水中硝基苯胺类化合物酶免疫化学分析技术研究

采用戊二醛法, 将4-硝基苯乙胺与牛血清蛋白(BSA)和卵清蛋白(OVA)共价偶联, 分别合成了免疫原4-硝基苯乙胺-BSA和包被原4-硝基苯乙胺-OVA, 经紫外分光光度计及飞行时间质谱扫描鉴定. 用合成的免疫抗原免疫新西兰大白兔, 并用合成的包被原进行间接竞争酶联免疫(ELISA)试验, 获得的抗血清效价达1∶32000. 方阵实验确定了包被抗原最佳浓度(0.5 mg/L)及抗血清最佳稀释度(1∶6000), 并建立了间接竞争ELISA方法. 工作曲线表明在1～1000 μg/L浓度范围内呈良好的线性关系, 该法IC₅₀值为(52.73±2.67) μg/L, 检测限为5.12 μg/L. 其它类似结构不干扰硝基苯胺的测定. 成功地建立了硝基苯胺类化合物的间接竞争酶免疫化学分析方法．     

甲氧基有机磷杀虫剂广谱特异性抗体的制备

以通用结构O,O-二甲基硫代磷酸酯为目标检测基团,制备针对甲氧基有机磷杀虫剂的广谱特异性抗体。利用O,O-二甲基硫代磷酸钠和氯乙酸合成半抗原S-羧甲基-O,O-二甲基二硫代磷酸酯(CMP),通过混合酸酐法(MA)和活性酯法(AE)分别与牛血清蛋白(BSA)和卵清蛋白(OVA)偶联。CMP-MA-BSA、CMP-AE-BSA作为免疫原均获得了免疫应答。其中,CMP-AE-BSA所获得的抗血清效价最高,为256000。研究了有机溶剂种类及含量、pH因素对ELISA曲线的影响,确定CMP酶联免疫分析方法(ELISA)的最佳工作条件,CMP的最低检测浓度为0.076μg/L,IC50为93.97μg/L。以14种常见有机磷杀虫剂为对象,检测抗体对其交叉反应,测定结果表明:抗体对马拉硫磷、稻丰散、乐果、亚胺硫磷、倍硫磷、甲基嘧啶磷、甲基对硫磷、杀螟硫磷及杀扑磷等均有识别作用。IC50分别为69.92、136.90、230.39、416.84、508.57、510.38、607.21、835.30和850.21μg/L。该技术可用于多种甲氧基有机磷杀虫剂的快速定性或半定量检测。     

单纯疱疹病毒抗原的电化学酶免疫法检测及其分型

将酶联免疫吸附试验与单扫描示波极谱法检测相联接，用自制的小型“Ｄｍｅ－Ｐｔ－Ａｇ／ＡｇＣｌ”三电极系统，与商品酶联板配套，直接检测酶促反应电活性产物，建立了ＥＬＩＳＡ－ＬＳＰ法检测单纯疱疹病毒抗原并进行分型的方法。     

双抗体夹心酶联免疫检测法测定蓖麻毒素

建立了双抗体夹心酶联免疫法检测蓖麻毒素的方法。优化了最佳蓖麻毒素多克隆抗体包被浓度和包被方法、蓖麻毒素单克隆抗体工作浓度、酶标记二抗体工作浓度和显色时间等实验条件。方法的线性范围在1.2~10.0μg/L之间,线性回归方程y=0.05x 0.42,相关系数为0.9962,检出限为0.2μg/L。将该方法用于检测实际水样蓖麻毒素加标样品,回收率为91.7%~104.0%;检测实际土壤加标样品,回收率为83.3%~98.0%;检测奶粉加标样品,回收率为83.3%~94.0%;检测实际血液加标样品,回收率为75.0%~82.0%。     

玉米赤霉醇酶标抗原的制备及其直接和间接竞争ELISA检测方法的建立与比较

采用活性酯法将半抗原玉米赤霉醇-16-羧丙基醚与辣根过氧化物酶连接,制备了三种结合比的酶标抗原。通过紫外吸收法和直接非竞争ELISA法对酶标抗原的偶联结果和抗原性进行鉴定。最终选择结合比为1.3∶1的酶标抗原建立直接竞争ELISA检测方法。并对建立的直接竞争ELISA(DC-ELISA)与间接竞争ELISA(IC-ELISA)方法在检出限、检测线性范围、检测时间和二抗的使用方面进行了比较。     

光致变色多孔聚苯乙烯功能微球的制备和性能

以甲苯/庚烷为致孔剂,利用分散聚合技术制备了多孔交联聚苯乙烯微球.研究了聚合单体、引发剂、稳定剂、交联剂等对微球平均粒径的影响,并初步评价了其在常温常压下吸附光致变色材料后的光致变色性能.结果表明,在最佳条件下制得的多孔聚合物微球平均粒径为1 μm;吸附光致变色材料后,其在紫外或日光照射下具有快速可逆的光致变色功能.利...     

