Marisa L. Wong scite author profile

Real-time PCR has become one of the most widely used methods of gene quantitation because it has a large dynamic range, boasts tremendous sensitivity, can be highly sequence-specific, has little to no post-amplification processing, and is amenable to increasing sample throughput. However, optimal benefit from these advantages requires a clear understanding of the many options available for running a real-time PCR experiment. Starting with the theory behind real-time PCR, this review discusses the key components of a real-time PCR experiment, including one-step or two-step PCR, absolute versus relative quantitation, mathematical models available for relative quantitation and amplification efficiency calculations, types of normalization or data correction, and detection chemistries. In addition, the many causes of variation as well as methods to calculate intra- and inter-assay variation are addressed.

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Structural characterization of the mouse high growth deletion and discovery of a novel fusion transcript between suppressor of cytokine signaling-2 ( Socs-2 ) and viral encoded semaphorin receptor ( Plexin C1 )

Wong

Islas‐Trejo

Medrano

2002

Gene

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Wong

Medrano

2005

BioTechniques

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Marisa L. Wong

Real-Time PCR for mRNA Quantitation

Structural characterization of the mouse high growth deletion and discovery of a novel fusion transcript between suppressor of cytokine signaling-2 ( Socs-2 ) and viral encoded semaphorin receptor ( Plexin C1 )

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