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化学发光酶免疫方法检测克伦特罗残留 总被引:11,自引:0,他引:11
建立了间接竞争化学发光酶免疫法(competitive indirect chemilumine scent enzyme immunoassy,ic-CLEIA)检测猪尿中残留克伦特罗(clenbuterol,CLB)的方法,并优化了竞争反应时间,Tween-20含量,PBS离子强度与pH4个参数。优化后的ic-CLEIA检出限可达0.01μg/L,检测范围为0.04~25.8μg/L,ED50为0.54μg/L;尿样检测的平均回收率为98%~120%,批内与批间相对标准偏差(variation of coefficent,CV)均小于10%。这些参数均优于目前广泛使用的ELISA方法,说明本CLEIA方法可替代ELISA法,用于实际尿样的检测。 相似文献
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酱油与白酒中邻苯二甲酸二甲酯的化学发光酶免疫分析方法研究 总被引:2,自引:0,他引:2
本研究以邻苯二甲酸二甲酯( DMP)为研究目标,以4-氨基邻苯二甲酸二甲酯为半抗原,通过重氮化法偶联载体蛋白并免疫动物,制备针对DMP的特异性兔多克隆抗体。通过棋盘滴定法和单因素实验确定最佳的实验参数,即包被原浓度为50μg/L,一抗浓度为92.5μg/L,二抗浓度为1μg/mL,药物稀释液为pH 6.0的纯水,竞争反应时间为40 min,基于此建立了间接竞争化学发光酶联免疫分析法检测DMP。本方法对DMP的检出限为0.29μg/L,线性检测范围为0.74~30.32μg/L,与13种结构和功能类似物的交叉反应率均<5%,通过倍比稀释降低白酒、酱油样品基质干扰,对样品的平均回收率在80.2%~116.0%之间,平均相对标准偏差<3.6%,结果与GC-MS法的测定结果相符。本方法适用于食品样品中DMP的快速检测。 相似文献
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叙述了化学发光免疫分析的分类及特点,从发光底物、增强剂、过氧化物酶、过氧化物及其他方面,对鲁米诺类化合物化学发光酶免疫分析的进展进行了综述,引用文献34篇。 相似文献
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以吡虫啉原药和3-巯基丙酸为原料,合成了吡虫啉半抗原,通过活泼酯法将其与载体蛋白钥孔血蓝蛋白(KLH)、牛血清白蛋白(BSA)偶联制备得到完全抗原,经免疫Balb/c雌性小鼠并与骨髓瘤细胞融合获得吡虫啉单克隆抗体,建立了用于吡虫啉检测的间接竞争化学发光酶联免疫分析方法(ic-CLEIA)。优化了方法的包被原稀释倍数、抗体稀释倍数、缓冲液种类、缓冲液的pH值、一抗竞争反应时间、酶标二抗稀释倍数等条件,最适条件为:包被原质量浓度62.50 ng/mL(稀释16 000倍),抗体质量浓度103.12 ng/mL(稀释64 000倍),缓冲液PBS(pH 7.4),抗原与抗体竞争反应时间30 min,酶标二抗稀释倍数1∶7 000。结果表明,在最适条件下该方法的检出限(IC10)为0.03 ng/mL,IC50为0.57 ng/mL,线性检测范围(IC20 ~ IC80)为0.083 ~ 3.99 ng/mL。与氯噻啉的交叉反应率为2.2%,与噻虫胺、呋虫胺、啶虫脒、噻虫啉、噻虫嗪5种吡虫啉结构类似物无明显交叉反应。对黄瓜和苹果样品的加标回收率为82.0% ~ 112%,相对标准偏差小于15%。实际样品检测结果与HPLC仪器方法相关性良好(r2 = 0.989)。结果表明,所建立的ic-CLEIA方法具有特异性强、灵敏度高的特点,可用于食品中吡虫啉残留的快速检测。 相似文献
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化学发光酶免疫法检测猪肉中氯丙嗪残留 总被引:4,自引:0,他引:4
采用棋盘滴定法确定包被抗原浓度和抗体稀释倍数,通过单因素实验优化了竞争反应时间、磷酸盐缓冲液浓度、甲醇含量、pH值等参数,建立了氯丙嗪的间接竞争化学发光酶免疫检测方法,并考察了方法的特异性、灵敏度和稳定性.结果表明,最佳反应条件为包被抗原浓度为0.05 μg/L;氯丙嗪抗体稀释32000倍;体系缓冲液为含10%甲醇、0.1 mol/L磷酸盐缓冲液(pH 7.0).本方法的IC50为0.12 μg/L;检出限为0.02 μg/L;线性范围0.02~24.78 μg/L;批内和批间相对标准偏差均小于10%.与其它结构类似物没有明显交叉反应.猪肉检测的平均回收率为87.4%~105.6%,与高效液相色谱方法的相关性良好.本方法具有较高的灵敏度和较好的稳定性. 相似文献
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针对保健食品中西地那非药物的非法添加问题,该研究采用辣根过氧化物酶(HRP)与鲁米诺为信号输出系统,结合直接竞争模式探索了保健食品中西地那非的直接竞争化学发光酶免疫分析方法。基于特异性多克隆抗体,通过逐步优化策略,确定最佳免疫分析条件为:包被原质量浓度为41.67 ng/mL,酶标抗体质量浓度为1.25 μg/mL,封闭液和洗涤液的吐温-20含量为0.05%,稀释液的甲醇添加量为5%,竞争反应时间为40 min。在该条件下,建立了西地那非的直接竞争化学发光免疫分析方法,该方法对西地那非的半抑制浓度(IC50)为0.17 ng/mL,线性检测范围(IC20~IC80)为0.024 ~ 1.21 ng/mL,检出限(IC10,LOD)为0.008 ng/mL。与他达那非等功能类似物无显著交叉;西地那非样品的加标回收率为82.0%~114%,相对标准偏差均小于15%。盲样检测结果与HPLC-MS/MS确证方法具有良好一致性,说明该方法准确可靠,适用于样品中西地那非的快速筛查。 相似文献
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增强化学发光酶免疫法对猪肉中盐酸克伦特罗的检测 总被引:4,自引:0,他引:4