生物样品中生物素的酶联免疫吸附分析两种包被方法的比较研究

通过对用猪肺炎霉浆菌包被或用其兔抗体包被两种方法的比较研究，得到一种高灵敏度和高准确度对生物样品中生物素含量直接定量的酶联免疫吸附分析（ELISA）法。猪肺炎霉浆菌包被法的检测限仅约为同类文献值的1／150，加标平均回收率为101.13%，均优于猪肺炎霉浆菌抗血清（抗体）包被法结果。表明猪肺炎霉浆菌比其抗体对酶标板有更强的物理吸附力。方法亦可用于其它待测定物的ELISA法。     

噻虫嗪单克隆抗体制备及酶联免疫吸附分析方法的建立

通过化学修饰合成了噻虫嗪人工半抗原,采用碳二亚胺法将该半抗原与牛血清蛋白(BSA)和卵清蛋白(OVA)偶联,成功制备了分子结合比合理的免疫原和包被原。经过免疫原免疫6周龄Balb/c小鼠、PEG介导免疫鼠脾细胞和骨髓瘤细胞的融合和阳性杂交瘤细胞的筛选和克隆化,获得了效价高达1∶6.4×105的抗噻虫嗪单克隆抗体,抗体亚类为IgG1型。优化了ELISA实验条件,建立了基于单克隆抗体技术的噻虫嗪残留间接竞争ELISA方法。本方法的抑制中浓度(IC50)为0.0255mg/L,检测灵敏度(IC20)为0.0022mg/L,检出限(IC10)为0.001mg/L。除噻虫胺外,该抗体与其它噻虫嗪结构类似物无交叉反应。以自来水为基质的噻虫嗪添加回收实验显示,0.01,0.5和10.0mg/L添加水平的回收率均大于75%,且各添加水平重复测定8次的相对标准偏差均小于8%,说明所建立的间接竞争ELISA准确度高,重复性好,适合水中噻虫嗪残留的检测。     

Preparation of Anti-Cadmium-EDTA Complex Polyclonal Antibody and Its Application for Determination of Cadmium in Aqueous Solution

Abstract

A polyclonal antibody that can recognize cadmium-ethylenediaminetetraacetic acid (CD-EDTA) complex was prepared via the injection of New Zealand white rabbits with Cd-1-(4-isothiocyanatobenzyl) ethylenediamine-N,N,N′,N′-tetraacetic acid–BSA (Cd-ITCBE-BSA). The polyclonal antibody displayed high levels of affinity for Cd-1-(4-isothiocyanatobenzyl) ethylenediamine-N,N,N′,N′-tetraacetic acid-OVA (Cd-ITCBE-OVA) with favorable titer of 1.28 × 10⁶. A simple, reliable, and economical indirect competitive immunoassay based on this polyclonal antibody was developed and validated for detection of cadmium. Assay optimization was performed with respect to chelator concentration, ionic strength, blocking solution, pH, and reaction time. The detection limit of the assay was 0.21 µg L^?1, and the effective linear range was from 10^?1 to 10³µg L^?1. The coefficient of variation (CV) of intra- and interassay were 1.0–8.2% and 2.3–6.9%, respectively. Results yielded low cross-reactivity of the assay to other tested metals such as Pb²⁺, Ni²⁺, Mg²⁺, Ca²⁺, Cu²⁺, Mn²⁺, Zn²⁺, Co²⁺, Cr³⁺, and Fe³⁺, except Hg²⁺, which showed a cross-reactivity of 7.4%. Spike recoveries of ultrapure water, tap water, and samples of the Yangtze River were 85.5–116.3%. These results show that this assay is suitable for quantitative detection of cadmium at trace levels in water samples.     

抗黄曲霉毒素B1多价纳米抗体融合蛋白的构建及活性分析

纳米抗体来源于天然缺失轻链的重链抗体可变区,是已知最小抗原结合单元.该研究构建了抗黄曲霉毒素B1(AFB1)纳米抗体的单价及多价串联体,分别与绿色荧光蛋白(GFP)编码片段融合并克隆至原核表达载体pET30.以大肠杆菌BL21(DE3)作为表达宿主,通过异丙基-β-D硫代吡喃半乳糖苷诱导,亲和层析技术分别纯化单、双及三...     

