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对大肠杆菌天冬氨酸tRNA氨基酰化起重要作用的2'-羟基和磷酸基团的测定:一项核苷酸类似物干扰研究。

Determination of 2'-hydroxyl and phosphate groups important for aminoacylation of Escherichia coli tRNAAsp: a nucleotide analogue interference study.

作者信息

Vörtler C S, Fedorova O, Persson T, Kutzke U, Eckstein F

机构信息

Max-Planck-Institut für experimentelle Medizin, Göttingen, Germany.

出版信息

RNA. 1998 Nov;4(11):1444-54. doi: 10.1017/s1355838298980967.

Abstract

2'-Deoxynucleoside 5'-a-thiotriphosphates have been incorporated randomly, replacing any of the four nucleotides separately and at a low level in Escherichia colitRNA(AsP)transcripts. After some tRNAs were charged with the cognate aminoacyl-tRNA synthetase and biotinylated, charged and uncharged tRNAs were separated by binding to Streptavidin. A comparison of the iodine cleavage pattern of charged and uncharged tRNAs indicated positions of 2'-deoxyphosphorothioate interference with charging. To separate the 2'-deoxy from the phosphorothioate effect, the same sequence of reactions was performed with the corresponding NTPalphaS. Several positions were identified with a 2'-deoxy or a phosphorothioate effect. tRNAs with single deoxy substitutions at the identified positions were prepared by enzymatic ligation of chemically synthesized halves. The kinetics of charging these tRNAs were determined. The 2'-deoxy effects identified by the interference assay were confirmed, showing a reduction in charging efficiency of between 2.5-6-fold, except for the terminal A76 with a 25-fold reduction. Inspection of the X-ray structure of the tRNA-synthetase complex showed consistency of most of these findings. Critical 2'-deoxy groups are localized mainly on the proposed contact surface with the synthetase or at the interface of the two tRNA domains. The same overall picture emerged for critical phosphorothioates. With the exception of 2'-deoxy-adenosine-containing tRNAs, multiple 2'-deoxy-substituted tRNAs, prepared by ligation of halves, showed a much larger reduction in charging efficiency than the mono-substituted tRNAs, indicating an additive effect.

摘要

2'-脱氧核苷5'-α-硫代三磷酸已被随机掺入,分别以低水平取代大肠杆菌tRNA(AsP)转录本中的四种核苷酸中的任何一种。一些tRNA与同源氨酰-tRNA合成酶结合并生物素化后,通过与链霉亲和素结合分离已充电和未充电的tRNA。对已充电和未充电tRNA的碘裂解模式进行比较,表明2'-脱氧硫代磷酸酯干扰充电的位置。为了区分2'-脱氧效应和硫代磷酸酯效应,用相应的NTPαS进行相同的反应序列。确定了几个具有2'-脱氧或硫代磷酸酯效应的位置。通过化学合成的半段的酶促连接制备在确定位置具有单个脱氧取代的tRNA。测定了这些tRNA的充电动力学。通过干扰试验确定的2'-脱氧效应得到证实,除了末端A76充电效率降低25倍外,充电效率降低了2.5至6倍。对tRNA-合成酶复合物的X射线结构的检查表明,这些发现中的大多数是一致的。关键的2'-脱氧基团主要位于与合成酶的拟接触表面上或两个tRNA结构域的界面处。关键硫代磷酸酯的情况也是如此。除了含2'-脱氧腺苷的tRNA外,通过半段连接制备的多个2'-脱氧取代的tRNA的充电效率降低幅度比单取代的tRNA大得多,表明存在累加效应。

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