首页 | 本学科首页   官方微博 | 高级检索  
     

A New 4.0-Generation Dendrimer Phosphorescence Labeling Reagent and Its Application to Determination of Trace Alkaline Phosphatase by Affinity Adsorption Solid Substrate-room Temperature Phosphorimetry
引用本文:李志明 刘佳铭 陈晓华 杨敏岚 陈新华 施秀美. A New 4.0-Generation Dendrimer Phosphorescence Labeling Reagent and Its Application to Determination of Trace Alkaline Phosphatase by Affinity Adsorption Solid Substrate-room Temperature Phosphorimetry[J]. 中国化学, 2007, 25(10): 1529-1535. DOI: 10.1002/cjoc.200790281
作者姓名:李志明 刘佳铭 陈晓华 杨敏岚 陈新华 施秀美
作者单位:[1]Department of Food and Biological Engineering, Zhangzhou Institute of Technology, Zhangzhou, Fujian 363000, China [2]Department of Chemistry and Environmental Science, Zhangzhou Normal College, Zhangzhou, Fujian 363000, China
基金项目:Project supported by Fujian Province Natural Science Foundation (Nos. C0510028, D0510027, 2006J0386).
摘    要:A Triton X-100-4.0G-D (4.0G-D refers to a 4.0-generation dendrimer) was brought forward as a new phosphorescence labeling reagent. Two types of specific affinity adsorption (AA) reactions (direct method and sandwich method) were carried out between the labeling product of Triton X-100-4:0G-D-Wheat germ agglutinin (WGA) and alkaline phosphatase (ALP), the product of AA reaction preserved the good characteristics of room temperature phosphorescence (RTP) of 4.0G-D and △Ip of the product was proportional to the content of ALP. According to the fact stated above, a new method for the determination of trace ALP by affinity adsorption solid substrate-room temperature phosphorimetry (AA-SS-RTP) was established on the basis of WGA labeled with the Triton X-100-4.0G-D. The detection limits were 0.20 ag·spot^-1 (corresponding concentration: 5.0×10^-16 g·mL^-1, namely 5.0×10^-18 mol·L^-1) for a direct method and 0.14 ag·spot^-1 (corresponding concentration: 3.5×10^-16 g·mL^-1, namely 3.5×10^-18 mol·L^-1) for a sandwich method, respectively. For their high sensitivity, good repeatability and high accuracy, the direct method and sandwich method have been successfully appfied to determine the content of ALP in human serum, and the results were coincided with the clinical detection results of the enzyme-linked immunosorbent assay method by the Zhangzhou Hospital of Traditional Chinese Medicine. Meanwhile, the mechanism for the determination of trace ALP by AA-SS-RTP was discussed.

关 键 词:碱性磷酸酶 麦芽 凝集素 含量测定 磷光光度法
修稿时间:2007-01-11

A New 4.0-Generation Dendrimer Phosphorescence Labeling Reagent and Its Application to Determination of Trace Alkaline Phosphatase by Affinity Adsorption Solid Substrate-room Temperature Phosphorimetry
LI, Zhi-Ming LIU, Jia-Ming CHEN, Xiao-Hua YANG, Min-Lan CHEN, Xin-Hua SHI, Xiu-Mei. A New 4.0-Generation Dendrimer Phosphorescence Labeling Reagent and Its Application to Determination of Trace Alkaline Phosphatase by Affinity Adsorption Solid Substrate-room Temperature Phosphorimetry[J]. Chinese Journal of Chemistry, 2007, 25(10): 1529-1535. DOI: 10.1002/cjoc.200790281
Authors:LI   Zhi-Ming LIU   Jia-Ming CHEN   Xiao-Hua YANG   Min-Lan CHEN   Xin-Hua SHI   Xiu-Mei
Affiliation:a Department of Food and Biological Engineering, Zhangzhou Institute of Technology, Zhangzhou, Fujian 363000, China; b Department of Chemistry and Environmental Science, Zhangzhou Normal College, Zhangzhou, Fujian 363000, China
Abstract:A Triton X‐100‐4.0G‐D (4.0G‐D refers to a 4.0‐generation dendrimer) was brought forward as a new phosphorescence labeling reagent. Two types of specific affinity adsorption (AA) reactions (direct method and sandwich method) were carried out between the labeling product of Triton X‐100‐4.0G‐D‐Wheat germ agglutinin (WGA) and alkaline phosphatase (ALP), the product of AA reaction preserved the good characteristics of room temperature phosphorescence (RTP) of 4.0G‐D and ΔIP of the product was proportional to the content of ALP. According to the fact stated above, a new method for the determination of trace ALP by affinity adsorption solid substrate‐room temperature phosphorimetry (AA‐SS‐RTP) was established on the basis of WGA labeled with the Triton X‐100‐4.0G‐D. The detection limits were 0.20 ag·spot?1 (corresponding concentration: 5.0×10?16 g·mL?1, namely 5.0×10?18 mol·L?1) for a direct method and 0.14 ag·spot?1 (corresponding concentration: 3.5×10?16 g·mL?1, namely 3.5×10?18 mol·L?1) for a sandwich method, respectively. For their high sensitivity, good repeatability and high accuracy, the direct method and sandwich method have been successfully applied to determine the content of ALP in human serum, and the results were coincided with the clinical detection results of the enzyme‐linked immunosorbent assay method by the Zhangzhou Hospital of Traditional Chinese Medicine. Meanwhile, the mechanism for the determination of trace ALP by AA‐SS‐RTP was discussed.
Keywords:alkaline phosphatase   4.0-generation dendrimer   label   wheat germ agglutinin   affinity adsorption solid substrate-room temperature phosphorimetry
本文献已被 维普 等数据库收录!
设为首页 | 免责声明 | 关于勤云 | 加入收藏

Copyright©北京勤云科技发展有限公司  京ICP备09084417号