免疫亲和色谱特异性剔除中药方剂四逆散中的柚皮苷

为了获得剔除柚皮苷(naringin)的中药方剂四逆散样品以供其药理活性探讨时使用,制备了抗柚皮苷抗体的免疫亲和色谱柱,用于特异性地剔除四逆散中的柚皮苷。首先合成了柚皮苷的完全抗原柚皮苷与牛血清白蛋白的结合物naringin-BSA,并用naringin-BSA对新西兰兔进行免疫获得抗血清,再将其纯化后与经CNBr活化的Sepharose 4B凝胶共价偶联制成免疫亲和色谱柱。将四逆散提取物样品溶液上样该色谱柱,洗脱,制得特异性剔除了柚皮苷的四逆散样品。由检测结果可知，naringin-BSA被成功合成。将其用于免疫新西兰兔,获得的抗血清的效价经酶联免疫吸附法（ELISA）测定达到1∶30000,抗体IgG的纯度达94%,交叉反应率低。在IgG与Sepharose 4B合成的IgG-Sepharose免疫亲和色谱柱中,IgG的偶联率为87%。用该免疫亲和色谱柱处理四逆散后,其中所含的柚皮苷几乎完全被剔除。结果证明,利用抗柚皮苷免疫亲和色谱,能特异性地剔除四逆散或其他样品中的柚皮苷成分。     

利用Pen a 1表位抗体亲和纯化目标蛋白的研究

以虾致敏蛋白Pen a 1(Tropomyosin)抗原表位为研究对象,建立了利用Pen a 1表位抗体亲和纯化致敏蛋白的新方法。Fmoc法合成致敏Pen a 1蛋白的C端含有3个抗原表位的第247~284位氨基酸对应的多肽片段,应用马来酰亚胺法将多肽与KLH(匙孔血蓝蛋白)、BSA(牛血清白蛋白)偶联制备人工免疫抗原(Peptide-KLH)和人工包被抗原(Peptide-BSA),免疫人工抗原免疫纯种新西兰白兔,获得多克隆抗血清,抗血清经辛酸-硫酸铵及特异性血清纯化预装柱(HiTrap rProtein A FF)纯化后与溴化氰活化琼脂糖凝4B(CNBrActivated Sepharose 4B)进行偶联。ELISA(酶联免疫吸附试验)测定该多克隆抗体效价为2.05×106,多肽对抗体的IC50(50%抑制浓度)为0.21 mg/L,交叉试验表明该抗体与虾中非Pen a 1蛋白无交叉反应性;Bradford法测定CNBr-Activated Sepharose 4B与抗体的偶联率为90.76%。间接竞争ELISA测定1 mL偶联介质的吸附容量为2.84 mg Pen a 1,免疫亲和柱的加标回收率为89.6%~93.6%,亲和柱使用寿命为4次。     

莱克多巴胺、沙丁胺醇与克伦特罗三合一免疫亲和柱的制备及应用

将莱克多巴胺抗体和克伦特罗抗体偶联到溴化氰活化的琼脂糖凝胶上,制成免疫亲和柱,对其柱性能进行测试,并优化了使用条件,结合高效液相色谱-串联质谱对实际饲料样品进行检测。结果表明:该免疫亲和柱对莱克多巴胺、沙丁胺醇、克伦特罗的柱容量依次为49,27,24 ng/mL胶,保质期为5个月,最佳洗脱液为甲醇,对3种物质的回收率为78.9%~96.5%,RSD均小于1.5%,检出限为0.1~1 ng/g。该法可同时检测饲料中3种瘦肉精的含量。     

