疏水型色谱饼对人血清蛋白质组学样品的快速分离与制备

建立了疏水型色谱饼(10 mm×20 mm i.d.)与反相色谱(RPLC)离线二维色谱快速分离制备人血清蛋白质组学样品,并用基体辅助激光解吸电离飞行时间质谱(MALDI-TOF MS)进行检测的方法。以4种标准蛋白质的稀溶液为模型进行分离富集,得到细胞色素c(Cyt-c)与肌红蛋白(Myo)的检出限均为1 pmol/μL,溶菌酶(Lys)和胰岛素（Ins）的检出限为0.1 pmol/μL。将此方法用于人血清蛋白质组学样品的分离与制备,随着血清处理量的增大,质谱可检出的组分数目与信号强度均增加,当血清处理量达到1.0 mL时,可检出低丰度蛋白质或多肽285个(相对分子质量均在15000以下)。研究中将1 μg Cyt-c加入到0.5 mL血清中,用上述方法在分离富集低丰度Cyt-c上取得了很好的效果。结果表明,采用疏水型色谱饼与反相色谱联用技术不仅可对血清样品中低丰度蛋白质进行有效的分离和富集,而且一次样品的处理量大,可显著提高低丰度蛋白质的分析、检测水平。     

生物色谱用于当归中活性成分筛选及分离研究

应用分子生物色谱技术研究了筛选和分离当归中的活性成分。以甲基丙烯酸缩水甘油酯为功能单体,通过原位聚合得到了整体柱基质,用二乙胺活化后,以吸附蛋白的方法得到了以牛血清白蛋白(BSA)为固定相的分子生物色谱柱。当归样品经甲醇提取,0.45μm膜过滤后,以BSA分子生物色谱柱为分离柱,以含2%(体积分数)甲醇的Tris-盐酸缓冲溶液为流动相进行分离,用二极管阵列检测器检测。结果表明:活性组分在BSA上的保留机理是疏水作用、静电作用和特定的与空间结构相关的多种因素的共同作用结果。将BSA柱上的保留组分进行了气相色谱-质谱分析,鉴定了8种成分,包括当归中的主要可挥发性成分(藁本内酯)。     

开管毛细管亲和液相色谱初探

 提出了一种新的亲和色谱模式开管毛细管亲和液相色谱。在内径为 5 0 μm的毛细管内表面键合一层三嗪染料配体 ,利用毛细管电泳仪的压力系统进行亲和色谱实验。采用流动相切换洗脱技术 ,牛血清白蛋白和溶菌酶获得了有效的分离。连续运行 10次 ,溶菌酶的出峰时间、峰面积和峰高的相对标准偏差分别为0 1% ,4 3% ,3 7%。在 8 6ng～ 2 8 7ng范围内 ,溶菌酶的进样量与峰面积和峰高都呈线性关系 ,其相关系数分别为 0 9946和 0 9988。     

嵌段共聚温敏亲和色谱固定相的制备及其对抗体的分离纯化

抗体药物在癌症治疗和免疫诊断中起着重要作用，但抗体的分离纯化通常采用酸性洗脱，易导致抗体聚集失活等问题。本研究以硅胶为基质，以温敏嵌段聚合物聚[(N-异丙基丙烯酰胺)-b-4-乙烯基吡啶](P[NIPAM-b-4VP])为间隔臂，以4-巯基乙基吡啶(MEP)为配基，制备了一种嵌段共聚温敏亲和色谱固定相SiO₂-P[NIPAM-b-4VP]-MEP,并以牛血清白蛋白(BSA)和γ-球蛋白为模型蛋白，对制备的温敏亲和色谱固定相的色谱性能进行了表征。分别考察了流动相盐浓度和温度对二者分离性能的影响。结果表明，在40℃时该固定相只选择性保留γ-球蛋白，而不保留BSA;在5℃时采用含0.6 mol/L NaCl的Tris-HCl(pH 8.0)缓冲溶液进行洗脱，γ-球蛋白的质量回收率为92.7%。该固定相对γ-球蛋白的吸附量为(71.5±2.1) mg/g(n=3),是传统温敏亲和色谱固定相SiO₂-PNIPAM-MEP的2倍。将该固定相用于人血清中IgG的分离纯化，仅通过改变流动相温度和盐浓度即可一步实现对抗体的分离纯化，纯度大于97.4%±0.7%...     

