出限为1.33μmol/L。     

水溶性丙烯酸树脂相对分子质量及其分布的测定

选用HPll00型高效液相色谱仪、HP PLgel MIXED—B双柱串联，以四氢呋喃作流动相，采用紫外吸收检测器测定了水溶性丙烯酸树脂的平均相对分子质量及其分布。确定了凝胶色谱(GPC)的最佳实验条件：流动相流速为1.5mL／min，进样质量浓度为1．0g／L，进样体积为40μg/L。该方法测定结果与粘度法测定结果相比相对误差小于6％。     

亲水性高聚物凝胶EGPM分离蛋白质的高速空间排除色谱

利用空间排除色谱分离生物高分子,过去都是采用软的亲水性凝胶为柱填料。例如Bio-Gel P(交联聚丙烯酰胺)、Sephadex(交联葡聚糖凝胶)、Sepharose(珠状琼脂糖)、Bio-Gel A(琼脂糖凝胶)等。这些凝胶不能承受较高的柱压,一般只能在0.002-0.02厘米/秒的流速下操作,才能保持凝胶的机械稳定性。这个流速比高效液相色谱所通用的流速约低一个数量级。因此,达到分离平衡的淋洗时间较长,分离周期往往需要几小时。此外,这类软凝胶一般需要较大的进样量方能检出,如对蛋白质的检测就需要毫克级的量。     

褐藻酸钠溶液的超声辐照效应及其对分子量参数的影响

观察了超声辐照过程中褐藻酸钠溶液的pH值、温度、表现特性粘度和表现分子量及其分布的变化,发现在超声辐照过程中,褐藻酸钠的表现平均分子量经历了下降→回升→再下降的过程;当超声辐照停止后,表现特性粘度和表观平均分子量又略有回升,因而推测在这一过程中褐藻酸钠的构象可能发生了变化。     

高效液相色谱仪自动进样器校准方法及不确定度评定

建立高效液相色谱仪自动进样器的校准方法,并对其测量不确定度进行评定。参考欧洲医药管理局《质量控制文件》提供的方法对液相色谱仪自动进样器的进样体积误差、进样残留和进样重复性建立校准方法,经评定得进样体积误差的相对扩展不确定度为1.8%。高效液相色谱仪自动进样器校准方法及不确定度评定方法的建立,为高效液相色谱仪自动进样器的校准提供依据。     

高效液相色谱法测定双氯芬酸钠凝胶的有关物质

建立了双氯芬酸钠凝胶中有关物质的高效液相色谱分离分析方法。采用梯度洗脱的方法对双氯芬酸钠凝胶的有关物质进行分离,流动相A为pH 2.0三氟乙酸溶液-甲醇(80:20),流动相B为乙腈-甲醇(80:20)。采用Waters XBridge色谱柱(5μm,150mm×4.6mm)进行分离,流速为1.0mL/min,进样体积为5μL,二极管阵列检测器,检测波长为254nm,柱温为30℃。在上述色谱条件下,双氯芬酸钠凝胶及特定杂质均在1.0～40.0mg/L质量浓度范围内线性关系良好,相关系数(r)均大于0.99;方法对特定杂质的回收率为97%～104%,相对标准偏差(RSD)不大于3.8%。该法简便、快速、准确、选择性好、灵敏度高,可用于含醇类辅料的双氯芬酸钠凝胶中有关物质的检测。     

壳聚糖／褐藻酸钠聚离子复合膜的渗透汽化分离性能研究

以红外光谱和扫描电镜表征壳聚糖／褐藻酸钠聚离子复合膜的结构与表面形态。研究了该膜组成、料液浓度、温度等对乙醇－水溶液的渗透汽化分离性能的影响。实验结果表明，壳聚糖／褐藻酸钠聚离子复合膜不仅对乙醇－水溶液，而且对许多水溶性有机溶剂与水的溶液都具有很高的渗透汽化脱水的选择分离性能。     

