诺如病毒常见流行株胶体金免疫层析快速检测方法

【背景】诺如病毒是全球引发急性胃肠炎的最主要病原之一,具有丰富的遗传多样性。【目的】建立一种简便快捷、适用于诺如病毒常见流行株的胶体金免疫层析检测方法。【方法】将抗诺如病毒衣壳蛋白的单克隆抗体1B10作为金标抗体、抗诺如病毒衣壳蛋白的单克隆抗体1D6作为检测线、羊抗鼠抗体作为质控线组装成胶体金试纸条。对试纸条的组装条件进行优化,确定最佳标记pH、金标抗体最佳浓缩比例及检测线(test line,T线)、质控线(control line,C线)最佳划线浓度等。对新方法进行性能评价,包括灵敏性试验、特异性试验、保存期试验及符合率实验等。【结果】所建立的诺如病毒胶体金试纸条检测方法最低检测浓度为5.9×105copies/μL。本方法与常见的腹泻病毒,如轮状病毒、星状病毒、腺病毒、肠道病毒均无交叉反应。批次间与批次内重复较好,保存期试验表明试纸条至少可以室温密封干燥保存一年时间。应用所建立的胶体金检测方法对24份临床粪便样本进行检测,检测结果与实时荧光RT-PCR方法的阳性符合率约为83%(15/18),常见流行株GII.2型、GII.4型、GII.17型均被成功检出。【结论】建立的胶体金试纸条检测方法具有较好的特异性与稳定性,可用于诺如病毒常见流行株检测及大规模流行病学调查。     

Ultrasensitive nanogold probe-based immunochromatographic assay for simultaneous detection of total aflatoxins in peanuts

An ultrasensitive immunochromatographic (IC) assay for simultaneous detection of total aflatoxins (AFB1, AFB2, AFG1, and AFG2) was developed to meet the requirement for rapidly monitoring aflatoxins in agro-products. The assay was based on a competitive format and its sensitivity was improved by using a novel criterion to screen the optimal amount of monoclonal antibody (MAb) labeled to nanogold particles. The visual detection limits (VDLs) for aflatoxins B1, B2, G1, and G2 in peanut matrix were 0.03, 0.06, 0.12, and 0.25 ng mL(-1), respectively, which were lower than those of published literatures. The results of IC assay were in good agreement with those of high performance liquid chromatography (HPLC) in the analysis of aflatoxins in peanuts, demonstrating the practical applicability of the developed assay in real samples. This qualitative test based on the visual evaluation of results did not require any equipment. Overall, to our knowledge, this is the first report of qualitative detection for total aflatoxins by immunochromatographic assay.     

三聚氰胺胶体金免疫层析试纸条的研制

通过胶体金免疫层析技术建立一种特异、便捷、快速的三聚氰胺抗原检测方法,对奶制品及饲料中的三聚氰胺残留水平监测提供参考。用柠檬酸三钠还原法制备的胶体金,标记纯化的三聚氰胺单克隆抗体,喷于试纸的金标垫。将MEL-OVA(三聚氰胺和卵清白蛋白的偶练物)和纯化的羊抗鼠IgG分别喷于试纸的T(检测线)处和C(质控线)处,通过挑选试纸条材料和调试工艺参数,并最终组装成试纸条。结果显示,制备的试纸监测体系方法检出限为50 g/L。试纸条对牛奶、奶粉和饲料中的三聚氰胺残留的检出限分别为100 g/L、100 ng/g和200 ng/g。将该法与LC-MS/MS法对比检测牛奶、奶粉和饲料样品,在试纸条检测范围内,与LC-MS/MS法检测结果一致性好,从而验证了该方法的有效性。制备的三聚氰胺胶体金检测试纸在常温干燥环境下至少可保质6个月,能够检测出三聚氰胺含量大于50 g/L的样品,适用于现场实际样品三聚氰胺残留水平监测,具有良好的应用前景。     

