Development of an Indirect Enzyme-Linked Immunosorbent Assay for Seromonitoring Contagious Bovine Pleuropneumonia Using Recombinant Lipoprotein LppQ of Mycoplasma mycoides subsp mycoides SC as Antigen

Mycoplasma mycoides subsp mycoides SC （MmmSC） is the etiological agent of contagious bovine pleuropneumonia （CBPP）. The lipoprotein LppQ encoded by lppQ gene is specific to MmmSC and is found in the type strain and in field strains isolated in Europe, Africa, and Australia, as well as in vaccine strains. No serological cross-reactions were observed with the related mycoplasmas of the Mycoplasma mycoides cluster. The N-terminal domain of the mature lipoprotein LppQ is hydrophilic, and it induces a strong, specific, early, and persistent immune response in naturally and experimentally infected animals. Mycoplasma-specific TGA （Trp） codons are utilized as stop codons in most other organisms. The lppQ N-terminal fragment from MmmSC HVRI X strain, the Chinese strain for CF antigen production, was mutated with one-step overlapping extension PCR. Sequence analysis confirmed the successful mutation from A to G in codon 198 in the lppQ gene. The fragment containing the mutation site was subcloned into the pET32a expression vector. The recombinant protein with molecular weight of 42 kDa was purified using the Ni-NTA His.Bind purification kit, with a purity of up to 95%. Western blot indicated that the standard positive serum of CBPP could react with the recombinant protein. The purified protein was diluted to 0.35 μg mL^-1, and coated to microtiter enzyme-linked immunosorbent assay （ELISA） plates. Indirect ELISA reaction conditions were optimized. The value of P/N was determined to be 4.8 （0.934/0.193）, the sensitivity to be 95.8% （46/48）, and the specificity to be 98.9% （161/163）. 3 817 cattle serum samples from three different provinces were detected by the indirect ELISA and CFT. The Kappa value is 0.63, which is middle or high agreement between the two methods.

SERODIAGNOSIS OF CLONORCHIASIS BY ENZYME—LINKED IMMUNOSORBENT ASSAY WITH HRP—SPA

In thes paper the authors used the Horseradish peroxidase labelledstaphylococcal protein A(HRP—SPA)in ELISA,for the detection of Clo-norchis sinensis infection.Serum tests were made on 116 confirmed cases ofclonorchiasis,103(88.8%)of them showed positive,while only 6(4.4%)werepositive among 138 healthy people.Samples were collected on filter paperstrips,111(95.7%)cases were positive among 116 comfirmed cases tested,but only 2(1.5%)were positive out of 138 healthy persons.The resultswere similar to those obtained by sheep antihuman IgG.Animal experimentalso showed that the SPA—ELISA can be used for the diagnosis ofclonorchiasis.In an endemic area,stool egg positive rate was 8.8%(62/703).whenchecked with SPA—ELISA,the rate of conformity in both filter paperstrips and stool examinations was 90.3(56/62).Among 641 serum testsfrom individuals negative in stool examinations,only 35(5.5%)reactedpositively.The authors suggested—that SPA—ELISA with soluble Clo-norchis antigens could be used in a large scale seroepidemiological surveyin endemic areas.

Microcystin-LR detection based on indirect competitive enzyme-linked immunosorbent assay

Microcystins(MCs)are a group of closely related toxic cyclic heptapeptides produced by common cyanobacte-ria,which cause lots of accidents and threatens human health.In this paper,an indirect competitive enzyme-linked immu-nosorbent assay(ic-ELISA)was established and used to detect microcystin-LR(MC-LR)in drinking and surface waters.The concentration of coating antigen was 5 mg/mL,the dilution of monoclonal antibody MC10E7 was 1:3000,the dilution of enzyme tracer(goat anti-mouse IgG-peroxidase)was 1:3000,the standard concentration of MC-LR ranged from 0.001 mg/L to 30 mg/L,and o-phenylenediamine was used as substrate.The assay showed high relativity with high performance liquid chromatography(HPLC)with a correlation coefficient of more than 99%.The relative standard deviation was less than 10%,the detection limit was achieved down to 0.01 mg/L and up to 5.1 mg/L.The quantitative detection range was from 0.03 mg/L to 3 mg/L,and the antibody had high specificity for[4-arginine]microcystins.It performed well in spite of the influence of the real samples.