褐藻酸钠对Cu~(2 )、Pb~(2 )交换与吸附性能的研究

本文研究了褐藻酸钠与Cu2 , Pb2 交换行为,通过海藻酸钠溶液与Cu2 , Pb2 的絮凝,测得两种离子最大交换量。考察了褐藻酸钠固体粉末与Cu2 , Pb2 在不同的反应条件下的离子交换与吸附行为。实验表明pH值,温度,时间,配比等条件是影响交换与吸附的因素,其吸附行为在一定的温度和一定的浓度范围内能较好的符合Freundlich等温吸附式     

茜素红S-牛血清白蛋白配合物的凝胶层析分离制备及紫外可见吸收光谱研究

用葡聚糖凝胶层析分离制备牛血清蛋白(BSA)-茜素红S(ARS)配合物。在420和530 nm处用紫外可见吸收光谱法同时测定含有BSA-ARS配合物和茜素红S的联立方程为:A420=4.89×103cARS 3.06×104cBSA-ARS,A530=4.60×102cARS 2.29×104cBSA-ARS;正交试验选择了合适的分离条件:柱直径1.0 cm,柱长30.0 cm,凝胶用量1.3 g,最佳进样浓度为ARS:5×10-3mol/L、BSA:1.49×10-4mol/L,进样体积1.5 mL,洗脱流速0.33 mL/min,分离度为1.25;测定了纯BSA-ARS配合物紫外吸收光谱,最大吸收峰在530 nm。     

进样阀(I)

高效液相色谱进样阀（或进样器）的作用是将一定量的样品送入色谱仪。样品在流动相的带动下进入色谱柱系统完成分离过程。现代高效液相色谱仪对于进样阀的要求如下：（１）耐高压,因为高效液相色谱通常要在３５．０ＭＰａ或更高的压力下工作;（２）进样量精确;（３）进样重复性好;（４）方便、适用,且可根据需要选择不同的进样量;（５）价格低廉;（６）保证在色谱柱中心进样,操作时不产生流量或压力波动。到目前为止,液相色谱进样阀共有３种形式：１．手动注射进样器;２．手动进样阀;３．自动进样器。从原理上讲,自动进样器是在…     

高效液相色谱法同时测定牙膏及漱口水中的23种致癌染料

建立了同时测定牙膏和漱口水中23种致癌染料的高效液相色谱(HPLC)检测方法。漱口水样品直接以乙醇溶解稀释,牙膏样品烘干后以乙醇超声提取。采用ZORBAX Eclipse XDB-Phenyl(150 mm×4.6 mm×5μm)色谱柱进行分离,以2.5 mmol/L磷酸二氢四丁基铵水溶液(pH 7.5)和甲醇-乙腈(体积比50∶50)为流动相进行梯度洗脱,二极管阵列检测器(DAD)在400、500、600 nm波长下检测,外标法定量。结果表明,23种致癌染料在32 min内完成色谱分离,在相应的质量浓度范围内线性良好,相关系数(r2)均不小于0.9991,检出限(LOD)和定量下限(LOQ)分别为0.06~0.66 mg/L和0.18~1.98 mg/L。以阴性牙膏和漱口水为样品基质,23种致癌染料在3个加标水平下的平均回收率分别为91.2%~104%和92.0%~103%,相对标准偏差(RSD,n=6)分别为2.5%~5.8%和2.3%~5.5%。对239个牙膏和88个漱口水样品进行检测,1个牙膏样品中检出碱性紫3。该方法灵敏度高,精密度好,准确度高,适用于牙膏和漱口水中致癌染料的测定,可为牙膏和漱口水的质量安全监控提供参考。     

Solvent and salting effects on sample preparation for the determination of fenofibric acid in human plasma by HPLC-DAD

The solvent and salting effects induced on the sample preparation procedure applied to plasma samples containing fenofibric acid and 4-chlorophenyl-4′-hydroxyphenyl methanone (internal standard) are evaluated. Sodium chloride addition during a deproteinization step using both methanol and phosphoric acid influences the recovery of the analytes as well as the selectivity of the process. The chromatographic method allows high sample volume injection (500 μl) with the focusing of both analytes in the stationary phase. The synthesized high porosity octadecylsilica material allows a fast elution gradient at 4 ml/min flow-rate and a complete analysis within 7 min. UV-detection is made at 295 nm and quantitation limit in the 20 ng/ml concentration level can be achieved. The method can be successfully applied for bioequivalence studies on fenofibrate, administrated as prodrug (fenofibric acid represents its main active metabolite) in pharmaceutical formulations. The main parameters used in studying the retention behavior of the internal standard and FEFA were also estimated.     

