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首页> 外文期刊>Nucleic Acids Research >Identifying the methyltransferases for m(5)U747 and m(5)U1939 in 23S rRNA using MALDI mass spectrometry
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Identifying the methyltransferases for m(5)U747 and m(5)U1939 in 23S rRNA using MALDI mass spectrometry

机译:使用MALDI质谱法鉴定23S rRNA中m(5)U747和m(5)U1939的甲基转移酶

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摘要

There are three sites of m(5)U modification in Escherichia coli stable RNAs: one at the invariant tRNA position U54 and two in 23S rRNA at the phylogenetically conserved positions U747 and U1939. Each of these sites is modified by its own methyltransferase, and the tRNA methyltransferase, TrmA, is well-characterised. Two open reading frames, YbjF and YgcA, are approximately 30% identical to TrmA, and here we determine the functions of these candidate methyltransferases using MALDI mass spectrometry. A purified recombinant version of YgcA retains its activity and specificity, and methylates U1939 in an RNA transcript in vitro. We were unable to generate a recombinant version of YbjF that retained in vitro activity, so the function of this enzyme was defined in vivo by engineering a ybjF knockout strain. Comparison of the methylation patterns in 23S rRNAs from YbjF(+) and YbjF(-) strains showed that the latter differed only in the lack of the m(5)U747 modification. With this report, the functions of all the E.coli m(5)U RNA methyltransferases are identified, and a more appropriate designation for YbjF would be RumB (RNA uridine methyltransferases B), in line with the recent nomenclature change for YgcA (now RumA).
机译:在大肠杆菌稳定的RNA中存在m(5)U修饰的三个位点:一个位于不变的tRNA位置U54,两个位于23S rRNA的系统发育保守位置U747和U1939。这些位点中的每一个都被其自己的甲基转移酶修饰,而tRNA甲基转移酶TrmA具有良好的特性。两个开放阅读框YbjF和YgcA与TrmA大约30%相同,在这里我们使用MALDI质谱法确定这些候选甲基转移酶的功能。纯化的YgcA重组体保留其活性和特异性,并在体外RNA转录物中甲基化U1939。我们无法产生保留体外活性的重组YbjF,因此该酶的功能在体内通过工程化ybjF敲除菌株来定义。 YbjF(+)和YbjF(-)菌株的23S rRNA中甲基化模式的比较表明,后者仅在缺少m(5)U747修饰的情况下有所不同。通过此报告,鉴定了所有大肠杆菌m(5)U RNA甲基转移酶的功能,根据最近YgcA命名法的变化,现在更合适的YbjF命名为RumB(RNA尿苷甲基转移酶B)。 RumA)。

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