基于纳米抗体建立icELISA检测乳制品中黄曲霉毒素M1

纳米抗体(nanobody,Nb)具有稳定性高、特异性强、易于表达等优势,已经成为小分子免疫分析的重要工具。为了监测乳制品中黄曲霉毒素M1(aflatoxin M1,AFM1)的污染情况,以先前从双峰驼AFM1免疫文库中淘选得到的抗AFM1型纳米抗体M6为研究对象,评估其理化性质并建立间接竞争酶联免疫吸附测定法(indirect competitive enzyme-linked immunosorbent assay,icELISA)。优化反应体系中封闭方法、甲醇溶液、pH值和离子强度等参数后,建立竞争抑制标准曲线,并进行方法学验证特异性和准确性。结果表明,Nb-M6具有良好的亲和力和热稳定性;Nb-icELISA的检测限(limit of detection,LOD)为0.111 ng/mL,半数抑制浓度(half maximal inhibitory concentration,IC_(50))为1.498 ng/mL,乳制品加标回收率为89.8%~104.1%,与高效液相色谱法的检测结果趋于一致。该方法操作简单、便捷,可应用于乳制品中AFM1的初步批量筛查。

基于VP6蛋白的牛轮状病毒抗体间接ELISA检测方法的建立与应用

为了建立牛轮状病毒(BRV)血清抗体的检测方法,从病料中克隆牛轮状病毒VP6基因,构建其表达载体,利用原核表达技术表达重组VP6蛋白,建立牛轮状病毒血清抗体间接ELISA检测方法。结果显示,重组VP6蛋白大小为40 ku,以包涵体形式表达,Western blot证实重组VP6蛋白有良好的反应原性;以4μg/mL浓度的抗原包被酶标板,一抗血清50倍稀释,酶标二抗稀释10000倍稀释,为最佳工作条件,阴阳临界值为0.233,表明该方法具有良好的特异性和敏感性。建立的检测BRV抗体的间接ELISA可用于临床BRV感染的检测。

间接竞争ELISA检测杏仁过敏原Amandin

Amandin是引起杏仁过敏的主要过敏原。通过提取、纯化得到Amandin蛋白并制备出抗Amandin抗体。该抗体与花生全蛋白、芝麻全蛋白、核桃JugR1、β-乳球蛋白、酪蛋白、溶菌酶均无交叉反应。通过优化包被原浓度、抗体浓度以及缓冲液pH值等条件,建立间接竞争酶联免疫吸附测定(enzyme-linked immunosorbent assay,ELISA)检测Amandin的方法。该方法的灵敏度为(0.66±0.04)μg/mL,检出限为(0.08±0.04)μg/mL。在饼干、面包、冰淇淋样品中的添加回收试验结果表明,该方法的回收率为68.22%~114.00%。稳定性结果表明Amandin蛋白在37℃条件下可以稳定保存7 d。

食品中黄曲霉毒素M_(1)的间接竞争酶联免疫法的建立

该文建立一种间接竞争酶联免疫法(indirect competitive enzyme-linked immunosorbent assay,ic-ELISA)快速测定食品中黄曲霉毒素M_(1)(aflatoxin M_(1),AFM_(1))的分析方法。AFM_(1)标准品用甲醇稀释,AFM_(1)标准品与AFM_(1)全抗原竞争结合AFM_(1)单克隆抗体,利用3,3′,5,5′-四甲基联苯胺(3,3′,5,5′-tetramethylbenzidine,TMB)单组分显色液显色后,酶标仪测定吸光度。在优化好的条件下,浓度范围为9.743~2.605×10^(3)pg/mL时具有良好的线性关系,相关系数(determination coefficient,R^(2))为0.9927,检出限IC_(10)为3.84 pg/mL,加标回收率为88.43%~105.75%。该方法适用性好、操作简单、灵敏度高,满足食品中AFM_(1)分析检测的需求。

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-ELISA was 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 of an Indirect ELISA Using Recombinant Truncated Envelope Glycoprotein for Detection of Antibodies against Japanese Encephalitis Virus

[ Objective] To develop an indirect ELISA assay for detecting antibodies against envelope glycoprotein （ E protein） of Japanese encephalitis virus （JEV）. [ Method] Specific primers were designed according to JEV sequences published in the GenBank. The cDNA of JEV E gene （about 1 000 10p） was amplified by the RT-PCR with the specific primers. After sequencing analysis, the E gene was cloned into pET30a expression vector and expressed in E. coli BL21 （DE3） with the induction of IPTG. After denaturation, purification and renaturation, the recombinant protein was analyzed by the SDS-PAGE and the westem blotting. An indirect ELISA was developed to detect antibodies against JEV. [ Result] The E protein was mainly expressed in inclusion body. With the purified E protein, the indirect ELISA was developed and displayed good specificity, sensitivity and repeatability, [ Conclusion]The developed ELISA using the truncated E protein as antigen is a simple, convenient and rapid serological method for diagnosis, monitoring antibody level and epidemiological investigation of JEV.

