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.

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.

Preparation of Monoclonal Antibodies to Trimethoprim and ELISA Kit for Rapid Detection

[Objective] This study was conducted to find out an approach for determining trimethoprim residues in water. [Method] Trimethoprim antigen was prepared through a series of reactions from trimethoprim hapten which was generated through the reaction between trimethoprim and maleic anhydride. And trimethoprim monoclonal antibodies were prepared by animal immune, and used to prepare ELISA kit to detect trimethoprim residues in water. Finally, the limit of detection （LED） of the ELISA kit was determined. [Result] The standard curve covered a concentration range of 0-80 μg/L. The LeD of trimethoprim in water using the ELISA kit was 2.34 μg/kg; the IC50 （half maximal inhibitory concentration） was 4.8 μg/L; the recovery rate of added trimethoprim standard ranged from 60.5% to 79.7%; within-and among-batches RSD was less than 10%. The trimethoprim monoclonal antibody was specific, as the cross-reactivity rate of trimethoprim antibody and diaveridine was less than 1%. The stability tests revealed that the ELISA kit was stable after being stored at 4 ℃ for 12 months. [Conclusion] The results will provide references for controlling the abuse of trimethoprim.

Concerns arise: wheat allergy risk in pre-packaged food products from China

Understanding and monitoring the cross-contamination of food allergens is crucial for safeguarding public health and ensuring food safety.Food allergen risk assessment,derived from classical toxicological principles,can identify and quantify the risk of allergies.This study aimed to investigate the risk of wheat allergic reactions to prepackaged foods from China through the utilization of food allergen risk assessment.A total of 575 products have been surveyed,wheat/gluten,milk and egg were major allergens labelled on products.According to voluntary incidental trace allergen labelling 3.0(VITAL®3.0)program,the number of products belonged to Action Level 2 were 303.Integration of precautionary allergen labeling(PAL)analysis indicated that 9.57%products would pose a potential risk to wheat allergic individuals.The probabilistic risk assessment results suggest that 7984 allergic reactions may arise among wheat-allergic consumers during 10000 eating occasions due to the consumption of pre-packaged food products with incorrect wheat-related allergen labelling.This study demonstrated that a risk assessment-based approach can support the guidance of allergen labelling and management of food allergen for pre-packaged food products,providing protection for allergic individuals in food consumption and for food manufacturers in food production and trade.

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。

国产结核分枝杆菌T细胞免疫反应检测试剂盒诊断结核病的临床试验研究

目的:评价国产结核分枝杆菌T细胞免疫反应检测试剂盒(简称“试验试剂盒”)在体外定性检测疑似结核病患者新鲜外周静脉抗凝血中结核分枝杆菌特异性T细胞免疫反应结果的检测效能。方法:采用国产试验试剂盒与已上市进口产品(简称“对照试剂盒”),针对2020年11月至2021年6月陕西省结核病防治院收治的335例及2021年7月至2022年6月第四军医大学第一附属医院收治的343例疑似结核病患者的新鲜外周静脉抗凝血进行检测效能的比较研究。结果:678例外周静脉抗凝血样本中,以对照试剂盒为参考标准,试验试剂盒检测的敏感度为93.97%(327/348),特异度为96.06%(317/330),一致率为94.99%(644/678);以病原学诊断和临床诊断结果为参考标准,试验试剂盒检测的敏感度为82.93%(277/334),特异度为81.69%(281/344),一致率为82.30%(558/678),对照试剂盒检测的敏感度为87.13%(291/334),特异度为83.43%(287/344),一致率为85.25%(578/678);204例病原学阳性患者外周静脉抗凝血样本中,试验试剂盒的结核病检出率为82.35%(168/204),对照试剂盒的结核病检出率为88.24%(180/204);130例病原学阴性患者的外周静脉抗凝血样本中,试验试剂盒的结核病检出率为83.85%(109/130),对照试剂盒的结核病检出率为85.38%(111/130);在344例非结核肺部疾病患者外周静脉抗凝血样本中,两种试剂盒检测的一致率为95.35%(328/344),试验试剂盒检测的特异度为81.69%(281/344),对照试剂盒检测的特异度为83.43%(287/344)。结论:国产结核分枝杆菌T细胞免疫反应检测试剂盒与进口已上市试剂盒,对疑似结核病患者新鲜外周静脉抗凝血体外检测结核分枝杆菌特异性T细胞免疫反应的结果具有较高的一致性,可以作为疑似结核病患者的替代诊断工具。

