胶体金免疫层析法快速检测牛奶、奶粉、饲料中的三聚氰胺

建立了快速检测牛奶、奶粉、饲料样品中三聚氰胺的胶体金免疫层析分析法。将三聚氰胺进行分子修饰得到两种衍生物,分别与牛血清白蛋白(BSA)和卵清白蛋白(OVA)相连制得免疫原和包被抗原。运用杂交瘤抗体制备技术得到抗三聚氰胺的单克隆抗体(mAb)。利用柠檬酸三钠还原法制得平均粒径18 nm的胶体金,将胶体金与抗三聚氰胺单克隆抗体相连,所形成的金标抗体(Au-mAb)包被在胶体金垫上,包被抗原和羊抗鼠二抗分别包被在硝酸纤维素膜(NC)上作为检测线(T线)和质控线(C线)。将胶金垫、NC膜、样品垫和吸水纸组装成免疫层析快速检测试剂条。将标准溶液(或待测液)滴加到样品垫上,10 min后可在NC膜C线和T线位置上用肉眼观察到胶体金的颜色(红色),通过比对颜色的深浅判断样品中三聚氰胺的含量。结果表明,三聚氰胺的检出限为10μg/L;选用了其它10种物质对免疫层析试剂条进行了特异性实验,免疫层析试剂条与2-氯-4,6-二氨基-1,3,5-三嗪和环丙氨嗪的交叉反应率约为1%,与其它8种物质没有交叉反应;加标样品用免疫层析试剂条和酶联免疫吸附分析法(ELISA)同时检查,结果一致。本方法适用于牛奶、奶粉、饲料样品中三聚氰胺的现场快速检测。     

胶体金免疫层析法快速检测水产品中河豚毒素的研究

该文将特异性识别河豚毒素的单克隆抗体加以胶体金标记用作示踪物,建立了豚毒素的胶体金免疫层析技术快速检测方法。优化了胶体金体系的pH值、抗原抗体浓度、离子浓度、表面活性剂种类以及样品前处理方法。结果显示：在最优条件下,建立的胶体金免疫层析法对河豚毒素的定量检出限为0.5 ng/mL,线性范围为0.8～10.6 ng/mL,定性检出限（裸眼判别）为12.0 ng/mL。河豚、织纹螺等样品的加标回收率为70.5%～110%,相对标准偏差为3.7%～7.1%,检测结果与LC-MS/MS法一致。所建立的胶体金免疫层析技术在现场快速检测方面具有良好的可行性和实用性,可用于大量样品的快速筛查和河豚毒素中毒后的快速诊断。     

胶体金免疫层析法快速检测腹泻性贝毒软海绵酸的研究

腹泻性贝毒是一类分布较广的赤潮毒素,严重威胁到人类的健康和安全。本文用胶体金标记利用细胞融合技术制备的抗软海绵酸单克隆抗体,使用卵清蛋白合成高偶联比的包被抗原,以硝酸纤维素膜为载体,利用免疫层析技术原理,建立了快速检测软海绵酸的免疫层析试纸条方法。方法检出限12 ng/mL(0.96纳克/条)。     

猪肉中1-氨基乙内酰脲的胶体金免疫层析法快速检测

基于免疫竞争胶体金免疫层析原理,研制了检测食用肉中呋喃妥因代谢物1-氨基乙内酰脲(AHD)的免疫试纸条。用柠檬酸钠还原法制备胶体金颗粒,标记抗1-氨基乙内酰脲的衍生物(CPAHD)的单克隆抗体并喷于玻璃纤维上,CPAHD-BSA(Bovine serum albumin)抗原和羊抗鼠IgG分别结合于硝酸纤维膜上,依次将样品垫、胶体金垫、硝酸纤维素膜和吸水纸组装切割成AHD胶体金免疫层析快速检测试纸条。在5 min内肉眼观察结果,该试纸条对AHD的最低检测限为2.33μg/L,除与呋喃妥因有弱交叉反应外,与其他同类物均无交叉反应,用该试纸条和ELISA(Enzyme linked immunosorbent assay)检测猪肉中添加的AHD,结果呈现很好的相关性。该方法灵敏度高,简便快速,无需特殊仪器设备,可作为呋喃妥因残留批量检测的筛选方法。     

胶体金免疫层析法检测罂粟碱的研究

建立了准确、快速,简便的检测食品中罂粟碱的胶体金免疫层析技术(GICA)。采用柠檬酸三钠还原法制备胶体金颗粒,标记罂粟碱(Papavarine)抗体。方法检出限为0.2μg/mL,正确检出率约为97%,特异性强,具有推广应用价值。     

