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硒修饰寡核糖核苷酸的化学合成及其酶促连接生成U6小核RNA茎环片段

Chemical synthesis of selenium-modified oligoribonucleotides and their enzymatic ligation leading to an U6 SnRNA stem-loop segment.

作者信息

Höbartner Claudia, Micura Ronald

机构信息

Institute of Organic Chemistry, Leopold Franzens University, Innrain 52a, A-6020 Innsbruck, Austria.

出版信息

J Am Chem Soc. 2004 Feb 4;126(4):1141-9. doi: 10.1021/ja038481k.

DOI:10.1021/ja038481k
PMID:14746483
Abstract

The derivatization of nucleic acids with selenium is highly promising to facilitate nucleic acids structure determination by X-ray crystallography using the multiwavelength anomalous dispersion (MAD) technique. The foundation for such an approach has been laid by Huang, Egli, and co-workers and was exemplified on small DNA duplexes. Here, we present a comprehensive study on the preparation of RNAs containing 2'-Se-methylpyrimidine nucleoside labels. This includes the synthesis of a novel 2'-Se-methylcytidine phosphoramidite 11 and its incorporation into oligoribonucleotides by solid-phase synthesis. Deprotection of the oligonucleotides is achieved in the presence of millimolar amounts of threo-1,4-dimercapto-2,3-butandiol (DTT). With this additive, oxidation products and follow-up side-products are suppressed and acceptable HPLC traces of the crude material are obtained, so far tested for sequences of up to 22-mers. Moreover, an extensive investigation on the enzymatic ligation of the selenium-containing oligoribonucleotides demonstrates the high flexibility of the selenium approach. Our target sequence, an U6 snRNA stem-loop motif comprising all naturally occurring nucleoside modifications beside the Se-label is achieved by ligation using T4 RNA ligase.

摘要

用硒对核酸进行衍生化,对于利用多波长反常散射(MAD)技术通过X射线晶体学确定核酸结构而言,极具前景。黄、埃格利及其同事已为此类方法奠定了基础,并以小DNA双链体为例进行了说明。在此,我们对含2'-硒甲基嘧啶核苷标记的RNA的制备进行了全面研究。这包括一种新型2'-硒甲基胞苷亚磷酰胺11的合成及其通过固相合成掺入寡核糖核苷酸。在存在毫摩尔量的苏式-1,4-二巯基-2,3-丁二醇(DTT)的情况下实现寡核苷酸的脱保护。有了这种添加剂,氧化产物和后续副产物受到抑制,获得了粗产物可接受的HPLC图谱,目前已对长达22聚体的序列进行了测试。此外,对含硒寡核糖核苷酸的酶促连接进行的广泛研究证明了硒方法的高度灵活性。我们的目标序列是一个U6 snRNA茎环基序,除了硒标记外,包含所有天然存在的核苷修饰,通过使用T4 RNA连接酶进行连接来实现。

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