首页> 美国卫生研究院文献>Nucleic Acids Research >Conformation of yeast 18S rRNA. Direct chemical probing of the 5 domain in ribosomal subunits and in deproteinized RNA by reverse transcriptase mapping of dimethyl sulfate-accessible.
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Conformation of yeast 18S rRNA. Direct chemical probing of the 5 domain in ribosomal subunits and in deproteinized RNA by reverse transcriptase mapping of dimethyl sulfate-accessible.

机译:酵母18S rRNA的构象。通过硫酸二甲酯可及的逆转录酶作图法直接化学探测核糖体亚基和脱蛋白RNA中的5域。

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摘要

The structure of the 5' domain of yeast 18S rRNA has been probed by dimethyl sulfate (DMS), either in "native" deproteinized molecules or in the 40S ribosomal subunits. DMS-reacted RNA has been used as a template for reverse transcription and a large number of reactive sites, corresponding to all types of bases have been mapped by a primer extension procedure, taking advantage of blocks in cDNA elongation immediately upstream from bases methylated at atom positions involved in the base-pair recognition of the template. Since the same atom positions are protected from DMS in base-paired nucleotides, the secondary structure status of each nucleotide can be directly assessed in this procedure, thus allowing to evaluate the potential contribution of proteins in modulating subunit rRNA conformation. While the DMS probing of deproteinized rRNA confirms a number of helical stems predicted by phylogenetic comparisons, it is remarkable that a few additional base-pairings, while proven by the comparative analysis, appear to require the presence of the bound ribosomal subunit proteins to be stabilized.
机译:酵母18S rRNA 5'结构域的结构已通过硫酸二甲酯(DMS)在“天然”脱蛋白分子或40S核糖体亚基中进行了探测。 DMS反应的RNA已被用作逆转录的模板,并且已通过引物延伸程序绘制了对应于所有类型碱基的大量反应位点,利用了在原子处甲基化的碱基紧邻上游的cDNA延伸中的嵌段模板的碱基对识别中涉及的位置。由于在碱基配对的核苷酸中相同的原子位置不受DMS的保护,因此可以在此过程中直接评估每个核苷酸的二级结构状态,从而可以评估蛋白质在调节亚基rRNA构象中的潜在作用。虽然DMS对脱蛋白rRNA的探测证实了系统发育比较所预测的许多螺旋茎,但值得注意的是,尽管通过比较分析证明了一些其他碱基配对,但似乎需要使结合的核糖体亚基蛋白稳定下来。

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