玉米赤霉醇人工抗原合成及其多克隆抗体的制备

对玉米赤霉醇(ZER)16-OH进行改造,设计合成了模拟玉米赤霉醇特征结构的半抗原———ZER-16-羧丙基丁醚。用混合酸酐法将其与载体蛋白BSA连接,用于免疫新西兰大白兔,制备的抗血清效价达1∶102 400。基于活性酯法合成的包被抗原建立了CI-ELISA检测方法,该法对玉米赤霉醇检测的线性范围为18.39~1744.70 ng/mL,检出限为8.61 ng/mL。     

ILs and MMPs Levels in Inflamed Human Dental Pulp: A Systematic Review

A wide range of mediators are released from the pulp tissue because of bacterial invasion which causes inflammation. Interleukins (ILs) and matrix metalloproteinases (MMPs) have a leading role in initiating and spreading of inflammation because of their synergic action. Biomarkers such as ILs and MMPs can be identified via several methods, establishing the inflammatory response of the dental pulp. The aim of this systematic review is to evaluate the levels of ILs and/or MMPs in human dental pulp. PubMed, OVID, Cochrane, Scopus, Web of Science and Wiley online library databases were searched for original clinical studies. After applying inclusion and exclusion criteria, a quality assessment of studies was performed based on a modified Newcastle-Ottawa scale. In the review were included articles that evaluated the presence of ILs and/or MMPs in pulp tissue using enzyme-linked immunosorbent assay (ELISA) or western blot or multiplex assay. Six articles were included in the present synthesis. Although various diagnostic methods were used, statistically significant higher levels of ILs and/or MMPs were mostly found in the experimental groups compared to healthy pulp samples. The biomarkers studied can be a promising tool to evaluate pulp tissue health or even in pulpitis treatment.     

Development of an enzyme‐linked immunosorbent assay and immunoaffinity chromatography for glycyrrhizic acid using an anti‐glycyrrhizic acid monoclonal antibody

In this work, a new monoclonal antibody specific for glycyrrhizic acid was prepared and characterized. A hybridoma secreting an anti‐glycyrrhizic acid monoclonal antibody was produced by fusing splenocytes from a mouse immunized against a glycyrrhizic acid–bovine serum albumin conjugate with the hypoxanthine–aminopterin–thymidine‐sensitive mouse myeloma cell line (Sp2/0‐Ag14). Subsequently, an indirect, competitive enzyme‐linked immunosorbent assay for glycyrrhizic acid was developed using the monoclonal antibody. In this assay, we detected an effective measuring range of 78.12–2500 ng/mL. Both intra‐assay and inter‐assay repeatability and precision were achieved, with relative standard deviations lower than 10%. In addition, glycyrrhizic acid levels in both formulated Chinese medicines and biological samples were determined with high sensitivity and efficiency. We then successfully developed a reliable immunoaffinity chromatography to separate glycyrrhizic acid completely from its parent medicine. These methods will contribute to further research investigations to better understand the interactions of glycyrrhizic acid with other drugs in the complex system of traditional Chinese medicine.     

Covalent immobilization of single-walled carbon nanotubes and single-stranded deoxyribonucleic acid nanocomposites on glassy carbon electrode: Preparation, characterization, and applications

Single-stranded deoxyribonucleic acid (ssDNA)-wrapped single-walled carbon nanotubes (SWNTs) were modified on the surface of glassy carbon electrode (GCE) by covalent modification technique. Field emission scanning electron microscope (FE-SEM), X-ray photoelectron spectrum (XPS), electrochemical impedance spectroscopy (EIS), and cyclic voltammetric (CV) were used to characterize the properties of this modified electrode. The results showed that SWNTs-ssDNA composites were successfully immobilized onto the surface of GCE. Moreover, this modified electrode exhibited high stability, largely active areas, and efficiently electrocatalytic activities. It had been used for the analysis of various biomolecules, such as dopamine (DA), uric acid (UA), and ascorbic acid (AA), and the results were satisfactory.     

Preparation,Identification, and Preliminary Application of Monoclonal Antibody Against Pyrethroid Insecticide Fenvalerate

Monoclonal antibodies (MAbs) against pyrethroid insecticide fenvalerate were achieved, identified, and applied in environmental water. Mice were immunized with a novel synthesized hapten conjugated with bovine serum albumin (BSA). Three positive clones of MAbs were obtained after cell fusion and hybridoma selection, among them MAb-2 (5B10) showed the highest reactivity toward fenvalerate. The IC₅₀ of MAb-2 was 94.5 ng mL^?1; moreover, it showed lower cross-reactivity with other pyrethroids such as bifenthrin, tetramethrin, deltamethrin and beta-cypermethrin. Optimization of enzyme-linked immunosorbent assay (ELISA) was studied. The limit of detection (LOD) of the assay was 8.8 ng mL^?1 and the detection range was 0.017–27.33 μg mL^?1. For preliminary application, addition recovery experiments in water samples were performed. The mean recoveries of three kinds of samples varied from 90.6% to 108.7% and the coefficients of variation ranged from 0.5% to 5.3%. The results showed that MAb-2 could be used for the detection of fenvalerate contamination in environmental water.     