建立了猪肉中克伦特罗(CLB)的直接竞争化学发光酶免疫检测(dc-CLEIA)方法。通过优化离子强度、pH值确立了化学发光酶免疫法的标准曲线,优化后dc-CLEIA的检出限可达0.02μg/L。猪肉中的盐酸克伦特罗用高氯酸提取、SPE净化后绘制基质曲线,基质曲线与标准曲线吻合,说明基质影响基本消除。测定0.10、1.0、5.0μg/kg 3个水平的添加回收率,平均回收率为83%~98%,批内与批间的相对标准偏差均小于15%。进一步研究了dc-CLEIA与HPLC两种方法测定猪肉样品的相关性,结果显示两者测定结果相关性良好,r=0.964 7,说明所建立的直接化学发光酶免疫方法可用于实际样品的检测,结果准确可靠。 相似文献
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化学发光酶免疫法测定游离三碘甲腺原氨酸 总被引:4,自引:0,他引:4
以辣根过氧化物酶为三碘甲腺原氨酸类似物的标记物,鲁米诺为化学发光反应底物,建立了一种高灵敏度化学发光免疫检测游离三碘甲腺原氨酸的方法。该法线性范围为0.90~80 ng/L,批内变异小于12.1%,批间相对标准偏差均小于15%,其余各项指标均良好。利用本法对血清样品进行了测定,关于甲状腺机能亢进组病人的临床诊断符合率达到83.3%。与其它化学发光免疫分析方法比较所得相关系数为0.9005。在方法条件选择上,以尽可能保持游离激素和蛋白结合激素之间的平衡为原则,提高游离三碘甲腺原氨酸浓度测定的准确性。 相似文献
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《Analytical letters》2012,45(17):2844-2856
Enrofloxacin, a widely used fluoroquinolone antibiotic, may be a cause of bacterial drug resistance and is forbidden in poultry. Consequently, a sensitive and rapid method is required for its determination. Aptamers, which are more stable and easily synthesized than antibodies, may serve as alternatives in the development of methods for rapid detection. Six single-strand DNA aptamers binding to enrofloxacin were selected by in vitro selection. Aptamer number 17 showed the highest affinity for enrofloxacin with a dissociation constant of 188 nM and the highest guanine concentration (35%), which was predicted to be crucial for strong affinity of the aptamer to enrofloxacin, and successfully distinguished enrofloxacin from its structure analogs. Using aptamer number 17, a novel chemiluminescent enzyme immunoassay associating with biotin-streptavidin was developed that allowed the determination of enrofloxacin to 2.26 ng/mL. Due to its capability to determine enrofloxacin in bovine milk, this newly selected aptamer may find broad application in food and environmental monitoring. 相似文献
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《Analytical letters》2012,45(16):1279-1289
Abstract The coupling of an enzyme immunoassay for factor VIII-related antigen with a commercial glucose oxidase based amperometric sensor permits the determination of 1.6 to 16 ng of factor XIII-related antigen in human plasma. Further pure amperometric sensors or amperometric enzyme sensors for determination of the main marker-enzymes of enzyme immunoassays are described. 相似文献
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Yuhui Chen Hang Ao Wencheng Xiao Prof. Huangxian Ju Prof. Jie Wu 《Chemistry (Weinheim an der Bergstrasse, Germany)》2022,28(67):e202201425
