两种谷胱甘肽亲和层析介质的制备及其对谷胱甘肽转移酶融合蛋白的纯化

以国产交联琼脂糖6FF为基质,分别以环氧氯丙烷(ECH)、1,4-丁二醇二缩水甘油醚(BDGE)为活化剂,偶联谷胱甘肽(GSH)得到两种连接臂长度不同的GSH亲和层析介质,并以两种自制介质对融合蛋白GST-ADAM15进行了纯化。结果表明:GSH-ECH-琼脂糖凝胶和GSH-BDGE-琼脂糖凝胶的配基密度分别达到了30～35μmol/mL和15～18μmol/mL,经两种介质纯化后的GST融合蛋白,纯度均达到95%以上,BDGE活化对目标蛋白的回收率占总蛋白26%,ECH活化为13%。相对而言,由于连接臂长度的不同,BDGE活化的介质纯化效果优于ECH。     

一种孔雀石绿免疫亲和柱及其制备方法和用途

<正>申请公布号:CN104174185A申请公布日:2014.12.03申请人:北京美正生物科技有限公司摘要本发明涉及一种孔雀石绿免疫亲和柱制备方法及其用途。该免疫亲和纯化柱利用蛋白G偶联到琼脂糖凝胶上载体,然后用抗孔雀石绿的抗体与琼脂糖上的蛋白G偶联。再利用交联剂对结合孔雀石绿抗体的蛋白G–琼脂糖凝胶载体进行交联。用交联后的载体制备免疫亲和柱。该纯化柱     

增强型绿色荧光蛋白的色谱分离和纯化

增强型绿色荧光蛋白(EGFP)是生物领域常用的标记物。在前期成功克隆表达EGFP的基础上,本实验建立了两步分离纯化EGFP的色谱方法,并验证其分离纯化效果,检验EGFP的活性。首先用金属螯合亲和色谱柱HisTrap HP对EGFP的重组菌体破碎上清液进行初步分离,再用葡聚糖凝胶排阻色谱柱Sephadex G-10 HR对其进行脱盐纯化。采用丙烯葡聚糖凝胶排阻色谱柱Sephacryl S-300 HR和十二烷基磺酸钠-聚丙烯酰胺凝胶电泳(SDS-PAGE)检测分离纯化后的EGFP纯度。最后通过荧光分光检测器和非变性聚丙烯酰胺凝胶电泳(Native-PAGE)验证分离纯化后的EGFP是否具有荧光活性。结果表明该方法可以简便快速地分离纯化EGFP,纯度超过98%,同时保持了EGFP的荧光活性。     

克拉维酸钾及主要原料中大分子蛋白杂质的测定EI北大核心CSCD

建立了凝胶排阻色谱对克拉维酸钾及其原料克拉维酸叔辛胺中的残余蛋白进行检测的方法。采用TSK gel G3000 SWXL凝胶色谱柱(5μm,7.8×300 mm),流动相为磷酸盐缓冲溶液,流速为0.8 m L/min,紫外检测波长为220 nm。对照品牛血清白蛋白(BSA)在0.249~49.9μg/m L内线性关系良好(R2=0.9997),平均回收率为101.2%,RSD为0.7%,检测限为0.05μg/m L。方法为同类药物中的大分子蛋白检测提供了有效手段。     

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。     

离子交换层析介质Q-琼脂糖凝胶的合成和吸附性能研究

以琼脂糖凝胶为基质，经2，3-环氧丙基三甲基氯化铵反应后，制得强碱型阴离子交换树脂Q-琼脂糖凝胶．考察了该反应的主要影响因素，并研究了对BSA蛋白质的吸附和对GL-7ACA酰化酶的分离性能，结果表明，其吸附性能、分离纯化性能均与国外同类产品相近。     

