Issue 7, 2008

Analysis of DNA and single-base mutations using magnetic particles for purification, amplification and DNAzyme detection

Abstract

The amplified detection of DNA or of single-base mismatches in DNA is achieved by the use of nucleic acid-functionalized magnetic particles that separate the recognition duplexes and, upon amplification, yield chemiluminescence-generating DNAzymes as reporter units. The analysis of M13 phage ssDNA is achieved by the hybridization of the analyte to capture nucleic acid-functionalized magnetic particles followed by the binding of a DNA machine unit to the analyte domain. The magnetic separation of the multi-component-functionalized magnetic particles, followed by their reaction with polymerase, dNTPs, and the nicking enzyme (Nb.BbvCI) activate the autonomous synthesis of the horseradish peroxidase-mimicking DNAzyme that acts as chemiluminescent reporter. The single-base mutation in DNA is achieved by coupling of the DNA machine to the mutant DNA/capture nucleic acid-functionalized magnetic particles hybrid structure. The activation of the polymerization/nicking cycles yield the chemiluminescent reporting DNAzyme. The magnetic separation of the DNA recognition hybrids improves the signal-to-noise ratio of the analytical protocol as compared to related DNAzyme synthesizing schemes.

Graphical abstract: Analysis of DNA and single-base mutations using magnetic particles for purification, amplification and DNAzyme detection

Article information

Article type
Paper
Submitted
05 Feb 2008
Accepted
17 Mar 2008
First published
23 Apr 2008

Analyst, 2008,133, 923-927

Analysis of DNA and single-base mutations using magnetic particles for purification, amplification and DNAzyme detection

I. Willner, Z. Cheglakov, Y. Weizmann and E. Sharon, Analyst, 2008, 133, 923 DOI: 10.1039/B802015A

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