克百威的免疫亲和色谱分析研究

 Sepharose CL-4B经碳酰二咪唑(CDI)活化后与纯化的克百威抗体共价偶联,合成了免疫亲和色谱(IAC)固定相,并用其制备了对克百威具有特异性亲和力的IAC柱。对IAC条件进行了优化,选择0.02 mol/L pH 7.2磷酸盐缓冲液(PB)作为吸附与平衡介质,60%（体积分数）甲醇水溶液作为洗脱剂。结果表明:在优化条件下,IAC柱对克百威的动态柱容量达1.58 mg/L。当标样溶液中克百威质量浓度低于 2　μg/L时,经IAC柱富集的效率高于167倍。在河水中按0.1 mg/L水平添加克百威标准品,经IAC柱分离富集,洗脱液采用包被抗体直接竞争酶联免疫吸附分析(ELISA)法检测,5次重复测定的平均回收率为89.8%,相对标准偏差为4.8%。同时采用高效液相色谱(HPLC)法测定洗脱液,与ELISA法测定结果基本一致。     

微囊藻毒素-LR免疫亲和层析柱的研制和应用

用CNBr-activated Sepharose4B和微囊藻毒素-LR的单克隆抗体制备了免疫亲和层析柱,测得抗体偶联率在75.7%~94.1%之间。制得的免疫亲和层析柱最大柱容量在76~95ng之间,柱空白为0,回收率在90.8%~105.1%之间。柱子再生重复使用6次后,回收率不低于75%。建立了免疫亲和层析柱-高效液相色谱测定水样中的微囊藻毒素-LR的方法。该法检出限为5ng/L;线性定量范围为10~500ng/L。实验结果显示,免疫亲和层析柱特异性好,一次净化能除去绝大部分干扰物,净化效果明显优于现有的固相萃取柱。     

环氧活化法制备免疫吸附剂及其对乙型肝炎表面抗原的吸附

分子采用环氧氯丙烷和1,4－二羟基正丁烷双缩水甘油醚活化交联壳聚糖树脂,经偶联抗－乙型肝炎表面抗原（HBsAg)单克隆抗体,制备树脂／抗体免疫吸附剂。含HBsAg的患者阳性血清的吸附实验结果表明,对HBsAg的吸附率可达44％,能使阳性血清转为阴性,通过对不同活化试剂制备的免疫吸附剂的活化过程和吸附性能的研究发现,活化试剂中的“手臂”结构有利于保持偶联抗的天然构象,使之具有较高的活性。     

基于碳纳米管和离子液体复合物修饰电极的免疫传感器检测莱克多巴胺

建立了一种新的电化学免疫传感器方法, 将多壁碳纳米管(MWCNTs)和室温离子液体1-丁基-3-甲基咪唑四氟硼酸盐([BMIM]BF₄)复合物, 和偶联了牛血清蛋白(BSA)的莱克多巴胺抗原, 使用Nafion固定在电极上, 利用莱克多巴胺抗体和抗原之间特定反应的竞争模式, 以K₃Fe(CN)₆为探针, 通过循环伏安法和差分脉冲伏安法监测免疫反应, 对溶液中莱克多巴胺的浓度进行检测. 线性范围宽(1～1500 ng/mL), 检测限可低至0.3 ng/mL. 同时, 我们对猪饲料实际样品进行测定, 回收率令人满意.     

酶解及有机溶剂提取对绵羊血浆和尿样中两种β2-受体激动剂含量测定的影响

采用酶解与有机溶剂提取对绵羊血浆和尿液进行前处理,超高效液相色谱-串联质谱(UPLC-MS/MS)测定两种样品中莱克多巴胺和沙丁胺醇含量,考察了酶解、有机溶剂提取对两种β2-受体激动剂含量测定的影响。结果表明,绵羊血浆中莱克多巴胺轭合率大于95%,沙丁胺醇轭合率约为40%,添加β-葡萄糖醛苷酶/芳基硫酸酯酶进行酶解可有效解离血浆中轭合的莱克多巴胺和沙丁胺醇,测得的含量显著提高;不经酶解处理血浆中莱克多巴胺、沙丁胺醇检测结果的相对偏差均大于40%,重复性差;绵羊尿液中莱克多巴胺轭合率约为57%,沙丁胺醇轭合率低于1%,酶解后尿液中莱克多巴胺检测结果显著提高,对于沙丁胺醇含量测定无显著影响;血浆样品基质复杂程度低于尿液样品,血浆样品目标化合物的基质抑制效应小于尿液样品;有机溶剂提取对血浆和尿液中莱克多巴胺和沙丁胺醇含量检测结果影响不显著,提取过程存在目标化合物损失的可能性,通过内标校正,可消除提取损失对检测结果的影响。     

