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RNA发夹的低能圆二色光谱揭示了λN抗终止活性所需的环构象。

Low energy CD of RNA hairpin unveils a loop conformation required for lambdaN antitermination activity.

作者信息

Johnson Neil P, Baase Walter A, von Hippel Peter H

机构信息

Institut de Pharmacologie et de Biologie Structurale, Toulouse, France.

出版信息

J Biol Chem. 2005 Sep 16;280(37):32177-83. doi: 10.1074/jbc.M504619200. Epub 2005 Jul 19.

DOI:10.1074/jbc.M504619200
PMID:16033760
Abstract

N protein coded by phage lambda is a transcription factor that stimulates the antitermination activity of Escherichia coli RNA polymerase by binding specifically to the nascent RNA transcript at a stemloop structure called boxB. We use a new biophysical technique, involving the monitoring of the low energy circular dichroism spectra of 2-aminopurine residues site-specifically placed in the boxB RNA loop, to investigate this binding interaction. The low energy CD spectra of these 2-aminopurine probes reflect specific asymmetric interactions with adjacent nucleotide bases. Consequently, these CD spectra provide detailed and specific conformational information about the RNA chain at these chromophores that cannot be obtained from changes in the related fluorescence signals of these probes. CD changes were observed on binding the N peptide to boxB RNA that correspond to structural changes that had been previously seen by NMR, thus validating our experimental approach. The low energy CD method was then used to quantify the ordered and disordered states of the free hairpin loop and to show that a significant fraction of the boxB loop assumes a product-like structure in the absence of protein. A boxB derivative with an intact stem and a reduced concentration of ordered loop was identified and used to show that the extent of the reaction between protein and boxB depends on the concentration of structured loop in the RNA reactant population. This result has general implications for the conformational specificity of RNA-protein interactions.

摘要

噬菌体λ编码的N蛋白是一种转录因子,它通过与一种名为boxB的茎环结构处的新生RNA转录本特异性结合,刺激大肠杆菌RNA聚合酶的抗终止活性。我们使用一种新的生物物理技术,即监测特异性定位在boxB RNA环中的2-氨基嘌呤残基的低能圆二色光谱,来研究这种结合相互作用。这些2-氨基嘌呤探针的低能CD光谱反映了与相邻核苷酸碱基的特定不对称相互作用。因此,这些CD光谱提供了关于这些发色团处RNA链的详细且特定的构象信息,而这些信息无法从这些探针相关荧光信号的变化中获得。在将N肽与boxB RNA结合时观察到了CD变化,这些变化与之前通过核磁共振观察到的结构变化相对应,从而验证了我们的实验方法。然后使用低能CD方法对游离发夹环的有序和无序状态进行定量,并表明在没有蛋白质的情况下,很大一部分boxB环呈现出类似产物的结构。鉴定出一种具有完整茎和降低的有序环浓度的boxB衍生物,并用于表明蛋白质与boxB之间反应的程度取决于RNA反应物群体中结构化环的浓度。这一结果对RNA-蛋白质相互作用的构象特异性具有普遍意义。

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