Preparation and characterization of microcellular polystyrene/polystyrene ionomer blends with supercritical carbon dioxide

The preparation of microcellular polystyrene (PS), lightly sulfonated polystyrene (SPS), zinc‐neutralized lightly sulfonated polystyrene (ZnSPS), and blends of PS/SPS and PS/ZnSPS via supercritical CO₂ was carried out with the pressure‐quench process. Both higher foaming temperature and lower pressure result in larger cell sizes, lower cell densities, and lower relative density for microcellular ionomers and blends as for microcellular PS. The difference among various microcellular samples is the change of cell size with the sample composition. The cell size decreases in the sequence from SPS, through PS/SPS blends, PS and PS/ZnSPS blends, to ZnSPS. The diffusivity of CO₂ in samples also decreases in the sequence from SPS, through PS/SPS blends, PS and PS/ZnSPS blends, to ZnSPS. For this series of samples with similar structure and identical solubility of CO₂, the varying diffusivity is responsible for the difference of cell sizes. © 2003 Wiley Periodicals, Inc. J Polym Sci Part B: Polym Phys 41: 368–377, 2003     

Physicochemical and adsorption properties of hypercross‐linked polystyrene with ultimate cross‐linking density

The paper describes unexpected properties of hypercross‐linked polystyrenes with ultimate cross‐linking degrees of 300, 400, and 500%, where three, four, or five methylene links, respectively, could bind each polystyrene phenyl ring to its spacious neighbors. The polymers exhibit a strong electron spin resonance signal, unusual spectra in IR, UV, and visible ranges, and they are not typical dielectrics. The nonfunctionalized hypercross‐linked polymers absorb significant amounts of inorganic acids, salts, and bases due to interactions of protons or other cations with electron‐donating fragments of the aromatic network with the high extent of mutual connectivity and also due to dispersion interactions of anions with the polymer matrix.     

Novel immunoassay and rapid immunoaffinity chromatography method for the detection and selective extraction of naringin in Citrus aurantium

In this work, a novel monoclonal antibody specific for naringin was prepared and characterized. Subsequently, an indirect competitive enzyme‐linked immunosorbent assay for naringin was developed, with an effective range from 4.8 to 156 ng/mL naringin. Next, an immunoaffinity column was obtained by coupling anti‐naringin monoclonal antibodies to CNBr‐activated Sepharose 4B and a rapid immunoaffinity chromatography assay for naringin was developed. The immunoaffinity column was used to separate naringin from Citrus aurantium. The results showed that 1 g of the dry Sepharose 4B can couple 10 mg of immunoglobulin G. And the immunoaffinity column can efficiently and specifically capture approximately 250 μg of naringin without cross reacting with its structurally similar compounds. Moreover, our results indicate that the application of immunoaffinity chromatography can simplify the pretreatment and the isolation process greatly compared to conventional methods, providing a potential method for extracting the target component from structurally similar compounds in natural products.     

以乙二胺为手臂分子制备的DNA修饰电极及其伏安性能

Carboxyl was formed on the surface of glassy carbon electrode(GCE) by electrochemical oxidation. Ethylenediamine(En) was used as the arm molecule to link carboxyl with dsDNA using 1-ethyl-3-(3-dimethylaminopropyl)-carbodiimide hydrochloride (EDC) and N- hydroxysuccinimide (NHS) as the activators to prepare dsDNA modified electrode(dsDNA/En/GCE). It was shown that dsDNA couM be covalently immobilized on the surface of GCE. ssDNA modified electrode(ssDNA/En/GCE) was obtained via the thermal denaturation of dsDNA/En/GCE. The dsDNA/En/GCE and ssDNA/En/GCE were characterized by voltammetry with methylene blue(MB) as the indicator. The results indicated that the currents of the redox peaks of MB at ssDNA/En/GCE were larger than those at dsDNA/En/GCE, and the currents of the redox peaks at En/GCE were the smallest. The peak-currents of MB at the DNA modified electrode had good reproducibility after multi-denaturation and hybridization cycles.