莱克多巴胺-印迹聚合物微球的制备及其色谱表征

以莱克多巴胺为模板分子,甲基丙烯酸为功能单体,乙二醇二甲基丙烯酸酯为交联剂,乙醇为致孔剂采用沉淀聚合法合成了对莱克多巴胺具有高特异识别性的分子印迹聚合物,平衡吸附量达145.6μg/g微球。将制备的印迹聚合物微球装填高效液相色谱柱(50 mm×4.6 mm i.d.)。印迹柱的印迹因子(IF)为1.2,印迹柱和非印迹柱的保留因子(k)分别为33.3和15.1,表明合成聚合物印迹效果明显。分别用10μg/mL克伦特罗、沙丁胺醇和莱克多巴胺3种β-兴奋剂溶液考察自制高效液相色谱柱的分离效果,克伦特罗和沙丁胺醇的选择性系数(α)分别为2.3和1.2,表明所制备的分子印迹柱对以上3种β-兴奋剂显示了良好的选择性。     

在线固相萃取-高效液相色谱-质谱法快速测定绵羊尿液中3种轭合态β-受体激动剂

采用双三元高效液相色谱和液相质谱联用(HPLC-MS/MS)建立了测定绵羊原始尿液及酶解后尿液中β-受体激动剂(沙丁胺醇、克伦特罗、莱克多巴胺)在线SPE(Turboflow)检测的方法。分别对Turboflow柱和分析柱条件进行优化,最终确定样品上样速率4 m L/min,进样体积100μL,样品净化时间0.5 min。本方法的回收率在91.3%~112.2%之间,线性范围为0.1~100μg/L,精密度RSD<1%,日间峰面积RSD<12%,说明方法的重现性和稳定性良好。在对酶解后的尿液检测中发现,对于苯酚类β-受体激动剂(沙丁胺醇、莱克多巴胺),酶解后的尿液中检出化合物含量明显高于未酶解样品,对苯胺类β-受体激动剂(克伦特罗)的影响不大。本方法只需对原始尿液或酶解后的尿液进行过膜处理,样品的在线净化、富集、柱平衡和最终分析可在15 min内完成,大大缩短了日常分析所需时间。本方法操作简单,可用于养殖动物β-受体激动剂大规模筛查。     

Improvement of the performance of an immunoaffinity extraction method via region-specific immobilization of IgG

Using papaverine as a model target, an immunoaffinity column of high selectivity and binding capacity was prepared by utilizing covalent linkage between the Fc portion of IgG and the surface of Sepharose 4B support. Compared with the commonly used random coupling method, the binding capacity of the region-specific immobilized antibodies was increased from 0.04 to 0.2 mol of antigens/mol of antibodies and a much larger concentration factor was thus achieved. The obtained immunoaffinity column has been successfully used in pretreatment of pericarpium papaveris samples. The method offers an improved approach to immunoaffinity extraction that should be useful for purification and concentration of other targeted compounds in highly complex mixture.     

Oriented immobilized anti‐hIgG via Fc fragment‐imprinted PHEMA cryogel for IgG purification

Antibodies are used in many applications, especially as diagnostic and therapeutic agents. Among the various techniques used for the purification of antibodies, immunoaffinity chromatography is by far the most common. For this purpose, oriented immobilization of antibodies is an important step for the efficiency of purification step. In this study, F_c fragment‐imprinted poly(hydroxyethyl methacrylate) cryogel (MIP) was prepared for the oriented immobilization of anti‐hIgG for IgG purification from human plasma. Non‐imprinted poly(hydroxyethyl methacrylate) cryogel (NIP) was also prepared for random immobilization of anti‐hIgG to compare the adsorption capacities of oriented (MIP/anti‐hIgG) and random (NIP/anti‐hIgG) cryogel columns. The amount of immobilized anti‐hIgG was 19.8 mg/g for the NIP column and 23.7 mg/g for the MIP column. Although the amount of immobilized anti‐hIgG was almost the same for the NIP and MIP columns, IgG adsorption capacity was found to be three times higher than the NIP/anti‐hIgG column (29.7 mg/g) for the MIP/anti‐hIgG column (86.9 mg/g). Higher IgG adsorption capacity was observed from human plasma (up to 106.4 mg/g) with the MIP/anti‐hIgG cryogel column. Adsorbed IgG was eluted using 1.0 m NaCl with a purity of 96.7%. The results obtained here are very encouraging and showed the usability of MIP/anti‐hIgG cryogel prepared via imprinting of Fc fragments as an alternative to conventional immunoaffinity techniques for IgG purification. Copyright © 2012 John Wiley & Sons, Ltd.     