DsbC介导HCV优势抗原表位原核可溶性表达与间接ELISA分析

目的DsbC蛋白与丙型肝炎病毒(HCV)优势抗原表位原核融合表达并纯化,获得一种特异优良的HCV血清抗体诊断抗原。方法通过生物信息学软件,筛选我国HCV主要流行株优势抗原片段并进行串联融合形成组合肽命名为P367,将P367与DsbC蛋白进行融合后在原核系统内可溶性表达并纯化获得重组抗原DsbC-P367,建立HCV-IgG血清学检测方法,通过对HCV阴阳性血清的检测,评价DsbC-P367与P367在血清学诊断差异,获得一种新型HCV-IgG血清学诊断抗原制作方法。结果通过信息学软件筛选获得的优势抗原表位来源于不同基因型,全长367个氨基酸。通过原核表达系统发现,DsbC-P367以可溶性表达形式存在,亲和纯化后其相对分子质量为63×10^(3),纯度为92%,Western blot实验初步证实重组DsbC-P367与P367蛋白均具有抗原性;对100份明确HCV阴阳性血清进行检测,DsbC-P367与P367灵敏度分别为96%、90%,特异度均为100%,与“金标准”比较,McNemer检验显示均P=1.00,Kappa分别为0.95、0.87,提示DsbC-P367相对于P367具有更优的灵敏度。结论重组获得的DsbC-P367融合肽在HCV血清学抗体检测中具有良好的灵敏度和特异度,可开发为HCV-IgG体外诊断试剂盒用于HCV感染的实验室诊断。

检测鸡毒支原体抗体的间接ELISA方法和HI试验方法的建立及初步应用

本研究旨在建立一种检测鸡毒支原体(Mycoplasma gallisepticum,MG)抗体的间接ELISA方法,结合HI试验,为MG感染的监测和净化提供一套有效的组合技术方案。以原核表达的VlhA 3.03重组蛋白(rVlhA)作为包被抗原,使用单一稀释法构建了关于血清抗体滴度与1∶500血清稀释度处S/P值的回归方程lg(抗体滴度)=1.257×lg(1∶500处S/P值)+3.709,R^(2)=0.9176,S/P临界值为0.32,临界滴度是1200。经验证,rVlhA-ELISA方法具有良好的特异性、重复性,最低能检出1∶2000稀释的阳性血清。选择国内MG分离株SH/2020-1作为血凝抑制抗原建立HI试验方法。使用rVlhA-ELISA方法联合HI试验进行血清样品检测,IDEXX-MG方法作为对照,借助RT-qPCR方法监测MG感染情况。结果表明rVlhA-ELISA方法和IDEXX-MG监测的血清抗体趋势与HI复核结果均一致;rVlhA-ELISA与HI联合判定结果与IDEXX-MG符合率可达91.53%。上述结果显示,本研究建立的rVlhA-ELISA方法和HI试验具有较好的临床应用价值,可以初步应用于MG感染的临床大规模、快速筛查并对结果进行复核。

基于免疫磁珠净化间接竞争酶联免疫吸附试验检测氟喹诺酮类药物

本研究旨在建立一种基于免疫磁珠进行分离、富集和净化前处理,检测鸡肉、鸡肝和鱼肉中氟喹诺酮类药物残留的间接竞争酶免疫吸附试验(indirect competitive enzyme-linked immunosorbent assay,icELISA)的研究方法。通过对合成免疫磁珠及免疫磁珠净化过程中单克隆抗体添加量、偶联时间、缓冲液pH、抗原添加量、抗原捕获时间、温度及包被条件等进行优化,初步建立了基于免疫磁珠净化的icELISA检测方法。结果显示:1)在1 mg的磁珠中,沙拉沙星(sarafloxacin,SAR)单克隆抗体最佳偶联量为15μg,偶联时间60 min,pH为4.4;2)最佳抗原添加量为1 ng·mL^(-1),捕获时间40 min,缓冲液为0.01 mol·L^(-1)PBS,IC50为0.73 ng·mL^(-1),线性范围为1.0~3.2 ng·mL^(-1);3)氟喹诺酮类药物在鸡肉、鸡肝、鱼肉的检测限均不超过1.33、2.17、2.31μg·kg^(-1),回收率为76.83%~98.70%,批内变异系数批间变异系数均不超过15%,经验证,鸡肉样本检测结果与高效液相色谱法(HPLC)结果一致。结果表明,与传统仪器检测方法相比,该方法提高了检测氟喹诺酮类药物的简便性、选择性以及检测效率,为氟喹诺酮类药物的残留检测提供了新思路。

