首页> 美国卫生研究院文献>Nucleic Acids Research >Studies on the primary structure of the ribosomal 23S RNA of Escherichia coli: II. A characterisation and an alignment of 24 sections spanning the entire molecule and its application to the localisation of specific fragments.
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Studies on the primary structure of the ribosomal 23S RNA of Escherichia coli: II. A characterisation and an alignment of 24 sections spanning the entire molecule and its application to the localisation of specific fragments.

机译:大肠杆菌核糖体23S RNA一级结构的研究:II。跨越整个分子的24个部分的表征和比对及其在特定片段的定位中的应用。

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摘要

We have employed new methodology to obtain 23S RNA fragments which includes a) the digestion of the RNA within 50S subunits and b) the limited hydrolysis of the 13S and 18S fragments. By comparing all 23S RNA fragments, obtained heretofore, we have characterised and aligned 24 sections of this RNA spanning nearly the entire molecule. These results allow the localisation of any new 23S RNA fragment by comparison of the fingerprint of its T1 ribonuclease digest to the characteristic ones of the different sections. In this way we obtained a more definite localisation of the binding sites of the 50S proteins L1, L5, L9, L18, L20, L23 and L25. We also specified a ribonuclease sensitive region of 23S RNA in native 50S subunits, extending from the 1100th nucleotide from the 5' end to the 1000th nucleotide from the 3' end; this region contains a cluster of 5 modified nucleotides and may be at the subunit interface.
机译:我们采用了新的方法来获得23S RNA片段,包括a)消化50S亚基中的RNA,以及b)13S和18S片段的有限水解。通过比较迄今获得的所有23S RNA片段,我们已经表征并对齐了该RNA的24个部分,几乎覆盖了整个分子。通过比较其T1核糖核酸酶消化物的指纹图谱与不同部分的特征图谱,这些结果可以定位任何新的23S RNA片段。通过这种方式,我们获得了50S蛋白L1,L5,L9,L18,L20,L23和L25的结合位点的更明确的定位。我们还指定了天然50S亚基中23S RNA的核糖核酸酶敏感区,从5'端的第1100个核苷酸延伸到3'端的第1000个核苷酸;该区域包含5个修饰核苷酸的簇,可能位于亚基界面。

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