体积排阻色谱-电感耦合等离子体质谱分析富硒大米含硒蛋白组成

建立体积排阻色谱-电感耦合等离子体质谱(SEC-HPLC-ICP-MS)联用技术分析富硒大米含硒蛋白组成方法。通过水提、盐提、碱提和醇提方法提取,并用丙酮沉淀蛋白,硒的回收率分别为9.6%,16.8%,48.2%和14.9%,纯化后的蛋白结合硒的量由大到小依次为碱溶谷蛋白>球蛋白>醇溶蛋白>清蛋白。蛋白液经SEC-HPLC-ICP-MS检测,通过蛋白色谱峰(λ=280 nm)和ICP-MS硒峰(78Se)对比分析,利用分子量标准曲线测定出4类蛋白中含硒蛋白的分子量。结果表明,富硒大米中清蛋白和醇溶蛋白并不是硒的主要存在蛋白。硒主要存在于>7 kDa的碱溶谷蛋白和球蛋白,其中碱溶含硒蛋白主要组分F1分子量为199.8 kDa。     

琼脂糖凝胶蛋白芯片片基的制备及应用

建立了一种制备琼脂糖凝胶修饰玻片的方法。以乙肝表面抗原为检测指标,比较了琼脂糖凝胶片基和常规的醛基片基固定抗体后的检测灵敏度,发现琼脂糖凝胶修饰后可以明显增加检测的荧光强度,并在10ng/L～100μg/L之间具有良好的线性关系。在此片基同时固定了抗HBsAg和抗HBeAg抗体,并以牛血清白蛋白和生物素标记抗体为阴性和阳性对照点,采用夹心式免疫反应法检测乙肝病毒的两种抗原,取得良好效果。     

氢化物发生-原子荧光光谱法(HG-AFS)测定特硬铅合金中硒和碲

建立了氢化物发生-原子荧光光谱法(HG-AFS)测定特硬铅合金中硒和碲的分析方法。试样经硝酸和酒石酸溶解,硫酸沉淀分离基体铅元素。移取部分试液,在40%盐酸介质中直接用氢化物发生-原子荧光光谱法(HG-AFS)测定样品中的硒;另移取部分试液,加入氢溴酸挥发除去砷、锑、锡、硒等元素,在40%盐酸介质中用氢化物发生-原子荧光光谱法(HG-AFS)测定样品中的碲。考察了测定的最佳条件、铅及共存元素对测定的影响。测定硒和碲的相对标准偏差分别为7.5%～9.3%和3.6%～13.0%,加标回收率分别为88%～92%和98%～102%。准确度和精密度均能满足分析需要,具有较强的实用性。     

氢化物发生-原子荧光光谱法测定高纯阴极铜中硒、碲

本文报道了采用氢化物发生-原子荧光光谱法(HG-AFS)测定高纯阴极铜中硒、碲。实验考察了盐酸、三氯化铁的浓度对氢化物发生效率的影响,探讨了铜和其它共存元素的干扰情况。该法测定硒、碲的检出限分别为0.27μg/L、0.11μg/L,加标回收率分别为94.9%～114.0%、91.8%～105.3%,精密度为1.5%～7.8%。     

微波消解-氢化物发生-原子荧光光谱法测定出口芳香油中痕量铅

采用微波消解技术溶样,氢化物发生-原子荧光光谱法测定了出口芳香油中痕量铅.系统地研究了微波消解、氢化物发生的最佳条件,方法简便快速,在选定的实验条件下,方法检出限为0.25 μg·L~(-1),相对标准偏差小于5%,回收率为86.5%～100.5%.     

Affinity Chromatography of Ribitol Dehydrogenase,a Possible New Zinc Enzyme from Mycobacterium Butyricum

Abstract

An effective purification procedure of ribitol dehydrogenase (RDH), a possible new zinc enzyme from Mycobacterium butyricum is described. The procedure took advantage of different chromatographic methods in which the most significant were two affinity chromatography steps. One of them was the immobilized metal ion affinity chromatography (IMAC), with the use of iminodiacetate-Sepharose 6B (IDA-Sepharose 6B) chelating Zn²⁺ ions (IDA-Zn) as an affinity sorbent. The enzyme was eluted with a decreasing pH gradient from 7 to 4. The other step was a biospecific affinity chromatography, where the enzyme retained on 5′ AMP-Sepharose 6B was eluted with 10 mM adenosine 5′-monophosphate (AMP). RDH was purified 174-fold with 10.2% of recovery, and the final preparation was homogenous in polyacrylamide gel electrophoresis.     

