Quantitative polymerase chain reaction using a recombinant DNA internal standard and time resolved fluorometry

被引:24
作者
Bortolin, S [1 ]
Christopoulos, TK [1 ]
Verhaegen, M [1 ]
机构
[1] UNIV WINDSOR,DEPT CHEM & BIOCHEM,WINDSOR,ON N9B 3P4,CANADA
来源
ANALYTICAL CHEMISTRY | 1996年 / 68卷 / 05期
关键词
D O I
10.1021/ac950898o
中图分类号
O65 [分析化学];
学科分类号
070302 ; 081704 ;
摘要
Using a 308 bp DNA fragment (target DNA) as a template, we have synthesized an internal standard (IS) that is of the same size and uses the same primers as the target but differs by a 26 bp centrally located sequence. We then designed quantitative polymerase chain reaction (PCR) assays in which the target DNA is coamplified with a constant amount of IS (20 000 molecules). The presence of IS compensates for the reaction-to-reaction variability of the amplification efficiency. The PCR products are assayed by two distinct hybridization protocols. The first approach (QPCR-1) requires that specific probes be immobilized onto microtiter wells, followed by hybridization with digoxigenin-labeled PCR product. In the second protocol (QPCR-2), PCR product is captured onto the wells and hybridized with digoxigenin-tailed specific probes, In both assays, the hybrids are detected using an anti-digoxigenin-alkaline phosphatase conjugate and 5'-fluorosalicylphosphate as substrate, The hydrolysis product forms a highly fluorescent complex with Tb3+-EDTA, as measured by time-resolved fluorometry. The ratio of the fluorescence values obtained for the amplified target DNA and IS is linearly related to the number of target DNA molecules present in the sample prior to amplification, The linear ranges are 1000-200 000 molecules for QPCR-1 and 2000-200 000 molecules for QPCR-2, The CVs ranged from 3.4 to 9.7%.
引用
收藏
页码:834 / 840
页数:7
相关论文
共 23 条
[1]   POLYMERASE CHAIN-REACTION STRATEGY [J].
ARNHEIM, N ;
ERLICH, H .
ANNUAL REVIEW OF BIOCHEMISTRY, 1992, 61 :131-156
[2]   ABSOLUTE MESSENGER-RNA QUANTIFICATION USING THE POLYMERASE CHAIN-REACTION (PCR) - A NOVEL-APPROACH BY A PCR AIDED TRANSCRIPT TITRATION ASSAY (PATTY) [J].
BECKERANDRE, M ;
HAHLBROCK, K .
NUCLEIC ACIDS RESEARCH, 1989, 17 (22) :9437-9446
[3]   TIME-RESOLVED IMMUNOFLUOROMETRIC DETERMINATION OF SPECIFIC MESSENGER-RNA SEQUENCES AMPLIFIED BY THE POLYMERASE CHAIN-REACTION [J].
BORTOLIN, S ;
CHRISTOPOULOS, TK .
ANALYTICAL CHEMISTRY, 1994, 66 (23) :4302-4307
[4]   QUANTIFICATION OF POLYMERASE CHAIN-REACTION PRODUCTS IN AGAROSE GELS WITH A FLUORESCENT EUROPIUM CHELATE AS LABEL AND TIME-RESOLVED FLUORESCENCE SPECTROSCOPY [J].
CHAN, A ;
DIAMANDIS, EP ;
KRAJDEN, M .
ANALYTICAL CHEMISTRY, 1993, 65 (02) :158-163
[5]   DETECTION OF SPECIFIC DNA-SEQUENCES BY FLUORESCENCE AMPLIFICATION - A COLOR COMPLEMENTATION ASSAY [J].
CHEHAB, FF ;
KAN, YW .
PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1989, 86 (23) :9178-9182
[6]   ENZYMATICALLY AMPLIFIED TIME-RESOLVED FLUORESCENCE IMMUNOASSAY WITH TERBIUM CHELATES [J].
CHRISTOPOULOS, TK ;
DIAMANDIS, EP .
ANALYTICAL CHEMISTRY, 1992, 64 (04) :342-346
[7]   MAXIMIZING SENSITIVITY AND SPECIFICITY OF PCR BY PREAMPLIFICATION HEATING [J].
DAQUILA, RT ;
BECHTEL, LJ ;
VIDELER, JA ;
ERON, JJ ;
GORCZYCA, P ;
KAPLAN, JC .
NUCLEIC ACIDS RESEARCH, 1991, 19 (13) :3749-3749
[8]   EUROPIUM CHELATE LABELS IN TIME-RESOLVED FLUORESCENCE IMMUNOASSAYS AND DNA HYBRIDIZATION ASSAYS [J].
DIAMANDIS, EP ;
CHRISTOPOULOS, TK .
ANALYTICAL CHEMISTRY, 1990, 62 (22) :A1149-+
[9]   ENZYME-AMPLIFIED LANTHANIDE LUMINESCENCE FOR ENZYME DETECTION IN BIOANALYTICAL ASSAYS [J].
EVANGELISTA, RA ;
POLLAK, A ;
TEMPLETON, EFG .
ANALYTICAL BIOCHEMISTRY, 1991, 197 (01) :213-224
[10]   ANALYSIS OF CYTOKINE MESSENGER-RNA AND DNA - DETECTION AND QUANTITATION BY COMPETITIVE POLYMERASE CHAIN-REACTION [J].
GILLILAND, G ;
PERRIN, S ;
BLANCHARD, K ;
BUNN, HF .
PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1990, 87 (07) :2725-2729
123