流感嗜血杆菌快速检测胶体金试纸的研制

以流感嗜血杆菌外膜蛋白P 6为检测标志物,利用胶体金免疫层析技术建立一种快速、灵敏、准确检测流感嗜血杆菌的方法。对P6蛋白(GenBank登录号:AGH02799)进行生物信息学分析,获取其胞外结构域中抗原表位最丰富的肽段,预测其中的线性抗原表位P6Line (62–75 aa),化学合成后经免疫、抗体纯化得到线性表位抗体,同时利用重组P6蛋白制备多克隆抗体,建立基于双抗体夹心免疫层析技术的流感嗜血杆菌快速检测方法,并对该方法的特异性、灵敏性、重复性和稳定性作出评价,同时对该方法进行临床模拟试验,平板培养法验证其准确性。建立的检测方法可在15 min内完成对样本的检测,检测敏感度高(1×10~5 CFU/mL)、特异性强,与其他诸如肺炎链球菌、卡他莫拉菌、肺炎支原体、嗜肺军团菌等常见9种的呼吸道病原菌无交叉反应;试纸条在25℃保存具有良好的重复性和稳定性;200份临床样品检测结果与平板培养法的阳性符合率为90.5%。P6蛋白具有高度的表面暴露性和较强的抗原性,可作为流感嗜血杆菌检测标的物,胶体金免疫层析法具有快速、简便、灵敏的特点,适用于呼吸道感染的临床快速检测。     

基于胶体金的8-羟基-2′-脱氧鸟苷免疫层析试纸条北大核心CSCD

8-羟基-2′-脱氧鸟苷(8-hydroxy-2′-deoxyguanosine,8-OHdG)是评价DNA氧化损伤较灵敏和稳定的生物标志物。文中采用竞争法建立一种快速、灵敏检测8-OHdG的胶体金免疫层析试纸条。将样品垫(玻璃纤维素膜)、结合垫(玻璃纤维素膜)、硝酸纤维素膜和吸水垫依此粘贴在聚氯乙烯(polyvinyl chloride,PVC)底板上,构建试纸条。通过柠檬酸钠还原三水合四氯金酸制备胶体金(gold nanoparticles,AuNPs),8-OHdG配对的抗体(antibody,Ab)包被于AuNPs的外层(Ab coated AuNPs,Ab@AuNPs)作为探针。牛血清蛋白(bovine serum protein,BSA)与8-OHdG用碳二亚胺盐酸盐偶联制备人工抗原,作为检测线的包被抗原。羊抗鼠多抗(imunoglobulin G,IgG)作为质控线的包被抗体。对试纸条的硝酸纤维素膜、上样液的配方、金标抗体喷涂量等实验参数进行了优化。结果表明,硝酸纤维素膜(nitrocellulose film,NC)膜采用CN 95,上样液的最优配方为1%BSA+3%吐温-20+3%蔗糖+0.9%NaCl溶液,最适金标抗体喷涂量为4μL。利用试纸条在可见光下检测8-OHdG,根据检测线(test line,T线)和质控线(control line,C线)的显色强度对比,可初步判断尿液中8-OHdG的含量水平。并通过T线的灰度值计算尿液中的8-OHdG的浓度,检测限为2.55μg/L。该方法简单、快速且有较好的特异性,可检测人体尿液中的8-OHdG含量,以初步评价人体的健康状态。     

基于胶体金标记米曲霉素的免疫层析试纸法快速筛查SLE

建立基于胶体金标记米曲霉素(AOL)的快速筛查系统性红斑狼疮(SLE)的免疫层析试纸法。

利用大肠杆菌BL21原核表达特异性识别核心岩藻糖基的AOL基因(FleA), 并进行纯化及胶体金标记。利用特异性识别IgG的Protein G以及胶体金标记的AOL共同建立快速筛查SLE的免疫层析试纸法(ICS)。

成功表达并纯化AOL重组蛋白, 并进行胶体金标记; 应用胶体金标记AOL的ICS检测SLE患者血清呈阳性反应, 而健康对照及其他自身免疫性疾病(类风湿关节炎、IgA肾病和结缔组织病等)呈阴性反应。

成功建立基于胶体金标记AOL的快速筛查SLE的ICS, 为SLE早期筛查提供了可靠依据。

     