动力学因素对液相色谱分离整体蛋白的影响

依据液相色谱分离整体蛋白的效果与色谱柱柱长基本无关的事实,研究了动力学因素对疏水相互作用色谱(HIC)分离整体蛋白的影响。首次提出了用于线性梯度洗脱条件下蛋白分离的“条件板高”(H)概念,并将其用于动力学因素对分离整体蛋白的影响的表征。分别用常用的色谱柱和色谱饼对标准蛋白进行了分离,绘制了类似于van Deemter的“条件板高”对流动相线速(u)的曲线图。发现对应于色谱柱最低“条件板高”的适合线速约为色谱饼的1/5～1/15,且色谱饼的适合线速范围也较色谱柱宽得多。据此,用装填有HIC填料的色谱饼(10 mm×20 mm i.d.)在12 min内便可完全分离7种标准蛋白。还用装填有HIC填料的色谱饼对重组人粒细胞集落刺激因子(rhG-CSF)进行了复性并同时纯化,在50 min内,仅用一步色谱法就可获得纯度≥97%的rhG-CSF,其质量回收率为39%,比活＞1×108 IU/mg。可以预计,装填极细颗粒的刚性色谱填料的色谱饼可在高负荷条件下进行整体蛋白的高速和高分离度的分离、纯化并同时复性,达到“三高”。     

用疏水色谱复性并同时纯化蛋白质的机理及其应用

变性蛋白表面的疏水氨基酸残基有与疏水色谱固定相(STHIC)颗粒相互作用的倾向, 两者之间的疏水相互作用能够抑制变性蛋白分子间的相互聚集. 同时疏水色谱固定相还能在分子水平上给变性蛋白分子提供足够高的能量, 使其瞬时脱水并折叠成其天然构象或不同的折叠中间体. 变性蛋白在疏水界面上的折叠不仅取决于其氨基酸之间的特异性相互作用及疏水色谱固定相的结构, 而且还取决于固定相和流动相之间的协同作用. 同时, 还提出了高效疏水相互色谱(HPHIC)进行蛋白折叠的机理及其进行蛋白折叠时能实现质量控制的原理. 在适当的色谱条件下, HPHIC 可使几种变性蛋白一步实现复性及同时纯化. 此外, 还设计制造出了直径比柱长大得多的实验室型和制备型“变性蛋白复性及同时纯化装置, USRPP”, 该“装置”具有完全除去变性剂、使蛋白质复性, 与杂蛋白分离及易于回收变性剂的“一石四鸟”功能. 该“装置”对变性蛋白的复性和纯化效率与通常使用的长柱相当. 在制备规模情况下, 该“装置”可以在低压梯度条件下简便、快速、而经济地应用于重组蛋白药物的制备. 文中以重组人干扰素-γ为例, 说明了制备型“装置”在其复性及同时纯化生产工艺中的应用.     

弱阳离子交换色谱中疏水作用对蛋白保留的影响

选取了四种常用的弱阳离子交换(WCX)商品柱以研究标准蛋白在其上的色谱保留行为。发现在疏水色谱(HIC)模式下,蛋白在这四种WCX商品柱上也有不同程度的保留特征,且洗脱曲线呈现出保留值随盐浓度变化的"U"型。从分子力学角度定性解释了因疏水相互作用力的存在影响了蛋白在WCX色谱柱上洗脱顺序的改变。运用计量置换理论(SDT)中的两组线性方程进一步证实了WCX和HIC中蛋白与固定相间相互作用力的性质,在HIC中为非选择性作用力,而在离子交换色谱(IEC)中为选择性作用力。这四种色谱柱中的两种事实上可在WCX和HIC两种模式下,对标准蛋白进行分离且有较好的分离效果,有可能作为二维色谱柱来使用。     

