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使用实时逆转录聚合酶链反应分析对mRNA进行绝对定量。

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

作者信息

Bustin S A

机构信息

Academic Department of Surgery, St Bartholomew's and the Royal London School of Medicine and Dentistry, Queen Mary and Westfield College, London E1 1BB, UK.

出版信息

J Mol Endocrinol. 2000 Oct;25(2):169-93. doi: 10.1677/jme.0.0250169.

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).

摘要

逆转录聚合酶链反应(RT-PCR)是检测低丰度mRNA最灵敏的方法,这种低丰度mRNA通常取自有限的组织样本。然而,它是一项复杂的技术,在其真正的灵敏度、可重复性和特异性方面存在诸多重大问题,并且作为一种定量方法,它还存在PCR固有的问题。最近引入的基于荧光的动力学RT-PCR方法显著简化了对mRNA进行可重复定量的过程,并有望克服这些局限性。尽管如此,它们的成功应用依赖于对实际问题的清晰理解,并且谨慎的实验设计、应用和验证对于准确的转录定量测量仍然至关重要。本综述讨论了所涉及的技术方面,对比了用于定量基因表达的传统RT-PCR方法和动力学RT-PCR方法,并比较了不同的动力学RT-PCR系统。通过展示管家基因家族甘油醛-3-磷酸脱氢酶(GAPDH)个体之间显著不同的转录水平,说明了这些检测方法的实用性。

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