Quantitative RT-PCR: Pitfalls and Potential

Willard M. Freeman(Wake Forest University), Stephen J. Walker(Wake Forest University), Kent E. Vrana(Wake Forest University)
BioTechniques
January 1, 1999
10.2144/99261rv01
Cited by 1,145Open Access
Full Text

Abstract

Reverse transcription PCR (RT-PCR) represents a sensitive and powerful tool for analyzing RNA. While it has tremendous potential for quantitative applications, a comprehensive knowledge of its technical aspects is required. Successful quantitative RT-PCR involves correction for experimental variations in individual RT and PCR efficiencies. This review addresses the mathematics of RT-PCR, choice of RNA standards (internal vs. external) and quantification strategies (competitive, noncompetitive and kinetic [real-time] amplification). Finally, the discussion turns to practical considerations in experimental design. It is hoped that this review will be appropriate for those undertaking these experiments for the first time or wishing to improve (or validate) a technique in what is frequently a confusing and contradictory field.

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