Development and evaluation of immunoassay for zeranol in bovine urine

A high affinity polyclonal antibody-based enzyme linked immunosorbent assay （ELISA） was developed for the quantification of zeranol in bovine urine. On the basis of urine matrix studies, the optimized dilution factors producing insignificant matrix interference were selected as 1：5 in pretreatment. In the improved ELISA, the linear response range was between 0.02 and 1 μg/ml, and the detection limit was 0.02 μg/ml for the assay. The overall recoveries and the coefficients of variation （CVs） were in the range of 82%-127% and 3.5%-8.8%, respectively. Thirty-six bovine urine samples spiked with zeranol （ranging from 0.2 to 10 μg/ml） were detected by the ELISA and liquid chromatography （LC） method, and good correlations were obtained between the two methods （R^2=0.9643）. We conclude that this improved ELISA is suitable tool for a mass zeranol screening and can be an altemative for the conventional LC method for zeranol in bovine urine.

Study on the Production of Pentachloronitrobenzene Monoclonal Antibody and Its ELISA Kit for Rapid Detection

[Objectives]This study was conducted to develop an enzyme-linked immunoassay kit that can detect the residual amount of pentachloronitrobenzene in Penaeus vannamei.[Methods]This study was conducted to develop an enzyme-linked immunoassay kit that can detect the residual amount of pentachloronitrobenzene in P.vannamei.[Results]The standard curve range of the kit was 0-8.1μg/L;the detection limit for P.vannamei was 0.912μg/kg;the recovery was 80.6%-103.5%;and the relative standard deviation range within batches was 5.3%-10.1%,and the relative standard deviation range between batches was 6.7%-8.1%.The specificity of the pentachloronitrobenzene monoclonal antibody was relatively good,and the cross-reaction rates with pentachlorophenol,hexachlorobenzene,tetrachlorophthalide,and chlorothalonil were low,all of which did not exceed 30%.The ELISA kit could be stored at 4℃for 12 months,showing good stability.[Conclusions]The detection kit has low cost,short time and small deviation,and is an ideal preliminary screening method.

新霉素ELISA检测方法的建立

目的:比较直接和间接竞争酶联免疫法(enzyme linked immunosorbent assay,ELISA)的优缺点,建立新霉素残留ELISA检测方法。方法:利用自制的新霉素多克隆抗体,采用直接竞争和间接竞争ELISA方法检测新霉素残留,并比较两种方法的优缺点。结果:新霉素抗血清和庆大霉素的交叉反应率为2.04%,和卡那霉素的交叉反应率为0.02%,和氨苄青霉素、红霉素、四环素的交叉反应率均小于0.01%。初步测试新霉素间接竞争ELISA法的准确性和回收率。板内误差小于4%,板间误差小于11%,回收率为135.5%～191.3%。直接竞争和间接竞争ELISA方法的检测极限分别为28.58ng/mL和51.74ng/mL,达到了国家对新霉素规定的500μg/kg MRL检测限。结论:建立了直接竞争和间接ELISA吸附检测方法,条件优化更成功的间接竞争ELISA可用于开发新霉素检测试剂盒。