Removal of poliovirus type 1 from a protein mixture using an immunoaffinity chromatography column.

An immunoaffinity matrix was prepared using human polyclonal antibody (Intragam) attached to Sepharose 4B activated with CNBr. The immunoaffinity matrix was then assessed with regard to its capacity to remove viruses. The challenge virus, poliovirus type 1 was loaded in high titre in either PBS or a preparation derived from human plasma known as supernatant II + III. This fraction is depleted of IgG and is used to prepare human albumin. It was shown that an average greater than 5 logs of spiked virus were removed in one passage through the column. This type of approach may prove useful as a viral removal method in biopharmaceutical manufacturing.     

Preparation of immunoaffinity mini-columns for the analysis of platelet activating factor (PAF) in biological samples.

Using an antibody to BN 52719, an analogue of platelet activating factor (PAF), immunoaffinity mini-columns for the separation of PAF from biological samples were prepared. Rabbits were immunized with BN 52719 and immunoglobulin G (IgG) from the antiserum was coupled with Sepharose 4B. The resulting suspension of the IgG-coated Sepharose 4B in 25 mM phosphate buffer (pH 6.9) was poured into a plastic mini-column (bed volume 2.0 x 0.8 cm). Stepwise elution of the column with methanol revealed that lyso-PAF is eluted with 20-30% methanol in water whereas PAF is eluted with 50-80% methanol. For the determination of PAF in biological samples, it is recommended that lipids are extracted from the samples and the extract, reconstituted in 20% methanol, is loaded on the column. The column is then washed with 50% methanol followed by elution of PAF with 80% methanol. A small amount of [3H]PAF is added to the samples for measurement of the recoveries of PAF during the procedures of extraction and elution. The PAF is then quantified by radioimmunoassay or bioassay. Employing the immunoaffinity mini-column and radioimmunoassay, the contents of PAF in macrophages and conditioned medium after stimulation with calcium ionophore A23187, or tumor promoters such as TPA and thapsigargin, were measured.     

Development and characterisation of an immunoaffinity chromatographic column for the on-line determination of the pesticide triclopyr

An immunoaffinity column for the selective extraction and concentration of the herbicide triclopyr from water samples and quantification on line by HPLC has been developed. The immunoaffinity device was prepared by immobilising triclopyr antibodies to hydrazide derivatized azlactona beds. Efficient desorption of bound triclopyr was achieved with 70% ethanol/water solution. The column was evaluated regarding selectivity, recovery, capacity, saturation volume and reusability. Obtained results show that immunoaffinity chromatography (IAC) can be used for quantitative extraction, concentration and determination of triclopyr from water samples.     

Spectral and fluorescent kinetics features of Nd3+ ion in Nb2O5, Ta2O5 and La2O3 mixed lithium zirconium silicate glasses

