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作 者:殷波涛[1] 李佩珊[2] 李时君[2] 张春燕[1] 陈妍[1] 李方和[1]
机构地区:[1]华中科技大学同济医学院附属同济医院,武汉430030 [2]武汉生物制品研究所有限责任公司,武汉430064
出 处:《中国生物制品学杂志》2012年第9期1211-1213,共3页Chinese Journal of Biologicals
摘 要:目的建立A群脑膜炎球菌荚膜多糖(Group A meningococcal polysaccharide,GAMP)排溢法ELISA,并进行验证及初步应用。方法采用改良过碘酸盐氧化法制备抗GAMP-HRP。以抗GAMP单克隆抗体包被酶标板,抗GAMP-HRP作为酶标抗体,建立检测GAMP的排溢法ELISA。采用棋盘滴定法确定包被抗体及酶标抗体的最佳工作浓度,并对其特异性、敏感性及重复性进行验证。采用建立的排溢法ELISA检测GAMP-TT系列层析样品中的GAMP抗原活性,并与传统一步法ELISA及二步法ELISA进行比较。结果建立的排溢法ELISA的包被抗体最佳浓度为20μg/ml,酶标抗体最佳工作浓度为1∶128。该方法的特异性良好,敏感性与一步法和二步法相当,批内和批间变异系数与一步法相当;该方法检测GAMP-TT层析样品中的GAMP抗原活性的结果与二步法ELISA基本一致。结论排溢法ELISA的操作步骤与一步法ELISA大致相似,但较二步法ELISA显著简化,其对一步法ELISA中Hooks效应的纠正效果与二步法ELISA相同。Objective To develop,verify and preliminarily apply an excluded ELISA method for group A meningococcal polysaccharide(GAMP).Methods Anti-GAMP-HRP was prepared by modified periodate oxidation method.An excluded ELISA method was developed using anti-GAMP monoclonal antibody as coating antibody,and anti-GAMP-HRP as enzyme-labeled antibody.The working concentrations of coating and enzyme-labeled antibodies were optimized by checkerboard titration,and the developed method was verified for specificity,sensitivity and reproducibility.A series of GAMP-TT samples purified by chromatography were determined for GAMP antigen activity by the developed method,and the results were compared with those by traditional one-step and two-step ELISA methods.Results The optimal concentrations of coating and enzyme-labeled antibodies for development of excluded ELISA were 20 μg / ml and 1 ∶ 128 respectively.The developed method showed high specificity,of which the sensitivity was equivalent to those of one-step and two-step ELISA methods,while the intra-and inter-coefficients of variation were equivalent to those of one-step ELISA method.The determination results of GAMP antigen activities of GAMP-TT samples by the developed method were basically consistent with those by two-step ELISA method.Conclusion The procedure for excluded ELISA was similar to that for one-step ELISA method,while was significantly simplified as compared with that for two-step ELISA method.The correction efficiency of Hooks effect in one-step ELISA by the developed method was identical to that by two-step ELISA method.
关 键 词:A群脑膜炎球菌荚膜多糖 单克隆抗体 排溢法酶联免疫吸附测定
分 类 号:R378.15[医药卫生—病原生物学] R392-33[医药卫生—基础医学]
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