Determination of Inorganic Sb(V) and Methylantimony Species by HPLC with Hydride Generation-Atomic Fluorescence Spectrometric Detection

 An on-line method for the separation and analysis of Sb(V) and Me₃Sb in the presence of Sb(III) in liquid samples is described. Inorganic and organic antimony species were separated using anion-exchange high-performance liquid chromatography (HPLC) coupled with hydride generation-atomic fluorescence detection (HG-AFS). Optimum conditions for the separation of antimony species by HPLC and the hydride generation conditions for the determination by HG-AFS were established. Matrix interference of the chromatographic determination was studied in relation to MgSO₄ and NaCl. The method developed was applied to the separation and determination of antimony species in spiked and natural water samples. The suitability of the method for analysis in microbial growth media and physiological studies involving methylantimony species is discussed. Received December 11, 2000. Revision April 26, 2001.     

Refolding and purification of rhNTA protein by chromatography

RhNTA protein is a new thrombolytic agent which has potential medicinal and commercial value. Protein refolding is a bottleneck for large‐scale production of valuable proteins expressed as inclusion bodies in Escherichia coli. The denatured rhNTA protein was refolded by an improved size‐exclusion chromatography refolding process achieved by combining an increasing arginine gradient and a decreasing urea gradient (two gradients) with a size‐exclusion chromatography refolding system. The refolding of denatured rhNTA protein showed that this method could significantly increase the activity recovery of protein at high protein concentration. The activity recovery of 37% was obtained from the initial rhNTA protein concentration up to 20 mg/mL. After refolding by two‐gradient size‐exclusion chromatography refolding processes, the refolded rhNTA was purified by ion‐exchange and affinity chromatography. The purified rhNTA protein showed one band in SDS‐PAGE and the specific activity of purified rhNTA protein was 110,000 U/mg. Copyright © 2008 John Wiley & Sons, Ltd.     

HG-AFS 法测定多金属矿中的痕量锡

研究了酒石酸介质中氢化物发生原子荧光光谱法 ( HG- AFS)测定多金属矿中痕量锡的方法 ,考察了不同酸介质和浓度对氢化物发生效率的影响 ,试验了共存元素的干扰情况。方法的检出限为 1 .4× 1 0 - 10 g/ m L,精密度 ( n=5)为3.71 %～ 5.38%。     

Hydride Generation Atomic Fluorescence Spectrometric Determination of Ultratrace Arsenic in High Purity Indium Oxide

A simple, sensitive, and interference free method was proposed for the determination of total arsenic in high purity indium oxide by hydride generation atomic fluorescence spectrometry (HG-AFS). Preconcentration was carried out by distillation of volatile arsenic trichloride. Hydrazine sulfate was used as a prereductant to reduce As (V) to As (III). The volatile arsenic trichloride generation was based on the reaction between As (III) and hydrochloric acid, and vapors were absorbed with water. The method provides a linear response range of 2 ng/mL–70 ng/mL, a detection limit of 0.1 ng/mL, a recovery of 96%–113%, and an average relative standard deviation of 2.42%. The method was validated by means of interlaboratory comparative analysis with the proposed method HG-AFS, and the comparison of data by using proposed method HG-AFS and reference methods of ICP-OES and spectrophotometry.     

Superoxide chemical transformation of diolepoxide polyaromatic hydrocarbon DNA adducts. Determination of benzo[a]pyrene-r-7,t-8,9,c-10-tetrahydrotetrol by gas chromatography.