A sensitive competitive flow injection chemiluminescence (CL-FIA) immunoassay for immunoglobulin G (IgG) was developed using gold nanoparticle as CL label. In the configuration, anti-IgG antibody was immobilized on a glass capillary column surface by 3-(aminopropyl)-triethoxysilane and glutaraldehyde to form immunoaffinity column. Analyte IgG and gold nanoparticle labeled IgG were passed through the immunoaffinity column mounted in a flow system and competed for the surface-confined anti-IgG antibody. CL emission was generated from the reaction between luminol and hydrogen peroxide in the presence of Au (III), generated from chemically oxidative dissolution of gold nanoparticle by an injection of 0.10 mol L⁻¹ HCl–0.10 mol L⁻¹ NaCl solution containing 0.10 mmol L⁻¹ Br₂. The concentration of analyte IgG was inversely related to the amount of bound gold nanoparticle labeled IgG and the CL intensity was linear with the concentration of analyte IgG from 1.0 ng mL⁻¹ to 40 ng mL⁻¹ with a detection limit of 5.2 × 10⁻¹⁰ g mL⁻¹. The whole assay time including the injections and washing steps was only 30 min for one sample, which was competitive with CL immunoassays based on a gold nanoparticle label and magnetic separation. This work demonstrates that the CL immunoassay incorporation of nanoparticle label and flow injection is promising for clinical assay with sensitivity and high-speed.     

Preparation and characterization of an immunoaffinity column for the selective extraction of salbutamol from pork sample

A rapid, simple, and reliable determination method for salbutamol in pork was developed with immunoaffinity column (IAC) extraction followed by HPLC analysis. The salbutamol immunoaffinity column was prepared by coupling CNBr-activated Sepharose-4B with the anti-salbutamol polyclonal antibody which was purified by caprylic acid-ammonium sulfate. The coupling rate of the antibody and Sepharose-4B was 98.6%, and the dynamic column capacity of IAC was 400 ng/mL gel. The average recoveries of salbutamol from spiked pork samples at levels of 2, 10, 20, and 50 ng/g ranged from 83.3% to 92.2%, with the relative standard deviations of 2.8-7.0% (n=5), and the limits of detection and qualification were 0.25 ng/g and 0.5 ng/g, respectively.     

Immunoaffinity column as sample cleanup method for determination of the beta-adrenergic agonist ractopamine and its metabolites

A monoclonal antibody-based immunoaffinity column (RAC-IAC) was developed as a cleanup method for the determination of ractopamine and ractopamine glucuronides. [14C]Ractopamine (5 microg) and [14C]ractopamine glucuronides (5 microg) were fortified into 10 mL cattle urine, and loaded onto an RAC-IAC (5 mg IgG/mL) column. The column was washed and the bound analytes were eluted. In the initial loading and washing, 22% of the radioactivity was washed off and the subsequent elution step recovered 78%. A blank column prepared from nonspecific IgG retained <10% of the radioactivity. The RAC-IACs were damaged by high methanol concentrations, preventing reuse. Elution of the analytes with 50mM glycine buffer, pH 2.8, prevented damage, and the columns could be reused at least 20 times with no change in performance. They were stored >3 months in phosphate-buffered saline with 0.02% sodium azide at 4 degrees C. The method was used with fortified cattle muscle, liver, and kidney samples with recoveries of 82.1+/-7.6, 87.8+/-1.9, and 92.5+/-0.4%, respectively (n = 3). Similar studies with sheep muscle, liver, and kidney samples gave recoveries of 91.8+/-0.2, 91.7+/-0.3, and 92.3+/-0.3, respectively (n = 3). Liver and kidney samples were diluted to prevent column plugging, but all of the eluants were suitable for liquid chromatography analysis. This IAC is a selective, efficient, and economical cleanup method in a variety of matrixes for ractopamine determination.     

An immunoaffinity column for the determination of peanut protein in chocolate.

An immunoaffinity column was prepared from rabbit polyclonal antiserum for the determination of peanut protein from food matrixes. The anti-peanut immunoglobulin G was isolated from antiserum by affinity chromatography on a column coupled with peanut protein and then attached to an AminoLink gel. The column was applied to the determination of peanut protein in chocolate after extraction, immunoaffinity chromatography, and enzyme-linked immunosorbent assay (ELISA). Overall recoveries from chocolate spiked with 0.2-3.2 micrograms/g of peanut protein averaged 77% (range, 72-84%), and the minimum detection limit was 0.1 microgram/g. Chromatography of extracts with the column improved detection limit and eliminated the matrix effect experienced with direct ELISA of chocolate extracts.