Sensitive and rapid high‐performance liquid chromatography tandem mass spectrometry method for estimation of fulvestrant in rabbit plasma

A rapid and sensitive high‐performance liquid chromatography and electrospray tandem mass spectrometry method was developed and validated for estimation of fulvestrant in rabbit plasma using liquid–liquid extraction. The separation and quantification of fulvestrant were achieved by reverse‐phase chromatography on a Sunfire C₁₈ column (50 × 2.1. i.d., 3.5 μm) with isocratic elution at a flow rate of 300 μL/min using norethistrone as an internal standard from 500 μL plasma sample. The method was validated over the concentration range from 0.092 to 16.937 ng/mL with a lower limit of detection of 0.023 ng/mL. The intra‐day and inter‐day accuracy and precision were within 10%. The recovery was 85 and 90% for fulvestrant and norethistrone respectively. The chromatographic run time was only 2.5 min. Copyright © 2009 John Wiley & Sons, Ltd.     

海藻酸钠水溶液的Sol-Gel转变与凝胶化点的决定

测定了 4个分子量和分子量分布不同、M G不同的海藻酸钠试样在不同浓度下的恒温 (2 5℃ )动态粘弹谱 ,发现 4个试样随溶液浓度升高都会发生溶胶 凝胶 (Sol gel)转变 .实验结果表明 ,该转变符合Winter和Chambon的凝胶化点临界状态的松弛模量G(t)方程 ,由tanδ不依赖于ω的判据求出了海藻酸钠水溶液随浓度变化发生Sol gel转变、出现物理凝胶化的凝胶化点溶液浓度cgel和临界指数n .cgel=7 6wt%～ 8 0wt% ,基本与分子量无关 ;分子量较高的 3个试样的n =0 32～ 0 38,而分子量低的试样的n =0 6 1.该结果表明 ,物理凝胶化主要是由大分子重复单元间的相互作用决定 ,分子链越长则凝胶化点的交联结构越完善     

Development of a large-volume, membrane-based injection system for gradient elution micro-liquid chromatography

A membrane unit which can be used to inject a large volume of sample solution was developed to facilitate reproducible and accurate gradient elution in micro-high-performance liquid chromatography (micro-HPLC). Since the membrane unit has a very low void volume, it facilitates the effective concentration of analytes in large sample volumes. Gradient elution micro-HPLC with the membrane unit allowed the efficient separation of n-alkyl benzoates, used as test samples, in a short time without marked gradient delay. In this study, the membrane unit could be loaded with up to 50 microg of n-hexyl benzoate, and more than 500 microL of sample solution could be applied. In about 50 chromatographic runs, the relative standard deviation (RSD) of the relative retention time of n-hexyl benzoate with respect to methyl benzoate was 0.530%.     

Assessment of the Plasma-Induced Changes under Acidic Conditions in the Apparent Molecular Volume of β-Endorphin, β-Lipotropin and γ-Lipotropin by Gel Permeation and Reversed Phase High Performance Liquid Chromatography

Abstract

Addition of radiolabeled β-endorphin, β-lipotropin and γ-lipotropin to plasma at acid pH results in an apparent reduction in size of these molecules as evidenced by gel permeation chromatography. These acid plasma-treated molecules, however, are indistinguishable from the untreated radiolabeled polypeptides when subjected to high performance liquid chromatographic separations suggesting no differences in molecular composition. As these apparent changes in polypeptide molecular volume are prevented by addition of Trasylol or sodium azide to the plasma, a likely explanation would appear to be an enzyme-dependent production of anionic lipids in plasma which at acid pH bind to the lipotropins and endorphins reducing their molar volume.     