亲和膜色谱

亲和膜色谱又称亲和膜分离，其在蛋白质的分离纯化中作为一种综合性的技术出现在80年代末。亲和膜色谱主要优点是克服了颗粒状多孔载体扩散传质阻力大的缺点，代之以对流传质，这样就可以在较低的操作压和较高的流速下对目标蛋白进行快速的分离和纯化，从而缩短操作时间、提高纯化效率。本文将就近年来亲和膜色谱及其在蛋白质分离和纯化中的应用作一综述性介绍。     

石油高沸馏分的顶替色谱研究

族组分的制备分离是石油高沸馏分分析中必不可少的先行步骤。本文提出采用常规分析色谱柱以顶替色谱模式取代经典柱色谱完成族组分制备分离,不仅提高了分离效率,缩短了分离时间,而且大大减少了溶剂浪费,降低了手工操作劳动强度。文献中已有将反相高效顶替色谱(HPDC)应用于简单亲水样品(特别是生化样品)组分化合物制备分离的报道,而正相HPDC用于分离复     

序言

色谱柱是色谱分离分析的“心脏”，液相色谱技术的每一次重大进展都与分离固定相的突破密切相关。如上世纪70年代末期高效液相色谱技术的建立和90年代初期“灌流色谱”（Perfusion Chromatography）的发展都是基于多孔硅胶和“穿透孔”分离固定相的发展。近年来，基于特殊孔结构的1．5～2．0μm高强度复合材料的制备成功地催生了超高效液相色谱（UPLC）分离技术，而整体柱材料作为新一代的分离介质，已成为色谱领域广泛研究的前沿课题之一，并已经在样品预处理、手性分离、生物分离分析等领域获得十分广泛的应用。我国色谱研究工作者在多孔硅胶固定相、手性分离固定相、亲和色谱固定相和整体柱固定相等研究领域都取得了重大的进展，有些方面的研究工作已达到或领先于国际先进水平。     

Candida rugosa脂肪酶同工酶的选择固定化

采用DEAE－Sepharose CL-6B离子交换层析，将Candida rugosa脂肪酶（CRL）分成了含同工酶CRL A和CRL B的3个组份，CRL A和CRL B在低水－有机溶剂双液相体系中催化（R，S）－普生甲酯的不对称水解反应，具有不同的对映体选择性。SDS聚丙烯酰胺凝胶电泳分析发现，CRL A和CRL B的分子量几乎相同（约为62000－64000Da)。等电聚焦显示CRL A在等电点pI5.6处有单一条带，CRL B在等电点pI4.2附近有2条带。圆二色谱分析未发现明显结构差异，但在极低的离子强度下它们在疏水载体YWG－C6H5上的吸附速度明显不同。50％异丙醇处理发现，CRL B可解离为CRL A和小分子酸性化合物。据此认为CRL A和CRL B在结构组成上存在着轻微差别，CRL A的活性位点处疏水腔的开放程度较CRL B大，CRL B上非共价结合有一些小分子酸性化合物。据此，分别将其选择性地固定在了疏水性不同的载体YWG－C6H5和YWG－NH2上。本文通过一个简单易行的选择吸附步骤、同时达到了同工酶的分离纯化及固定化目的，提供了一种分离结构上相近的同工酶的便利方法。     

Hofmeister effects in enzymatic activity: weak and strong electrolyte influences on the activity of Candida rugosa lipase

The effects of weak and strong electrolytes on the enzymatic activity of Candida rugosa lipase are explored. Weak electrolytes, used as buffers, set the pH, while strong electrolytes regulate the ionic strength. The interplay between pH and ionic strength has been assumed to be the determinant of enzymatic activity. In experiments that probe activities by varying these parameters, there has been little attention focused on the role of specific electrolyte effects. Here we show that both buffers and the choice of background electrolyte ion strongly affect the enzymatic activity of Candida rugosa lipase. The effects here shown are dramatic at high salt concentration; indeed, a 2 M concentration of NaSCN is able to fully inactivate the lipase. By contrast, Na2SO4 acts generally as an activator, whereas NaCl shows a quasi-neutral behavior. Such specific ion effects are well-known and are classified among the "Hofmeister effects". However, there has been little awareness of them, or of their potential for optimization of activities in the enzyme community. Rather than the effects per se, the focus here is on their origin. New insights into mechanism are proposed.     