雌二醇单克隆抗体制备及胶体金侧流层析免疫分析方法的建立

目的探讨雌二醇(17β-estradiol,E2)的3号位和17号位引入活性基团制备的半抗原对抗体灵敏度的影响,选用灵敏度较高的抗体建立一种牛奶中E2胶体金侧流层析免疫分析方法(colloidalgold-basedlateral flow immunoassay,CG-LFA)。方法从E2的3号位羟基和17号位羟基引入活性基团分别制备半抗原H1a和H2,偶联载体蛋白制备完全抗原,经过动物免疫和细胞融合筛选,制备单克隆抗体(monoclonal antibodies,mAbs),采用间接竞争酶联免疫吸附实验(indirect competitive enzyme-linked immunosorbent assay,icELISA)对mAbs性能进行评估,筛选出灵敏度最高的mAb,最后采用静电吸附法将胶体金标记抗体为探针,构建牛奶中E2的CG-LFA。结果制备了H1a-7B7、H1a-7B12、H1a-9C7、H1a-10E7、H2-2E2、H2-3C10、H2-4A10和H2-6D28种mAbs,经过icELISA评估,其半数抑制浓度(half maximal inhibitory concentration,IC50)分别为0.116、0.207、0.072、0.370、0.442、6.170、0.415和4.411 ng/mL,最终选取H1a-9C7,构建牛奶中E2的LFA,消线(cut-off)值为6.00ng/mL,与苯甲酸雌二醇和雌三醇的交叉反应率分别为101.31%和2.43%,在真实样本加标回收实验中,检测结果与液相色谱-串联质谱法(liquid chromatography-tandem mass spectrometry,LC-MS/MS)结果一致。结论E2的3号位引入活性基团设计合成的半抗原所制备的E2抗体灵敏度,比17号位引入活性基团制备的抗体灵敏度高,并且建立的LFA准确度良好,为牛奶中E2快速检测提供了一定的技术手段。

基于寡核苷酸链信号放大快速检测谷物中赭曲霉毒素A

该研究以柠檬酸钠还原法制备粒径均一的金纳米粒子(gold nanoparticles,AuNPs),并将AuNPs与赭曲霉毒素A(ochratoxin A,OTA)抗体通过静电吸附作用偶联,再与6-羧基荧光素(6-carboxyfluorescein,6-FAM)修饰的寡核苷酸链(single stranded DNA,ssDNA)通过金硫键偶联,制备出荧光探针,利用AuNPs近距离淬灭荧光基团信号作用和1,4-二巯基苏糖醇(dithiothreitol,DTT)解离寡核苷酸链作用,建立基于寡核苷酸链信号放大快速检测谷物中OTA的方法。经过优化试验条件,该方法的检测限为0.0044μg/L,特异性良好。使用该方法测定玉米、大米、燕麦3种谷物中的OTA含量,添加回收率为91.2%~102.3%,变异系数小于10%,检测结果与超高效液相色谱串联质谱检测结果接近,证明该方法能够用于检测谷物样品中OTA的含量。

非洲猪瘟病毒抗体ELISA检测方法的建立及初步评价

为建立非洲猪瘟病毒(ASFV)抗体检测方法,分别用ASFV重组蛋白p30、p72、pA104R作为包被原建立间接酶联免疫吸附试验(ELISA)方法,并进行初步评价。结果显示,ASFV重组蛋白p30、p72及pA104R分别按照25 ng/孔、50 ng/孔、50 ng/孔包被,血清样品均100倍稀释,辣根过氧化物酶(HRP)标记的羊抗猪IgG均20000倍稀释作为酶标试剂条件最优。p30-ELISA、p72-ELISA、pA104R-ELISA临界值分别为0.502、0.567、0.550。样品检测S/P值≥临界值判为阳性,否则判为阴性。3种方法分别检测梯度稀释的ASFV阳性血清、ASFV(CD2v缺失)阳性血清,p72-ELISA灵敏度最高,为1∶64、1∶128;3种方法检测猪瘟病毒、猪繁殖与呼吸综合征病毒、猪圆环病毒2型、猪伪狂犬病病毒、猪流行性腹泻病毒阳性血清各5份,ASFV阴性血清200份,结果均为阴性;3种方法批间、批内重复性变异系数均小于10%。说明建立的方法均可用于ASFV的血清学检测,为非洲猪瘟的防控提供了多样化的检测方法。

