首页> 美国卫生研究院文献>Nucleic Acids Research >Effect of the higher-order structure of tRNAs on the stability of hybrids with oligodeoxyribonucleotides: separation of tRNA by an efficient solution hybridization.
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Effect of the higher-order structure of tRNAs on the stability of hybrids with oligodeoxyribonucleotides: separation of tRNA by an efficient solution hybridization.

机译:tRNA高阶结构对寡聚脱氧核糖核苷酸杂交体稳定性的影响:通过有效的溶液杂交分离tRNA。

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摘要

In the course of developing a method to purify a single tRNA species efficiently, we have examined hybridization efficiencies between some tRNAs and short oligodeoxyribonucleotide probes both by the filter and solution hybridization methods without denaturants. The hybridization efficiencies varied considerably among probes which are complementary to different regions of the tRNAs, although there was little efficiency variation in the probes toward DNA substrates including the same nucleotide sequence. This efficiency variation was shown to be due to tRNA-specific higher-order structures as well as a hypermodified nucleotide in the anticodon loop. Characterization of the tRNA-probe hybrids by both nondenaturing gel electrophoresis and chemical modification showed the existence of two stable hybridizing states as a function of ionic strength. Our results indicate that RNA molecules with a number of intramolecular base pairings are able to form stable hybrids with complementary sequences under nondenaturing conditions. On the basis of these data, an appropriate probe was designed to successfully purify yeast tRNA(Phe) by making a tRNA(Phe)-probe hybrid, which has a longer retention time in hydroxyapatite high performance liquid chromatography than the tRNA(Phe) itself.
机译:在开发一种有效纯化单个tRNA物种的方法的过程中,我们已经通过不使用变性剂的滤膜和溶液杂交方法研究了某些tRNA与短寡脱氧核糖核苷酸探针之间的杂交效率。在与tRNA的不同区域互补的探针之间,杂交效率差异很大,尽管探针对包括相同核苷酸序列的DNA底物几乎没有效率变化。该效率变化被证明是由于tRNA特异性的高阶结构以及反密码子环中的超修饰核苷酸所致。通过非变性凝胶电泳和化学修饰对tRNA-探针杂种进行表征的过程表明,存在两种稳定的杂交状态,这是离子强度的函数。我们的结果表明,具有多个分子内碱基配对的RNA分子能够在非变性条件下与互补序列形成稳定的杂交体。根据这些数据,设计了一种合适的探针,可通过制备tRNA(Phe)-探针杂种来成功纯化酵母tRNA(Phe),该杂种在羟基磷灰石高效液相色谱中的保留时间比tRNA(Phe)本身更长。

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