河豚毒素单抗ELISA检测试剂盒的研制

目的研制快速检测河豚鱼类中的河豚毒素(tetrodotoxin,TTX)试剂盒.方法在生产的抗TTX单克隆抗体基础上,利用间接竞争酶联免疫吸附方法研制TTX快速检测试剂盒.结果该试剂盒的最低检出浓度为5ng/ml,标准曲线的线性范围为5～500ng/ml,回归方程为Y＝-0.3546x+1.1006,r=0.99(P<0.05);河豚鱼25和100ng/ml 2个水平的加标回收率为72.45%～111.24%;试剂盒常温下可保存225d;与牛血清白蛋白(BSA)无交叉反应;实验室内的变异系数和实验室间的变异系数均<20%.结论该试剂盒快速、简单、灵敏,可满足实际工作需要.

黄曲霉毒素B1酶联免疫试剂盒稳定性研究

目的:研究自制黄曲霉毒素B1(AFB1)酶联免疫试剂盒在不同温度下的稳定性。方法:比较研制出的AFB1酶联免疫试剂盒在4℃和37℃保存条件下加入不同质量浓度的AFB1后其空白对照孔OD值的变化范围、IC20、IC50、IC80及RSD值的变化情况,及标准曲线的R2值等指标。结果:4℃保存270d空白对照孔OD值变化范围为1.129～1.777,IC20、IC50、IC80及RSD分别为0.05ng/mL和27.36%、0.27ng/mL和27.58%、0.92ng/mL和19.82%,该保存时间内各标准曲线线性关系良好(R2值均大于0.97);37℃加速破坏条件下保存13d内空白对照孔OD值变化范围为1.200～1.809,IC20、IC50、IC80及RSD变化分别为0.06ng/mL和27.71%、0.25ng/mL和25.66%、1.181ng/mL和21.89%,该保存时间内各标准曲线线性关系良好(R2值均大于0.98)。结论:研制的AFB1酶联免疫试剂盒在4℃和37℃加速破坏条件下分别保存270d和13d,试剂盒空白对照孔的OD值均大于1.0,各项指标可满足现场检测要求。

禽流感病毒夹心ELISA诊断试剂盒的研制及应用

将成熟的禽流感病毒(AIV)夹心ELISA快速检测方法组装成诊断试剂盒.试剂盒由1～11号试剂、一块酶标板和一份说明书组成.对试剂盒内各组份进行了特异性、敏感性、重复性及保存期的测定.结果表明,在-10℃下能保存6个月,而且特异性强、敏感性高、重复性好,操作简单、方便,能快速、准确地检测出样品中是否带有AIV抗原.先后制备了8个批次的诊断试剂盒,于湖北、安徽及河南等地的养禽场、兽医站、农科院、农业院校等化验室应用,取得了良好的效果.

酶联免疫吸附试验在食品检测中的应用

本文简要介绍了ELISA的基本原理和类型,详述了国内外使用ELISA方法在食品过敏源、农药残留、致病微生物、转基因等方面检测的最新研究进展,列出了部分目前市售用于食品检测的试剂盒,并对该检测技术的发展趋势及其在食品安全检测中的应用前景进行了展望。

三种ELISA试剂盒检测猪流行性乙型脑炎病毒血清IgG抗体比较

目的比较国内常用商品化ELISA试剂盒检测猪流行性乙型脑炎病毒血清IgG抗体的诊断效果。方法选用3种猪乙脑病毒血清IgG抗体ELISA检测试剂盒(Keqian,Lvshiyuan,Tianchen),以微量中和试验为金标准,对90份猪血清进行检测分析。结果中和试验的阳性检出率为34.4%(31/90),Keqian,Lvshiyuan和Tianchen阳性检出率分别为50.0%(45/90),47.8%(43/90)和38.9%(35/90)。灵敏度最高的是Keqian,为90.32%,但其特异度只有71.19%;Tianchen的灵敏度和特异度分别为83.87%和79.66%;Lvshiyuan的灵敏度和特异度分别仅为41.94%和16.95%。与中和试验比较,Tianchen试剂盒的κ系数最高为0.63,其次是Keqian为0.57,Lvshiyuan仅为0.04。显示3种试剂盒具稳定性。结论目前国内商品化猪乙脑病毒血清IgG抗体ELISA检测试剂盒诊断结果差异较大,与中和试验相比存在较高的假阴性,质量有待提高。

