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Quantification of HIV-1 DNA Using Real-Time Recombinase Polymerase Amplification
Author(s) -
Zachary Crannell,
Brittany A. Rohrman,
Rebecca Richards–Kortum
Publication year - 2014
Publication title -
analytical chemistry
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 2.117
H-Index - 332
eISSN - 1520-6882
pISSN - 0003-2700
DOI - 10.1021/ac5011298
Subject(s) - recombinase polymerase amplification , nucleic acid , chemistry , dna , standard curve , real time polymerase chain reaction , recombinase , dna polymerase , digital polymerase chain reaction , polymerase , microbiology and biotechnology , computational biology , polymerase chain reaction , chromatography , biochemistry , biology , recombination , loop mediated isothermal amplification , gene
Although recombinase polymerase amplification (RPA) has many advantages for the detection of pathogenic nucleic acids in point-of-care applications, RPA has not yet been implemented to quantify sample concentration using a standard curve. Here, we describe a real-time RPA assay with an internal positive control and an algorithm that analyzes real-time fluorescence data to quantify HIV-1 DNA. We show that DNA concentration and the onset of detectable amplification are correlated by an exponential standard curve. In a set of experiments in which the standard curve and algorithm were used to analyze and quantify additional DNA samples, the algorithm predicted an average concentration within 1 order of magnitude of the correct concentration for all HIV-1 DNA concentrations tested. These results suggest that quantitative RPA (qRPA) may serve as a powerful tool for quantifying nucleic acids and may be adapted for use in single-sample point-of-care diagnostic systems.

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