Department of Biological Sciences, 111 Research Drive, Iacocca Hall D226, Bethlehem, PA 18015-4732, USA.
Anal Biochem. 2010 Apr 15;399(2):230-6. doi: 10.1016/j.ab.2009.12.037. Epub 2010 Jan 4.
An important molecular mechanism to create protein diversity from a limited set of genes is A-to-I RNA editing. RNA editing converts single adenosines into inosines in pre-mRNA. These single base conversions can have a wide variety of consequences. Editing can lead to codon changes and, consequently, altered protein function. Moreover, editing can alter splice sites and influences miRNA biogenesis and target recognition. The two enzymes responsible for editing in mammals are adenosine deaminase acting on RNA (ADAR) 1 and 2. However, it is currently largely unknown how the activity of these enzymes is regulated in vivo. Editing activity does not always correlate with ADAR expression levels, suggesting posttranscriptional or posttranslational mechanisms for controlling activity. To investigate how editing is regulated in mammalian cells, we have developed a straightforward quantitative reporter system to detect editing levels. By employing luciferase activity as a readout, we could easily detect different levels of editing in a cellular context. In addition, increased levels of ADAR2 correlated with increased levels of luciferase activity. This reporter system therefore sets the stage for the effective screening of cDNA libraries or small molecules for strong modulators of intracellular editing to ultimately elucidate how A-to-I editing is regulated in vivo.
产生蛋白质多样性的一个重要分子机制是 A 到 I 的 RNA 编辑。RNA 编辑将前体 mRNA 中的单个腺苷酸转换为肌苷。这些单碱基转换可能产生广泛的后果。编辑可以导致密码子的改变,从而改变蛋白质的功能。此外,编辑可以改变剪接位点,并影响 miRNA 的生物发生和靶标识别。在哺乳动物中负责编辑的两种酶是腺嘌呤脱氨酶作用于 RNA(ADAR)1 和 2。然而,目前对于这些酶的活性在体内是如何被调节的还知之甚少。编辑活性并不总是与 ADAR 表达水平相关,这表明存在转录后或翻译后机制来控制其活性。为了研究编辑在哺乳动物细胞中的调控机制,我们开发了一种简单的定量报告系统来检测编辑水平。通过将荧光素酶活性作为读出信号,我们可以在细胞环境中轻松检测到不同水平的编辑。此外,ADAR2 水平的增加与荧光素酶活性水平的增加相关。因此,该报告系统为筛选 cDNA 文库或小分子调节剂以最终阐明体内 A 到 I 编辑的调控机制奠定了基础。
