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用于RNA定量的对照选择。

Control selection for RNA quantitation.

作者信息

Suzuki T, Higgins P J, Crawford D R

机构信息

Albany Medical College, NY, USA.

出版信息

Biotechniques. 2000 Aug;29(2):332-7. doi: 10.2144/00292rv02.

Abstract

The study of mammalian gene expression is often carried out at the level of mRNA. In such analyses, one usually measures the amount of an mRNA of interest under different conditions such as stress, growth, development, cell and tissue localization or as part of an evaluation of the effects of gene transfection. A variety of techniques exist to measure gene expression and most commonly involve Northern hybridization analysis, ribonuclease protection or RT-PCR. Common to all of these assays is the inclusion of a so-called loading or internal control (i.e., analysis of an mRNA that does not change in relative abundance during the course of treatments). Here, we discuss the uses and pitfalls of the most popular of these controls, glyceraldehyde 3-phosphate dehydrogenase (GAPDH) and beta-actin, with special emphasis on precautions associated with the use of GAPDH.

摘要

对哺乳动物基因表达的研究通常在mRNA水平上进行。在这类分析中,人们通常会测量在不同条件下(如应激、生长、发育、细胞和组织定位)感兴趣的mRNA的量,或者作为基因转染效果评估的一部分。存在多种测量基因表达的技术,最常见的包括Northern杂交分析、核糖核酸酶保护或RT-PCR。所有这些检测方法的共同之处在于都包含一个所谓的上样或内参对照(即分析在处理过程中相对丰度不变的mRNA)。在此,我们讨论这些对照中最常用的甘油醛-3-磷酸脱氢酶(GAPDH)和β-肌动蛋白的用途及陷阱,特别强调与使用GAPDH相关的注意事项。

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