Absolute quantification of mRNA using real-time reverse transcription polymerase chain reaction assays

SA Bustin - Journal of molecular endocrinology, 2000 - jme.bioscientifica.com
Journal of molecular endocrinology, 2000jme.bioscientifica.com
The reverse transcription polymerase chain reaction (RT-PCR) is the most sensitive method
for the detection of low-abundance mRNA, often obtained from limited tissue samples.
However, it is a complex technique, there are substantial problems associated with its true
sensitivity, reproducibility and specificity and, as a quantitative method, it suffers from the
problems inherent in PCR. The recent introduction of fluorescence-based kinetic RT-PCR
procedures significantly simplifies the process of producing reproducible quantification of …
Abstract
The reverse transcription polymerase chain reaction (RT-PCR) is the most sensitive method for the detection of low-abundance mRNA, often obtained from limited tissue samples. However, it is a complex technique, there are substantial problems associated with its true sensitivity, reproducibility and specificity and, as a quantitative method, it suffers from the problems inherent in PCR. The recent introduction of fluorescence-based kinetic RT-PCR procedures significantly simplifies the process of producing reproducible quantification of mRNAs and promises to overcome these limitations. Nevertheless, their successful application depends on a clear understanding of the practical problems, and careful experimental design, application and validation remain essential for accurate quantitative measurements of transcription. This review discusses the technical aspects involved, contrasts conventional and kinetic RT-PCR methods for quantitating gene expression and compares the different kinetic RT-PCR systems. It illustrates the usefulness of these assays by demonstrating the significantly different levels of transcription between individuals of the housekeeping gene family, glyceraldehyde-3-phosphate-dehydrogenase (GAPDH).
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