Simple but robust testing assays are essential for screening and diagnosis of individuals infected with severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2) in COVID-19 pandemic. Here, we described a chemiluminescent imaging assay (CLIA) for sensitive and convenient detection of SARS-CoV-2 nucleocapsid protein (NP) by a target-induced enzyme activity regulation (T-EAR) strategy. The T-EAR used a pair of antibody-DNA probes to recognize SARS-CoV-2 NP and proximity-induce rolling circle amplification for mass-production of pyrophosphate to coordinate with Cu2+, which prevented the reduction of Cu2+ to Cu+ by sodium ascorbate as well as the Cu+-caused inactivation of horseradish peroxidase (HRP). The activity retention of HRP produced strong CL signal for the detection of SARS-CoV-2 NP by catalyzing the oxidation of luminol by H2O2. The T-EAR based CLIA showed a wide detection range from 1 pg/mL to 100 ng/mL (13 fM to 1.3 nM) with the requirement of only 0.75 μL of sample. This CLIA had advantages of good sensitivity, simple wash-free operation, acceptable accuracy, and high-throughput imaging detection, displaying potential applicability in screening assay of COVID-19 infection. 相似文献
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《Analytical letters》2012,45(8):1841-1859
Abstract A flow-injection sandwich enzyme immunoassay for human IgG as model antigen by using horseradish peroxidase as label, polystyrene beads as solid support, and the enhanced chemiluminescence reaction for peroxidase quantitation is described. the kinetics of antigen—immobilized antibody interaction has been studied and the quantitative time-concentration ranges of reactions have been estimated. Each of the two immunochemical steps of analysis have been pursued in the kinetic regime. the time for each immunochemical step was reduced to 2–3 min. the enhanced luminescent reaction involving luminol and p-iodophenol as substrates was used to detect the peroxidase label. the conditions for chemiluminescent reaction were optimized. the detection limit for peroxidase in a 3 min assay was 5–10?16 moles/tube. the detection limit for IgG, in the developed immunoassay, is 10?9 M, the overall time of the assay being 5–10 min. 相似文献
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《Analytical letters》2012,45(14):2189-2202
An ultra-sensitive indirect competitive chemiluminescence enzyme immunoassay was developed for screening diethylstilbestrol in fish and shrimp samples. The concentration of diethylstilbestrol that caused 50% inhibition of the binding enzyme marker (IC50) was 0.32 ng/mL and the limit of detection was 0.0068 ng/mL; the linear range was from 0.028 ng/mL to 3.60 ng/mL. The assay showed cross-reactivity of 7.1% and 2.8% with dienestrol and hexoestrol, respectively, but negligible cross-reactivity with estradiol, estrone, ethinyloestradiol, and progestin. The recovery from spiked fish and shrimp samples varied from 68.5% to 92.5%, and the mean coefficients of variation within groups and between groups were 6.2% and 8.0%, respectively. Our results indicated that the assay is a simple, sensitive, specific, and accurate method for screening fish and shrimp samples for diethylstilbestrol. 相似文献