一种超高灵敏的埃博拉病毒胶体碳侧流免疫层析检测方法的建立

埃博拉出血热 (Ebola hemorrhagic fever, EHF) 由于其高感染性和高致死率特点,快速鉴别诊断并实施隔离是最有效的防止疫情扩散的措施。文中建立了一种可以快速、高灵敏筛查埃博拉病毒 (Ebola virus,EBOV)感染的现场检测技术,用碳纳米颗粒标记抗EBOV基质蛋白VP40兔多克隆抗体,组装成一种可在15 min内检测埃博拉病毒的胶体碳侧流免疫层析试纸条。将标记胶体碳颗粒的兔多抗喷涂于玻璃纤维素膜上制备碳标垫;以1 mg/mL的抗VP40单克隆抗体 (McAb,4B7F9) 和羊抗兔IgG,按照2 μL/cm的包被量印迹于硝酸纤维膜上,分别作为检测线与质控线,组装试纸条。该试纸条能够特异地检测EBOV重组VP40蛋白、EBOV病毒样颗粒(Virus-like particles,VLP) 和灭活EBOV,而与马尔堡病毒样颗粒 (MARV-VLP)、流感病毒A/PR/8 (IAV/PR/8)、黄热病毒 (YFV-17D)、登革热病毒2型 (DEN2) 无交叉反应,显示良好的特异性,对1 500份阴性血清进行检测,假阳性率为1.3‰,仅为WHO授权ReEBOV?胶体金试纸的1/100;该胶体碳试纸条检测灭活EBOV的最低检出限为100 ng/mL (相当于106 copies/mL),远优于ReEBOV?胶体金试纸条检出限 (10 μg/mL,相当于108 copies /mL)。热稳定性评价显示试纸条可在室温稳定保存1年以上。文中建立的EBOV胶体碳免疫层析试纸条能够快速、超高灵敏、特异地检测EBOV,为现场快速筛查EBOV感染提供一种新方法。     

A sensitive immunochromatographic assay using gold nanoparticles for the semiquantitative detection of prostate-specific antigen in serum

In prostate cancer screening, prostate-specific antigen (PSA) has been utilized as a valuable biomarker. There are routinely used procedures based on enzyme-linked immunosorbent assay (ELISA) for PSA detection. The procedures based on ELISA, however, are time consuming, complicated, and costly. We have developed a rapid, very simple, cost effective and sensitive immunochromatographic assay using gold nanoparticles and evaluated its applications for first screening of prostate cancer in serum samples. The sensitive immunochromatographic assay requires only 40 μL of the serum sample. The assay used is rapid and simple, that it totally takes approx 15 min to complete. The method for sensitive immunochromatographic assay has the other advantage of decreasing the antibody concentration that is used for the test line. In this study, we show the advantage to decrease the antibody concentration and the evaluation of our sensitive immunochromatographic assay for the semiquantitative detection of PSA in serum. The results obtained from 163 serum samples using sensitive immunochromatographic assay are compared with the results obtained using the chemiluminescent enzyme immunoassay (CLEIA) and normal immunochromatographic assay. The results obtained in the sensitive immunochromatographic assay correlated well with the values obtained in CLEIA. We concluded that our sensitive immunochromatographic assay is applicable to the first screening test for the diagnosis of prostate cancer. Our developed sensitive immunochromatographic assay is a promising candidate for diagnosis or research use, which may become commercially available in the near future.     

Development of rapid one-step immunochromatographic assay

An analytical system for a one-step immunoassay has been constructed using the concept of immunochromatography. The system employed two different antibodies that bound distinct epitopes of an analyte molecule: an antibody labeled with a signal generator (e.g., colloidal gold), which was placed in the dry state at a predetermined site on a glass-fiber membrane, and another antibody immobilized on the surface of a nitrocellulose membrane. Three membranes, one with the tracer, one with immobilized antibody, and a cellulose membrane as the absorbent of medium (in a sequence from the bottom), were attached to a plastic film and cut into strips. Aqueous medium containing analyte absorbed from the bottom end of the immunostrip dissolved the labeled antibody, and the antigen-antibody binding complex formed was transported into the next nitrocellulose membrane by the flow caused by capillary action. The complex subsequently reacted with the immobilized antibody, which generated a signal in proportion to the analyte concentration. The convective mass transfer of the immunoreactant to the binding partner allowed the assay to be performed with no handling of reagents. The reaction, however, was carried out under nonequilibrium conditions, which resulted in decreased sensitivity as compared with assays performed in an equilibrium mode (e.g., ELISA). To minimize such sacrifice, major factors that control system performance were identified and the system was then devised under optimal conditions.     