Production of native and recombinant lipases by Candida rugosa

The yeast Candida rugosa produces multiple lipase isoenzymes sharing high sequence homology but with some differences in their catalytic properties. The regulation of C. rugosa lipase (CRL) synthesis and secretion in C. rugosa obeys a complex pattern. Fermentation processes for both wild-type and mutant C. rugosa strains are available for lipase production. Native CRL preparations have been extensively used for biotransformations. However, their inherent mixture of isoforms with variable profiles complicates interpretation and brings into question the reproducibility achieved between preparations. Although heterologous CRLs gene expression had been hampered owing to a nonuniversal codon usage, recent advances have made heterologous CRLs available. This will expand and improve the industrial utility of CRLs even further. The purpose of this review is to provide a summary of the recent advances on the production of native and recombinant lipases by C. rugosa.     

Analysis of selected ionic liquid cations by ion exchange chromatography and reversed-phase high performance liquid chromatography

The chromatographic behavior of 8 ionic liquids - 7 homologues of 1-alkyl-3-methylimidazolium and 4-methyl-N-butylpyridinium - has been investigated with a strong cation exchange adsorbent. In particular, the dependence of the retention properties of these solutes on mobile phase composition, pH, and buffer concentration was evaluated with the aim of optimizing and improving the selectivity and retention of solute separation. While using the SCX stationary phase, several interactions occurred with varying strengths, depending on the mobile phase composition. Cation exchange, nonspecific hydrophobic interactions, and adsorption chromatography behavior were observed. Reversed phase chromatography occurred at low concentrations of acetonitrile, electrostatic and adsorption interactions at higher organic modifier concentrations. Elevated buffer concentrations lowered the retention factors without affecting the selectivity of ionic liquids. Obtained results were further compared to the chromatographic behaviour of ionic liquids in the reversed phase system. All analyzed ionic liquids follow reversed-phase behavior while being separated. Much lower selectivity in the range of highly hydrophilic compounds is obtained. This suggests preferred use of ion chromatography for separation and analysis of compounds below 4 carbon atoms in the alkyl side chain.     

Preparation of a silica‐based high‐performance hydrophobic interaction chromatography stationary phase for protein separation and renaturation

In this work, based on the structural characteristics of bio‐membrane molecules, a novel type of high‐performance hydrophobic interaction chromatography stationary phase was prepared using cholesterol as a ligand. Investigating the separation performance of this stationary phase, the effect of pH and salt concentration of the mobile phase on the retention time, the absorption capacity, and the hydrophobic ability revealed that this stationary phase had a high loading capacity and moderate hydrophobic interactions compared with four different hydrophobic interaction chromatography stationary phase ligands. Five types of standard proteins could be baseline separated with a great selection for protein separation. When 3.0 M urea was added to the mobile phase, it could be refolded with simultaneous purification of denatured lysozyme by one‐step chromatography. The mass recovery of lysozyme reached 89.5%, and the active recovery was 96.8%. Compared with traditional hydrophobic interaction chromatography, this new stationary phase has a good hydrophobic ability and a significant refolding efficiency.     

Separation and Immobilization of Lipase from Penicillium simplicissimum by Selective Adsorption on Hydrophobic Supports