胶体金免疫层析法对组织样品中磺胺甲嗯唑残留的快速检测

研究了用于快速检测组织样品中磺胺甲嗯唑残留的胶体金免疫层析检测试剂。采用免疫竞争法,将抗磺胺甲嗯唑多克隆抗体-胶体金复合物包被在胶体金结合垫上,同时将人工合成的磺胺甲嗯唑抗原包被在硝酸纤维素薄膜表面作为检测线（T线）,将抗磺胺甲嗯唑多克隆抗体的羊抗兔二抗包被在硝酸纤维素薄膜表面作为质控线（C线）。T线的人工抗原与待测样品中的磺胺甲嗯唑竞争结合胶体金标记的磺胺甲嗯唑多克隆抗体,通过T线与C线的显色对比读出结果。采用该检测试剂检测组织试样时,定量下限可达20μg／L,整个检测过程只需3—5min,且与磺胺嘧啶、磺胺二甲基嘧啶、盐酸克伦特罗、四环素、青霉素、链霉素无交叉反应。检测试剂具有较高的灵敏度及特异性,操作便捷,稳定可靠,可作为组织中磺胺甲嗯唑残留现场监控的有效筛检手段。     

胶体金免疫层析法对组织样品中磺胺甲噁唑残留的快速检测

研究了用于快速检测组织样品中磺胺甲噁唑残留的胶体金免疫层析检测试剂.采用免疫竞争法,将抗磺胺甲噁唑多克隆抗体-胶体金复合物包被在胶体金结合垫上,同时将人工合成的磺胺甲噁唑抗原包被在硝酸纤维素薄膜表面作为检测线(T线),将抗磺胺甲噁唑多克隆抗体的羊抗兔二抗包被在硝酸纤维素薄膜表面作为质控线(C线).T线的人工抗原与待测样品中的磺胺甲噁唑竞争结合胶体金标记的磺胺甲噁唑多克隆抗体,通过T线与C线的显色对比读出结果.采用该检测试剂检测组织试样时,定量下限可达20 μg/L,整个检测过程只需3 ～5 min,且与磺胺嘧啶、磺胺二甲基嘧啶、盐酸克伦特罗、四环素、青霉素、链霉素无交叉反应.检测试剂具有较高的灵敏度及特异性,操作便捷,稳定可靠,可作为组织中磺胺甲噁唑残留现场监控的有效筛检手段.     

快速检测甲胎蛋白的免疫层析试条的研制

研制了可简便、快速检出原发性肝癌标志物－－人血清中甲胎蛋白（AFP）的免疫层析试条。为此，研究了用国产试剂和材料制备胶体金、用此胶体金标记抗AFP单抗的影响因素以及抗AFP抗体固化条件、抗AFP抗体与其AFP结合能力等。结果表明，自制国产胶体金质量不亚于进口商品；金标单抗和固化抗体活性稳定，能分别显示出结合AFP分子不同表位的特异性。所得检测试条的检出速度在5至20min内，检测阳性阈值定为20ng AFP/mL血清。     

氟苯尼考胶体金免疫层析定量检测方法的建立

建立了定量检测氟苯尼考的胶体金免疫层析方法.对胶体金标记抗体时溶液pH和抗体浓度、金标抗体用量、检测线上抗原浓度以及检测时间进行了优化.采用胶体金试纸条读取仪测定试纸条检测线和质控线的信号强度,以标准品的浓度为横坐标,阳性样本和阴性样本的检测线/质控线的信号比值(Bx/B0)为纵坐标建立标准曲线.结果表明,胶体金免疫层析试纸定量检测氟苯尼考的线性范围为0.1~1.5 ng/mL,检出限为0.08 ng/mL,检测时间为15 min.本方法具有简便、快速和可定量等特点,适于大批量样品的现场筛查.     