重症大疱性类天疱疮患者血清抗体变化规律与病情相关性的研究

目的：研究重症大疱性类天疱疮（ bullous pemphigoid ， BP ）患者血清中抗体BP180NC16a的酶联免疫吸附试验（ELISA）指数变化情况，观察其与病情变化的相关性，并分析用于病情监测和指导治疗的临床意义。方法对12例皮损面积＞50％的重症大疱性类天疱疮患者血清抗体BP180 NC16 a水平在不同时期进行监测及评分，并分析之间的关系。结果12例患者，平均年龄65岁，皮损面积均大于全身体表面积的50％以上。皮疹主要表现为疱壁紧张的大疱、水疱，部分有口腔黏膜损害。患者皮损面积和病情评分与血清抗体BP180NC16a-ELISA指数具有显著性关联（P＜0．05），患者疾病活动期和临床缓解期抗体BP180NC16a-ELISA指数几乎与病情呈平行变化，并且该指数可以预测病情，从而指导治疗。结论重症大疱性类天疱疮多为老年患者，病情危重，在发病早期不易诊断，因而延误治疗导致死亡。血清中抗体BP180 NC16 a-ELISA 指数可反映疾病的活动程度，用于病情监测，为治疗时根据个体差异选用适量的糖皮质激素快速控制病情提供了有利的实验室证据。

抗-HCV酶联免疫吸附试验试剂的评价

目的评价国内外11种抗-HCV酶联免疫吸附试验(ELISA)试剂的质量。方法采用艾滋病参比实验室基础血清盘、BBI阳转血清盘、美国CAP特性血清盘,对国产和进口的试剂进行质量测评。评价指标包括敏感性、特异性、阳性预测值、阴性预测值等。结果11种抗-HCV ELISA检测试剂的敏感性均为100%,多数试剂特异性>90%。阳转血清盘评价显示5种试剂平均延长天数<2d,大多数试剂未检出抗-NS3。所有试剂均检测能出抗核心区抗体。美国CAP特性血清盘评价显示所有试剂检测结果与标准结果一致率均为100%。结论11种抗-HCV酶联免疫吸附试验试剂有较高的敏感性,特异性有差异。由于ELISA抗-HCV试剂敏感性高,实用性强,适合于我国一般人群的筛查检测。

A MONOCLONAL ANTIBODY RECOGNIZING NON DERIVATIVE 13 HYDROXY GIBBERELLINS AND THEIR GLUCOSIDES *

The production and characterization of a monoclonal antibody (MAb AB10) against GA 3 glucoside as well as GA 3 is described. MAb AB10 was derived from an immunogen in which human serum albumin (HSA) was linked to GA 3 at carbon 3. This antibody showed high affinity for GA 3 glucoside as well as for 13 hydroxy gibberellins (GA 1, GA 3, GA 5, etc). The affinity of MAb AB10 for 13 hydroxy GAs was significantly reduced by methylation of the 7 oic acid but not by glycosylation of 3 hydroxyl group. Based on this antibody, both of competitive enzyme linked immunosorbent assays (ELISAs) for GA 3 glucoside and for GA 3 were developed. These two ELISAs displayed linear detection ranges from 0 2 pmol to 20 pmol. Using these assays, the fluctuation of GA 3 like and GA 3 glucoside like substances in the leaves of Rumex japonicus was investigated. The results indicated that the glycosylation of free GAs was connected with leaf senescence and that the function of 6 benzyl amino purine in retarding the leaf senescence was probably related to delaying the process of glycosylation of free GAs.

