Literature DB >> 22065445

Quantification of transcript levels with quantitative RT-PCR.

Karen L Carleton1.   

Abstract

Differential gene expression is a key factor driving phenotypic divergence. Determining when and where gene expression has diverged between organisms requires a quantitative method. While large-scale approaches such as microarrays or high-throughput mRNA sequencing can identify candidates, quantitative RT-PCR is the definitive method for confirming gene expression differences. Here, we describe the steps for performing qRT-PCR including extracting total RNA, reverse-transcribing it to make a pool of cDNA, and then quantifying relative expression of a few candidate genes using real-time or quantitative PCR.

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Year:  2011        PMID: 22065445     DOI: 10.1007/978-1-61779-228-1_17

Source DB:  PubMed          Journal:  Methods Mol Biol        ISSN: 1064-3745


  9 in total

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8.  A unified analytic framework for prioritization of non-coding variants of uncertain significance in heritable breast and ovarian cancer.

Authors:  Eliseos J Mucaki; Natasha G Caminsky; Ami M Perri; Ruipeng Lu; Alain Laederach; Matthew Halvorsen; Joan H M Knoll; Peter K Rogan
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Authors:  Jie Wang; Kai Lu; Haipeng Nie; Qisen Zeng; Bowen Wu; Junjie Qian; Zhongming Fang
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  9 in total

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