A novel enhancement assay for immunochromatographic test strips using gold nanoparticles

The immunochromatographic assay is a well-known and convenient diagnostic system. In this report, the development of a novel enhancement assay for the test strips is described. Additionally, this highly sensitive immunochromatographic assay was applied to detect human chorionic gonadotropin hormone (HCG) as the model case. The primary antibody-conjugated gold nanoparticles were used as the enhancer of the standard method. The primary antibodies were immobilized within a defined detection zone (test line) on the diagnostic nitrocellulose membrane. The secondary antibodies were conjugated with colloidal gold nanoparticles. In combination with an effective sample pretreatment, the gold-conjugated antibodies and the primary antibodies formed a sandwich complex with the target protein. Within the test line, the sandwich complex was immobilized, and furthermore, concentrated by the enhancer resulting in a localized surface plasmon resonance (LSPR) phenomenon and a distinct red color on the test line. The intensity of color of the red test line (signal intensity), which correlated directly with the concentration of the target protein in the standard or spiked samples, was assessed visually and by computer image analysis using a three-determination analysis. Under optimum conditions, the limit of detection (LOD) for HCG assay was 1 pg/mL. When using human serum, 10 pg/mL of HCG could be detected. We have also spiked total prostate-specific antigen (TPSA) in female serum. The LOD for TPSA was determined as 0.2 ng/mL. With this method, the quantitative determination of the target protein could be completed in less than 15 min. Our novel immunochromatographic strips using the enhancing method based on LSPR of gold nanoparticles are useful as a rapid and simple screening method for the detection of important analytes for medical applications, environmental monitoring, food control, and biosecurity.      

胶体金免疫层析方法快速检测腹泻性贝毒软海绵酸的初步研究

建立了赤潮毒素腹泻性贝毒软海绵酸的快速胶体金免疫层析检测方法。通过细胞融合,制备抗软海绵酸单克隆抗体,胶体金标记抗体,建立快速检测软海绵酸的免疫层析试纸条方法。检出限500 ng/mL(50 ng/条),探讨了影响测试方法的因素和提高灵敏度的可能手段。     

An immunochromatographic assay for rapid and simultaneous detection of levonorgestrel and methylprednisolone in water samples

Synthetic contraceptive levonorgestrel (LNG) and glucocorticoid methylprednisolone (MP) residues are eventually discarded to environmental water system and function as environmental hormones, displaying potential risk to humans and ecosystems, thus there is an urgent need for fast, sensitive and simultaneous detection of these compounds in water samples. In this study, a competitive immunochromatographic assay (ICA) using colloidal gold-labeled polyclonal antibodies as probes for rapid and simultaneous detection of LNG and MP in water samples was developed. The visual detection limits of LNG and MP in water samples were 10 ng/mL. The detection process could be completed within 10 min. There was no cross-reactivity of the ICA with other seven compounds. The strips could be stored at 4℃ for 10 weeks without significant loss of activity. The assay is a suitable tool for rapid and semiquantitative detection of LNG and MP in water samples on site.     

Colloidal gold-based immunochromatographic assay for detection of diethylstilbestrol residues

One-step membrane-based competitive colloidal gold-based immunoassays in immunochromatographic formats for the rapid detection of diethylstilbestrol (DES) were developed. Nitro-cellulose membrane strip was separately coated with goat anti-rabbit IgG (control line) and DES hapten-ovalubumin conjugate (test line). Anti-DES polyclonal antibody labeled with colloidal gold particles was first incubated with DES. A positive reaction as a result of the remaining antibody-gold conjugate combining with antigen coated on the membrane was obvious by visual detection, with detection limits for immunochromatographic of 0.5 microg/kg for detecting DES standard solution, and the limit of detection was 5 microg/kg for detecting the DES spiked in swine pork and liver. The assay time for test was less than 5 min, suitable for rapid testing on-site.     

Development of an immunochromatographic assay for rapid detection of 1-Aminohydantoin in urine specimens

A rapid immunochromatographic assay was developed and validated for detection of 1-aminohydantoin (AHD) in urine specimens. Colloidal gold-labeled polyclonal antibody specific to AHD derivative was used as the marker; based on the competitive reactivity theory, the metabolite of nitrofurantoin after derivatization with benzaldehyde would compete with carboxyphenyl AHD derivative-conjugated ovalbumin. The test strip could efficaciously detect the novel analyte with a visual detection limit of 10 ng mL(-1) and high specificity. The reliability of the assay was determined by testing 80 standard samples comparing with enzyme-linked immunosorbent assay. The semi-quantitative detection was accomplished in less than 15 min with low cost, especially for requirements of rapid and simple screening. This is the first publication of an immunochromatographic assay for detection of nitrofuran residues.     

Development of ELISA and immunochromatographic assay for ofloxacin

Two rapid,sensitive and reliable immunoassay methods,namely competitive indirect enzyme-linked immunosorbent assay(CI- ELISA)and colloidal gold-based immunochromatographic assay(CGIA),were developed to detect ofloxacin(OFL).The linear range of the CI-ELISAwas from 0.5 to 128 ng/mL with a limit of detection(LOD)of 0.35 ng/mL.Good recoveries were obtained in analyzing simulated swine urine samples.The CGIA could accurately estimate OFL at concentrations as low as 10 ng/mL in less than 10 min,and test results were read visually without any instrument.     