猪肉中2-(三氟甲基)吩噻嗪的Ic-ELISA检测

为了快速检测猪肉中的镇静剂2-(三氟甲基)吩噻嗪(2-(trifluoromethyl)phenothiazine,TFPTZ),分别用偶氮苯甲酸法、混合酸酐法合成了半抗原、完全抗原,通过免疫新西兰大耳白兔获得了多克隆抗体,采用间接竞争酶联免疫方法(Ic-ELISA)对猪肉中TFPTZ进行了定量分析,实验条件:包被抗原浓度1.25μg/mL,多克隆抗体稀释16000倍,37℃包被3 h,封闭液为质量分数1%的牛血清白蛋白(BSA),TFPTZ稀释液为含体积分数10%的DMSO的PBS,竞争反应60 min.该方法相关系数R^(2)为0.9991,IC_(50)为1.5002μg/L,最低检测限IC_(10)为0.2841μg/L,线性(IC_(20)~IC_(80))为0.4307~5.2252μg/L,与5种TFPTZ结构类似物的交叉反应率小于1.2%,样品添加回收率为93.26%~109.13%,变异系数小于6%,实际样品检测结果与高效液相色谱法测定结果高度一致,表明建立的快速检测猪肉中TFPTZ的Ic-ELISA方法具有良好的准确度,适用于快速检测猪肉中TFPTZ的残留量.

大熊猫源犬细小病毒VP2基因的原核表达及间接ELISA检测方法的建立

【目的】建立一种检测大熊猫血清中犬细小病毒(canine parvovirus,CPV)抗体的间接酶联免疫吸附剂测定(enzyme linked immunosorbent assay,ELISA)方法。【方法】以大熊猫源CPV DNA为模板,利用PCR扩增VP2基因,再用原核表达系统对VP2基因进行表达,经纯化后的蛋白作为ELISA包被抗原;制备并纯化兔抗大熊猫IgG,采用辣根过氧化物酶(horseradish peroxidase,HRP)标记作为间接ELISA酶标二抗,通过棋盘法确定抗原包被质量浓度及血清稀释度等条件,并评估建立方法与商业试剂盒检测样品结果的符合率。【结果】原核表达成功获得约70 ku的VP2蛋白,将其作为间接ELISA包被抗原,抗原最佳包被质量浓度为2.0μg/mL,血清最佳稀释度为1∶400,用该方法进行检测血清样品时OD450≥0.258为阳性,反之为阴性。采用建立的ELISA方法检测大熊猫血清样本阳性率为60.0%,高于商业化检测试剂盒检测的阳性率(52.5%),两者总符合率达到87.5%。【结论】本研究首次建立了基于大熊猫源CPV VP2蛋白为抗原、自制HRP标记兔抗大熊猫IgG为酶标二抗的间接ELISA方法,该方法特异性强、灵敏性较高、重复性好,为大熊猫血清中CPV抗体的检测提供了技术支持。

IIF-SSS及BP180、BP230抗体检测在大疱性类天疱疮病情评估中的应用价值分析

目的分析盐裂皮肤间接免疫荧光(IIF-SSS)及大疱性类天疱疮(BP)180、BP230抗体检测在BP病情评估中的应用价值。方法选取2018年7月至2020年7月郑州大学附属郑州中心医院收治的150例BP患者作为研究对象,收集患者就诊时及就诊后第30、60、180天的IIF-SSS滴度、BP180与BP230抗体水平、自身免疫性大疱性皮肤病严重程度评分(ABSIS)等资料,并根据皮损消退后6个月内是否复发将其分为复发组与非复发组,分析IIF-SSS滴度以及BP180、BP230抗体水平与ABSIS的相关性及对BP复发的预测价值。结果150例BP患者皮损消退后6个月内复发58例(38.67%),设为复发组;未复发92例(61.33%).设为未复发组。就诊后第30、60、180天,复发组患者IIF-SSS滴度、BP180与BP230抗体水平以及ABSIS均明显高于未复发组(就诊后第30天:t=4.256、2.828、2.894、2.612,P<0.001、P=0.005、P=0.004、P=0.010:就诊后第60天:t=3.959、10.080、5.312、3.182,P<0.001、P<0.001、P<0.001、P=0.002;就诊后第180天:t=2.928、12.240、17.020、8.575,P=0.004、P<0.001、P<0.001、P<0.001);Pearson相关性分析结果显示,IIF-SSS滴度以及BP180、BP230抗体水平与ABSIS均呈显著正相关性(r=0.215、0.243、0.196,P=0.008、0.003、0.016);受试者工作特征(ROC)曲线分析结果显示,IIF-SSS联合BP180、BP230抗体检测预测BP复发的曲线下面积(AUC)为0.826,敏感度为81.7%,特异度为78.8%结论IIF-SSS与BP180、BP230抗体检测能够有效评估BP患者病情严重程度,对BP复发具有较高的预测价值。