甲拌磷残留检测间接竞争ELISA试剂盒的研制

研制用于检测甲拌磷残留量的间接竞争ELISA试剂盒。甲拌磷包被抗原的最佳工作质量浓度为4mg/L,抗体的最佳稀释倍数为8000,甲拌磷多克隆抗体交叉反应率小于20%,甲拌磷抑制率回归曲线为y=18.846x+6.9949,在1～5000μg/L范围内呈线性关系,检测限为4.90μg/L,IC50为191.37μg/L。甲拌磷试剂盒的添加回收率均高于75%,供试样品检测结果的批内和批间变异系数均低于10%。试剂盒在4℃或-20℃下有效期为270d。

三种试剂盒与放射配体法检测谷氨酸脱羧酶抗体的比较

目的为合理选择谷氨酸脱羧酶抗体(GAD-Ab)检测试剂盒及准确判定结果提供依据。方法采用2种酶联免疫吸附测定(ELISA)试剂盒和1种免疫放射(IRMA)试剂盒检测88例已经放射配体(RLA)法核实抗体滴度的血清标本,对比各试剂盒检测结果与 RLA 法的一致性并选择一致性较好的试剂盒;与 RLA 法同时检测140例门诊连续就诊糖尿病患者的血清标本,确定经该试剂盒筛查后需采用 RLA 法复查标本的浓度范围。结果①3种试剂盒与 RLA 法检测结果一致性为Medizym 试剂盒(75%)>RSR 试剂盒(73.9%)>Biomerica 试剂盒(62.5%),Kappa 值分别为Medizym 试剂盒(0.408,中度)>RSR 试剂盒(0.405,中度)>Biomerica 试剂盒(0.185,较差);②3种试剂盒受试者工作特征(ROC)曲线下面积:Medizym 试剂盒(0.812)>RSR 试剂盒(0.727)>Biomerica 试剂盒(0.666);③3种试剂盒检测结果与 RLA 法相关性为 RSR 试剂盒(r=0.992)>Medizym 试剂盒(r=0.791)>Biomerica 试剂盒(r=-0.055);④RSR 试剂盒检测标本浓度为0.25～0.99 U/ml 者需进一步采用 RLA 法复查。结论 RSR 和 Medizym 试剂盒检测 GAD-Ab 效果较好。RSR 试剂盒检测GAD-Ab 浓度值为0.25～0.99 U/ml 时,建议采用 RLA 法复查。

不同品牌霉菌毒素检测试剂盒的质量评价

目的评价当前国内外应用较广的9个不同品牌黄曲霉毒素B1、玉米赤霉烯酮、呕吐毒素检测试剂盒的准确性。方法选取3种不同浓度的质控样品、4种饲料原料样品(玉米干全酒精糟、玉米胚芽粕、麦麸、豆粕)、2种饲料产品样品(蛋鸡配合饲料、牛浓缩饲料)。采用3种不同浓度的质控样(用萃取液点板6个孔)的检测结果变异系数(variable coefficient, CV)作为精密度评价指标。采用质控样的6个单独检测结果变异系数作为系统的精密度评价指标,采用实际样品的检测结果评价试剂盒的适用性。结果呕吐毒素试剂盒CV值平均值2号品牌2.7%, 3号品牌3.4%。玉米赤霉烯酮试剂盒CV值平均值3号品牌4.6%, 2号品牌5.5%, 4号品牌5.4%。黄曲霉毒素B1试剂盒CV值平均值5号品牌3.3%, 8号品牌3.7%, 2号品牌4.1%。结论依据试剂盒精密度、准确度、灵敏度和适应性综合评估2号品牌呕吐毒素试剂盒综合结果优秀, 9号品牌玉米赤霉烯酮试剂盒综合结果较好, 5号品牌黄曲霉毒素B1综合结果较好。同时,就检测上述3种常见毒素而言,没有发现一个品牌的试剂盒可以同时在多个毒素检测上表现优秀。