Benzo[a]pyrene-r-7,t-8,9,c-10-tetrahydrotetrol (100 pg, 342 fmol) was measured using the following sequence of steps: (1) chemical transformation with potassium superoxide to 2,3-pyrenedicarboxylic acid; (2) electrophore derivatization with pentafluorobenzyl bromide; (3) sample clean-up by high-performance liquid chromatography and (4) measurement by gas chromatography with electron-capture detection and by gas chromatography with electron-capture negative-ion mass spectrometry. The overall, absolute yields obtained by the two procedures were 69% and 60%, respectively. This work completes the first stage towards the establishment of a general method for detecting diolepoxide polyaromatic hydrocarbon DNA adducts by gas chromatography.     

质谱法分析大肠癌组织中踝蛋白的磷酸化修饰

踝蛋白的磷酸化修饰,特别是肿瘤等病理条件下的踝蛋白磷酸化状态,与肿瘤的发病、转移机理密切相关。本研究采用盐析、离子交换层析和电泳分离并纯化了人大肠癌组织中的踝蛋白(Talin),经胰酶水解获得其肽段混合物,进一步分别利用固定化Fe3+亲和层析和TiO2亲和层析在酸性条件下对其中磷酸化修饰肽段进行吸附,并以1%氨水进行洗脱。在Michrom Magic C18色谱柱上,以A:99%水+1%乙腈+0.1%甲酸和B:99%乙腈+1%水+0.1%甲酸两种流动相进行梯度洗脱分离,采用ESI质谱进行依赖数据的二级子离子扫描。结果显示,固定化Fe3+富集到8个磷酸化肽段而TiO2富集到9个磷酸化肽段。本研究提供了一种快速、准确地鉴定从人大肠癌组织中分离表征踝蛋白的方法。     

Simultaneous Determination of Arsenic and Lead in Vegetable Oil by Atomic Fluorescence Spectrometry after Vortex-Assisted Extraction

Hydride generation atomic fluorescence spectrometry (HG-AFS) is used for the determination of hydride-forming elements due to its high sensitivity, simplicity, and low cost. A new HG-AFS method for the simultaneous determination of arsenic and lead in vegetable oil is reported. Vortex-assisted extraction with dilute nitric acid was used to isolate arsenic and lead from vegetable oil. The conditions influencing the fluorescence signal, including the carrier fluid, oxidizing agent, and reducing agent, were optimized. The interferences of coexisting ions were also evaluated. Under the optimized conditions, the limits of detection were 0.6 and 0.4?µg?kg^?1 for arsenic and lead. The recoveries were from 84.4 to 105% for both metals in vegetable oil. The optimized method was used for the determination of arsenic and lead in commercial vegetable oil. The analytical results by this approach were in good agreement with values obtained by inductively coupled plasma mass spectrometry with microwave digestion.     

A study of low level selenium determination by hydride generation atomic fluorescence spectrometry in water soluble protein and peptide fractions

Development of a method for very low level selenium determination in water soluble protein and peptide fractions, obtained after various separation procedures, is presented. A hydride generation atomic fluorescence spectrometry (HG-AFS) detection system was optimised and the influence of Cu(II), Sb(V), As(III) and HNO₃ interferences in the measurement of Se by HG-AFS was investigated. A destruction procedure using HNO₃ and H₂O₂ was also optimised and the average recovery of the digestion of a solution of selenomethioneine was 92 ± 4% (n=14). Combination of this digestion with the detection system gave reliable results. Accuracy was tested by comparison with two independent methods. A very low detection limit (DL) of 0.2 ng/g of measuring solution was achieved. The whole procedure from weighing to measuring was performed in the same Teflon tube. The addition of HNO₃ to the fractions before long term storage at -20°C was necessary to prevent adsorption on the test tubes.Selenium was measured in water soluble protein and peptide fractions obtained after extraction, and Sephadex G-75 chromatography performed on liver samples from: i) hens exposed to As₂O₃, ii) hens fed with a high fat feed and iii) the certified reference material dogfish liver (CRM DOLT-2). Because of the very low DL we were able to observe the Se distribution in chromatographic fractions of samples of organisms which were not exposed to excess amounts of Se. The presence of selenium associated with metallothioneins was observed.