Serological diagnosis of nasopharyngeal carcinoma by enzyme linked immunosorbant assay:optimization,standardization and diagnostic criteria

Objectives To produce an enzyme linked immunosorbant assay (ELISA) to detect antibodies against Epstein Barr virus (EBV) specified nuclear antigen 1 (EBNA 1) and the 18kD EBV matrix protein, and to determine and optimize its sensitivity and specificity for the diagnosis of nasopharyngeal carcinoma (NPC).Methods We used a combination of highly purified glutathione transferase fusion proteins of the 40kD carboxy domain of EBNA1 and the 18kD EBV matrix protein for coating ELISA plates. In three separate studies, we tested for IgA antibodies in serum specimens from 28 EBV seronegative donors, 284 EBV seropositive donors and 160 newly diagnosed NPC patients. By comparing the sensitivity and specificity of diagnosis obtained for different cutoff values, we derived several quantitative parameters to evaluate assay performance, establish objective diagnostic criteria which optimize the intrinsic diagnostic capability of the assay and assess the significance of individual test results, respectively. Optimum cutoff optical density (OD) is defined as the cutoff OD where sensitivity of the assay equals its specificity, and resolution of the assay is indicated by the value of sensitivity (or specificity) determined at the optimum cutoff OD. Diagnosis of NPC was achieved by setting a cutoff zone at +/-20% of this value.Results All the EBV seronegative donors tested were not reactive, and most of the EBV seropositive donors were weakly reactive, while the majority of NPC patients were moderately or strongly reactive. While the assay was thus shown to be specific for EBV, there was an overlap in the level of these serum antibodies between few individuals of the two latter groups. It was shown that the assay performed equally well in two separate studies conducted under different testing conditions and using different collections of sera in that assay resolution determined on these occasions were 86% and 87% respectively. Diagnosis of NPC can be achieved at the same expected sensitivity of 89% and 83% determined at the lower and upper limits of the cutoff zones, with the corresponding values of specificity being 78% and 91%. It was further shown in the third study that resolution of the assay can be increased to 90% using an assay produced with a higher concentration of the same antigens, and that diagnosis of NPC can be achieved at a higher sensitivity ranging between 86% and 95% at a corresponding specificity of 93% and 86%.Conclusions After optimization and standardization, the ELISA can achieve a sensitivity ranging from 86% to 95%, with corresponding specificities of 93% and 86% respectively for the diagnosis of NPC.

酶联免疫法快速检测保健食品中吲哚美辛和阿西美辛

针对保健食品中吲哚美辛和阿西美辛的非法添加问题,以吲哚美辛和阿西美辛分别作为免疫半抗原和包被半抗原,通过活泼酯法与载体蛋白偶联制备完全抗原,免疫动物筛选获得了可同时识别吲哚美辛和阿西美辛的兔多克隆抗体,并建立了抗风湿类保健食品中吲哚美辛和阿西美辛同时检测的间接竞争酶联免疫分析方法。方法对吲哚美辛的检出限为0.3 ng/mL,半抑制质量浓度(IC 50)为5.6 ng/mL,线性范围为0.9~32.9 ng/mL;对阿西美辛的检出限为1.1 ng/mL,IC 50为7.4 ng/mL,线性范围为2.2~24.3 ng/mL;与多种非甾体抗炎药无交叉反应。片剂、硬胶囊和软胶囊3种剂型的抗风湿类保健食品经甲醇超声提取,通过标准稀释液稀释消除基质效应,吲哚美辛和阿西美辛的添加回收率为80.0%~119.7%,相对标准偏差低于15%;检测结果与液相色谱-串联质谱法检测结果的线性相关系数均大于0.99,结果一致性良好,可用于保健食品中吲哚美辛和阿西美辛的快速筛查。