Lipases are an enzyme class of a great importance as biocatalysts applied to organic chemistry. However, it is still necessary to search for new enzymes with special characteristics such as good stability towards high temperatures, organic solvents, and high stereoselectivity presence. The present work’s aim was to immobilize the lipases pool produced by Penicillium simplissicimum, a filamentous fungi strain isolated from Brazilian babassu cake residue. P. simplissicimum lipases were separated into three different fractions using selective adsorption method on different hydrophobic supports (butyl-, phenyl-, and octyl-agarose) at low ionic strength. After immobilization, it was observed that these fractions’ hyperactivation is in the range of 131% to 1133%. This phenomenon probably occurs due to enzyme open form stabilization when immobilized onto hydrophobic supports. Those fractions showed different thermal stability, specificity, and enantioselectivity towards some substrates. Enantiomeric ratio for the hydrolysis of (R,S) 2-O-butyryl-2-phenylacetic acid ranged from 1 to 7.9 for different immobilized P. simplissicimum lipase fractions. Asymmetry factor for diethyl 2-phenylmalonate hydrolysis ranged from 11.8 to 16.4 according to the immobilized P. simplissicimum lipase fractions. Those results showed that sequential adsorption methodology was an efficient strategy to obtain new biocatalysts with different enantioselectivity degrees, thermostability, and specificity prepared with a crude extract produced by a simple and low-cost technology.     

稻壳纤维的柱层析性能研究

试验了稻壳纤维作为柱层析介质的性能,并制成亲和层析介质经脂肪酶。结果表明稻壳纤维层析过程为化学物理混合吸附过程,亲和层析性能良好,层析可将脂肪酶纯化２倍,回收率达８１．６％。适合较大规模层析分离。     

Preparation of a weak anion exchange/hydrophobic interaction dual‐function mixed‐mode chromatography stationary phase for protein separation using click chemistry

In this study, 3‐diethylamino‐1‐propyne was covalently bonded to the azide‐silica by a click reaction to obtain a novel dual‐function mixed‐mode chromatography stationary phase for protein separation with a ligand containing tertiary amine and two ethyl groups capable of electrostatic and hydrophobic interaction functionalities, which can display hydrophobic interaction chromatography character in a high‐salt‐concentration mobile phase and weak anion exchange character in a low‐salt‐concentration mobile phase employed for protein separation. As a result, it can be employed to separate proteins with weak anion exchange and hydrophobic interaction modes, respectively. The resolution and selectivity of the stationary phase were evaluated in both hydrophobic interaction and ion exchange modes with standard proteins, respectively, which can be comparable to that of conventional weak anion exchange and hydrophobic interaction chromatography columns. Therefore, the synthesized weak anion exchange/hydrophobic interaction dual‐function mixed‐mode chromatography column can be used to replace two corresponding conventional weak anion exchange and hydrophobic interaction chromatography columns to separate proteins. Based on this mixed‐mode chromatography stationary phase, a new off‐line two‐dimensional liquid chromatography technology using only a single dual‐function mixed‐mode chromatography column was developed. Nine kinds of tested proteins can be separated completely using the developed method within 2.0 h.     

Ion pairing high-performance liquid chromatography of catecholamines

Catecholamine standards have been separated by ion pairing reversed-phase high-performance liquid chromatography (HPLC). A trace substance was separable from four standards when low concentrations of methanol were used in the elution buffer. This method has allowed separation of an unknown uterine catecholamine, partially purified on a boronate affinity gel column, from the standards: norepinephrine, epinephrine, normetanephrine and metanephrine.     

On-column sample preconcentration in electrokinetic chromatography by sweeping with polymeric pseudo-stationary phases

This paper demonstrates in a practical manner the on-column preconcentration of hydrophobic solutes, such as quinine, alkyl phenones, and progesterone, by the sweeping mechanism using polymeric surfactants with highly acidic ionic head groups. The sulfonated and sulfated copolymers used showed high electrophoretic mobilities, high solubility, and good stability in organic/aqueous solutions with low pH values. More than 1000-fold increase in signal was observed for quinine, heptanophenone, and progesterone using sweeping in reversed-flow electrokinetic chromatography at low pH. The detection limit of quinine can be lower than 42 ppb (ng/mL) using a diode array UV detector. Quinine, a cationic hydrophobic solute with a relatively high retention factor, can be concentrated 5800 to 10,000-fold and separated from other hydrophobic solutes using a separation buffer containing a relatively high concentration of organic modifier. Under these conditions, detection of 12.5 ppb of quinine with a signal-to-noise ratio of 15 is achieved. The retention times and peak heights of hydrophobic solutes are shown to be reproducible.