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基于核酸适配体-质粒DNA复合物信号放大的荧光免疫传感技术
引用本文:朱静,黄勇,蒋小平,谭钟扬,蒋健晖,沈国励,俞汝勤.基于核酸适配体-质粒DNA复合物信号放大的荧光免疫传感技术[J].分析化学,2009,37(11).
作者姓名:朱静  黄勇  蒋小平  谭钟扬  蒋健晖  沈国励  俞汝勤
作者单位:湖南大学化学化工学院化学生物传感与计量学国家重点实验室,长沙,410082
基金项目:国家"十一五"重大科技支撑计划  
摘    要:提出了一种简便、高灵敏的荧光免疫传感新技术,通过抗体/抗原/核酸适配体-质粒DNA复合物的特异性识别与双链质粒DNA与荧光染料SYBR Green Ⅰ的嵌合作用, 实现对血小板衍生增长因子BB(PDGF-BB)的检测.生物识别反应在微孔板中进行,PDGF-BB抗原与微孔板底部预包被的PDGF-BB抗体免疫反应后,加入核酸适配体-质粒DNA复合物与抗原形成夹心复合物.加入DNA双链嵌合染料SYBR Green Ⅰ与夹心复合物的双链DNA部分结合可产生强荧光,其荧光强度可用于定量测定PDGF-BB浓度.实验考察了离子浓度、核酸适配体的延伸引物片段与质粒PUC19的反应比例、染料SYBR Green Ⅰ浓度等分析条件对荧光信号的影响.在优化反应条件下,PDGF-BB检测的线性范围为0.2~200 μg/L,检出限为0.1 μg/L,并且实现了对人血清中PDGF-BB的定量检测.

关 键 词:核酸适配体  血小板衍生增长因子  核酸适配体-质粒脱氧核糖核酸复合物  免疫传感

A New Fluorescence Immunosensing Method Based on Aptamer-plasmid Complex Amplification
ZHU Jing,HUANG Yong,JIANG Xiao-Ping,TAN Zhong-Yang,JIANG Jian-Hui,SHEN Guo-Li,YU Ru-Qin.A New Fluorescence Immunosensing Method Based on Aptamer-plasmid Complex Amplification[J].Chinese Journal of Analytical Chemistry,2009,37(11).
Authors:ZHU Jing  HUANG Yong  JIANG Xiao-Ping  TAN Zhong-Yang  JIANG Jian-Hui  SHEN Guo-Li  YU Ru-Qin
Institution:ZHU Jing,HUANG Yong,JIANG Xiao-Ping,TAN Zhong-Yang,JIANG Jian-Hui,SHEN Guo-Li,YU Ru-Qin ( State Key Laboratory of Chemo/Biosensing and Chemometrics,Hunan University,Changsha 410082)
Abstract:A novel simple,sensitive fluorescence immunosensing method based on aptamer-plasmid complex amplification was developed. This method utilized the specific recognition between antibody and antigen as well as aptamer-plasmid complex and the intercalation of fluorescence dye SYBR Green Ⅰ in the groove of duplex plasmid DNA in detection of Platelet-Derived Growth Factor BB (PDGF-BB). The immunoassay was performed in the microtiter wells in which rabbit anti PDGF-BB antibody was immobilized. The PDGF BB analyte was captured by the primary antibody and then sandwiched by the aptamer-plasmid DNA complex. The introduction of fluorescence dye SYBR Green Ⅰ allows for the detection of the sandwiched immunocomplex of antibody/anigen/aptamer-plasmid complex. Under the optimized conditions of salt concentration,ratio of aptamer to PUC19,and SYBR Green Ⅰ concentration,the proposed method offers a linear detection range from 0.2 μg/L to 200 μg/L with a detection limit of 0.1μg/L.
Keywords:Aptamer  platelet-derived growth factor  aptamer-plasmid complex  immunosense  
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