土拉弗朗西斯菌胶体金免疫层析快速检测方法的建立

目的建立胶体金免疫层析技术快速定量检测土拉弗朗西斯菌。方法利用胶体金标记和双抗体夹心免疫层析技术,建立土拉弗朗西斯菌的快速检测方法,评价其特异性和敏感性,并拟合检测曲线进行定量检测。在面粉、饼干、果冻、梨汁等食品样品中添加土拉弗朗西斯菌的FopA蛋白模拟污染样品,评价该方法对固体、半固体、液体等食品样品的检测能力。结果该法可在10min内完成定性和定量检测,灵敏度为750ng／ml,线性范围750～24000ng/ml、回收率为56．7％-89．2％。结论所建立的检测土拉弗朗西斯菌的胶体金免疫层析方法,能快速、灵敏、特异、准确地检测样品中的土拉弗朗西斯菌,适用于现场快速检测。     

Development and validation of an immunochromatographic assay for rapid detection of sulfadiazine in eggs and chickens

A rapid immunochromatographic assay (ICA) was developed and validated for the detection of sulfadiazine in eggs and chickens. Based on the competitive reaction mechanism, the competitor of sulfadiazine (sulfadiazine-BSA conjugate) was immobilized to the defined detection zone on a nitrocellulose membrane which acted as the capture reagent, and the monoclonal antibody against sulfadiazine was conjugated to colloidal gold particles which served as the detection reagent for the preparation of the immunochromatographic strips to test sulfadiazine. With this method, the semi-quantitative detection of sulfadiazine was accomplished in less than 15min, with high sensitivity to sulfadiazine (5ng/g) and low cross-reactivities with other sulfonamides. With experimental egg and chicken samples spiked with sulfadiazine at concentrations of 10, 20, and 100ng/g, recoveries were demonstrated to be from 71% to 97% in egg samples and 71% to 95% in chicken samples. This method was compared with the enzyme-linked immunosorbent assay by testing 52 egg samples from the animal experiment, and compared with the high-performance liquid chromatographic method by testing 56 chicken samples, with an agreement rate of 100% for both comparisons, by using the maximum allowed residue of sulfadiazine (i.e. 100ng/g) as the cut-off level as set by the European Union and China. The accuracy of ICA was also confirmed in an initial study with marketed egg and chicken samples. In conclusion, the method is rapid and accurate for the detection of sulfadiazine in eggs and chickens.     

Monoclonal antibodies labeled with colloidal gold for immunochromatographic express analysis of diphtheria toxin

A one-step immunochromatographic method for the detection of the diphtheria toxin in different water samples (phosphate buffer, milk, and human nasopharyngeal swab) was developed using a conjugate of monoclonal antibodies labeled with colloidal gold. The detection limit of diphtheria toxin was 10 ng/ml, the time of the analysis was 15 min. The use of silver to enhance the reaction sensitivity and scanning equipment to evaluate the immunochromatography results decreased the detection limit to 1.25 ng/ml.     

A nanogram-level colloidal gold single reagent quantitative protein assay

We have developed a nanogram-level quantitative protein assay based on the binding of colloidal gold to proteins adhered to nitrocellulose paper. The protein–gold complex produces a purple color proportional to the amount of protein present, and the intensity of the stain is quantified by densitometry. Typical assays require minimal starting material (10–20 μl) containing 1 to 5 μg protein. A small volume (2 μl) of protein solution is applied to nitrocellulose paper in a grid array and dried. The nitrocellulose is incubated in colloidal gold suspension with gentle agitation (2–16 h), rinsed with water, and scanned. Densitometric analysis of the scanned images allows quantitation of the unknown sample protein concentration by comparison with protein standards placed on the same nitrocellulose grid. The assay requires significantly less sample than do conventional protein assays. In this report, the Golddots assay is calibrated against weighed protein samples and compared with the Pierce Micro BCA Protein Assay Kit. In addition, the Golddots assay is evaluated with several known proteins with different physical properties.     

A convenient immunochromatographic test strip for rapid detection of Scylla serrata reovirus

<正>Dear Editor,Scylla serrata reovirus(SsRV),first discovered in China in 2004,is now known to be widespread in the mud crab(Scylla serrata)farming pond of China.(Chen et al.,2008).Since there are no effective treatments currently available for this viral pathogen,early diagnosis is the     

Rapid detection of glycyrrhizin by immunochromatographic assay

An immunochromatographic assay was developed for detecting glycyrrhizin (1). The qualitative assay is based on a competitive immunoassay using anti-1 monoclonal antibody (MAb) and a detector reagent that contains colloidal gold particles coated with anti-1 MAb. The immunochromatographic strip test, which has a detection limit of 250 ng/mL, is useful as a rapid screening method for detecting glycyrrhizin in plants, biological fluids and food samples.