On‐line electroextraction in capillary electrophoresis: Application on the determination of glutamic acid in soy sauces

We present an on‐line, single step coupling between liquid‐liquid extraction and capillary electrophoresis with capacitively coupled contactless conductivity detection, which allows an efficient analysis of complex food matrices with high sodium content. The sodium depletion was demonstrated using an aqueous two‐phase system. The aqueous two‐phase system enables the electrically driven extraction of the target compounds. The sample was prepared in Dextran‐rich phase (8% w/v 500 kDa Dextran, DEX). The background electrolyte (acetic acid 5.0 mol/L) contained 6% w/v of 6 kDa PEG. As proof of applicability, we employed the developed method for glutamic acid quantification on soy sauces. The peak area of glutamic acid presents no significant difference (α = 0.05), while the peak area of the sodium presented a reduction of 11.7 ± 0.2 and 19 ± 3% for premium and low‐cost soy sauce samples analyzed. The glutamic acid concentration for premium soy sauce sample was 2.7 ± 0.8 and 4.8 ± 0.4 g/L, and for low‐cost soy sauce sample, the concentration was 9.9 ± 0.9 g/L, which agreed with those obtained by other analytical techniques.     

Determination of carnitine by high-performance liquid chromatography using 9-anthryldiazomethane

The high-performance liquid chromatographic determination of carnitine chloride was investigated by using 9-anthryldiazomethane (ADAM) as a pre-column derivatization reagent. Carnitine chloride and the internal standard N,N-dimethylglycine reacted with ADAM to give a stable ester derivative in the presence of sodium dodecyl sulphate (SDS) used to mask the basic function. The ADAM derivative of carnitine was separated from decomposition products of the reagent and related compounds such as amino acid derivatives on a silica gel column eluted with methanol-5% aqueous SDS-phosphoric acid (990:10:1). The calibration plot was linear over a sample concentration range from 0.02 to 100 ng per injection. The detection limit for carnitine chloride was about 1 pg per injection (signal to noise ratio = 4), by fluorometric detection.     

Solidified floating organic drop microextraction combined with high performance liquid chromatography for the determination of carbamazepine in human plasma and urine samples

Solidified floating organic drop microextraction (SFODME) in combination with high performance liquid chromatography was used for separation/preconcentration and determination of carbamazepine (CBZ) in human plasma and urine samples. Parameters that affect the extraction efficiency such as the type and volume of extraction solvent, ionic strength, sodium hydroxide concentration, stirring rate, sample volume and extraction time, were investigated and optimized. Under the optimum conditions (extraction solvent, 40 μL of 1-undecanol; sodium hydroxide concentration, 1 mol/L; temperature, 50 ℃; stirring speed, 400 r/min; sample volume, 8 mL; sodium chloride concentration, 3% (w/v) and extraction time, 60 min) the calibration curve was found to be linear in the mass concentration range of 0.4-700.0 μg/L. The limit of detection (LOD) was 0.1 μg/L and the relative standard deviation (RSD) for six replicate extraction and determination of carbamazepine at 100 μg/L level was found to be 4.1%. The method was successfully applied to the determination of CBZ in human plasma and urine samples.     

HPLC Determination of 6-Thiouric Acid and 6-Mercaptopurine in Organ Transplant Patient Serum

Abstract

A sensitive high performance liquid chromatographic method for the simultaneous determination of 6-thiouric acid and 6-mercaptopurine in serum is described. Our intent was to develop a procedure that could be used for pharmacokinetic studies and therapeutic drug monitoring in organ transplant patients taking azathioprine. Serum samples were precipitated with acetonitrile containing 6-n-propyl-2-thiouracil as the internal standard. The chromatographic separation was performed with an octadecylsilane column and gradient solvent system consisting of acetonitrile and 0.01 M sodium dihydrogen phosphate, pH 6.1. An initial acetonitrile concentration of 1% was used to elute 6-thiouric acid but was increased to 16% to recover the 6-mercaptopurine and internal standard. The flow rate was increased from 1.3 ml/min to 1.5 ml/min during the analysis. The column effluent was monitored at 353 nm and 323 nm for detection of 6-thiouric acid and 6-mercaptopurine, respectively. Statistical analysis of standard curve data showed good intra- and inter-day accuracy, precision and reproducibility throughout a concentration range of 10–2500 ng for 6-thiouric acid and 10–500 ng for 6-mercaptopurine/ml of serum. The method has been applied to the quantification of 6-thiouric acid and 6-mercaptopurine in serum from two kidney allograft recipients.