QUANTIFICATION OF POLYMERASE CHAIN-REACTION PRODUCTS IN AGAROSE GELS WITH A FLUORESCENT EUROPIUM CHELATE AS LABEL AND TIME-RESOLVED FLUORESCENCE SPECTROSCOPY

被引：25

作者：

CHAN, A

DIAMANDIS, EP

KRAJDEN, M

机构：

[1] TORONTO HOSP, TORONTO WESTERN DIV, DEPT CLIN BIOCHEM, 399 BATHURST ST, TORONTO M5T 2S8, ON, CANADA

[2] UNIV TORONTO, DEPT CLIN BIOCHEM & MICROBIOL, TORONTO M5G 1L5, ONTARIO, CANADA

[3] TORONTO HOSP, TORONTO WESTERN DIV, DEPT MICROBIOL, TORONTO M5T 2S8, ON, CANADA

来源：

ANALYTICAL CHEMISTRY | 1993年 / 65卷 / 02期

关键词：

D O I：

10.1021/ac00050a012

中图分类号：

O65 [分析化学];

学科分类号：

070302 ; 081704 ;

摘要：

We have 5'-end-labeled one polymerase chain reaction (PCR) primer with the europium chelator 4,7-bis(chlorosulfophenyl)-1,10-phenanthroline-2,9-dicarboxylic acid (BCPDA). After performing PCR in the presence of another unlabeled primer, we separated the 362 bp PCR product with 2% low melting point agarose gel electrophoresis. The gel was then immersed into a Eu3+ solution. During soaking, Eu3+ diffuses into the gel and associates with BCPDA to form a fluorescent complex of long fluorescence lifetime. This complex can be quantified by scanning the gel with a time-resolved fluorometric reader. Because BCPDA and Eu3+ are not fluorescent by themselves, background signals are very low. The detection limit was about 5 ng of DNA. We have also shown that the BCPDA-labeled product could be blotted and detected on the membrane by using an anti-BCPDA antibody. These two technologies may find applications other than in PCR, e.g. in fluorescence-based DNA sequencing and in solution hybridization.

引用

页码：158 / 163

页数：6

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