Development and validation of an immunochromatographic assay for rapid multi-residues detection of cephems in milk

A one-step immunochromatographic assay (ICA) was developed for the detection of seven kinds of cephems in milk. Polyclonal antibodies (PcAb) with group-specific to cephems were raised in rabbits after immunization with cephalexin-keyhole limpet hemocyanin (KLH) conjugate. The specificity of anti-sera was determined by indirect competitive enzyme-linked immunosorbent assay (icELISA), and the 50% inhibitions (IC₅₀) of cephalexin and cefadroxil were obtained at 1.5 ng mL⁻¹; IC₅₀ of cefatiofur, cefapirin, cefazolin, cefalothin and cefotaxine were 4, 3.7, 3.2, 4.5 and 5 ng mL⁻¹, respectively. The PcAb against cephems were conjugated to colloidal gold particles as the detection reagent for ICA strips to test for cephems. This method achieved semi-quantitative detection of cephems in <5 min, with high sensitivity to cephalexin and cefadroxil (both 0.5 ng mL⁻¹). At the same time, cefatiofur, cefapirin, cefazolin, cefalothin and cefotaxine were detected at <100 ng mL⁻¹ in spiked processed-milk samples. This method was compared with an enzyme-linked immunosorbent assay by testing 40 milk samples, and the positive samples were validated by a high-performance liquid chromatographic method, with an agreement rate of 100% for both comparisons. In conclusion, the method was rapid and accurate for the multi-residue detection of cephems in milk.     

Enzyme-linked immunosorbent assay and colloidal gold immunoassay for ochratoxin A: investigation of analytical conditions and sample matrix on assay performance

A polyclonal antibody against ochratoxin A (OTA) was produced from rabbits immunized with the OTA–BSA conjugate. A competitive direct enzyme-linked immunosorbent assay (cdELISA) and a membrane-base colloidal gold immunoassay in flow-through format were developed for the rapid detection of OTA in various food matrices. In the cdELISA, the concentration causing 50% inhibition was 0.07 ng mL⁻¹, and the effects of different chemical conditions (ionic strength, pH value, and organic solvent) were studied. The sensitivity of the assay was higher than those previously reported. A simple, rapid, and efficient extraction method was developed and 74–110% recoveries of spiked samples were obtained. Fifty percent methanol extracts of some food samples such as barley, wheat, oat, corn, rice, and raisins could be analyzed directly by immunoassay after dilution in PBS; grape juice and beer samples could be analyzed directly after dilution with PBS; for coffee samples, a more complex method was used to remove the matrix effect effectively. Membrane-based colloidal gold immunoassays had a visual detection limit of 1.0 ng mL⁻¹ for OTA with a detection time of less than 10 min. For the validation of the cdELISA and membrane-based colloidal gold immunoassay, samples were analyzed by high-performance liquid chromatography. The correlation between data obtained using the microwell assay and HPLC was good (R ² = 0.984). The developed immunoassay methods are suitable for the rapid quantitative or qualitative determination of OTA in food samples.     

Pretreatment-free immunochromatographic assay for the detection of streptomycin and its application to the control of milk and dairy products

A rapid pretreatment-free immunochromatographic assay was developed for the control of the streptomycin (STR) content in milk and dairy products. The assay is based on the competition between an immobilized STR–protein conjugate and STR in a sample to be tested for the binding to monoclonal anti-STR antibodies conjugated to colloidal gold during the flow of the sample along a membrane strip with immobilized reactants. It is possible to improve the cut-off level of positive and negative samples distinguished by a change in the molar STR to protein ratio in the immobilized conjugate. The cut-off level (500 ng mL⁻¹) thus achieved corresponds to the stated MRL of STR in milk and dairy products. For STR concentrations in the range of 16–250 ng mL⁻¹ its content can be quantitatively measured based on the degree of binding of a colloidal gold label in the test strip zone with the immobilized STR–protein conjugate. The duration of the assay is 10 min. The selected sizes of membrane pores and colloidal gold particles allow the assay to be carried out at room temperature without additional reactants and pretreatment. The applicability of the assay for milk, whole milk, sour clotted milk, and kefir with different fat content (from 0.5% to 6%) was confirmed. The results of quantitative immunochromatographic assay show good correlation with traditional ELISA (r was equal to 0.935 and 0.940 for the series tested).