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Exoribonuclease R in Mycoplasma genitalium can carry out both RNA processing and degradative functions and is sensitive to RNA ribose methylation

机译:生殖器支原体中的核糖核酸外切酶R既可以进行RNA加工,又可以进行降解,并且对RNA核糖甲基化敏感

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Mycoplasma genitalium, a small bacterium having minimal genome size, has only one identified exoribonuclease, RNase R (MgR). We have purified MgR to homogeneity, and compared its RNA degradative properties to those of its Escherichia coli homologs RNase R (EcR) and RNase II (EcII). MgR is active on a number of substrates including oligoribonucleotides, poly(A), rRNA, and precursors to tRNA. Unlike EcR, which degrades rRNA and pre-tRNA without formation of intermediate products, MgR appears sensitive to certain RNA structural features and forms specific products from these stable RNA substrates. The 3'-ends of two MgR degradation products of 23S rRNA were mapped by RT-PCR to positions 2499 and 2553, each being 1 nucleotide downstream of a 2'-O- methylation site. The sensitivity of MgR to ribose methylation is further demonstrated by the degradation patterns of 16S rRNA and a synthetic methylated oligoribonucleotide. Remarkably, MgR removes the 3'-trailer sequence from a pre-tRNA, generating product with the mature 3'-end more efficiently than EcII does. In contrast, EcR degrades this pre-tRNA without the formation of specific products. Our results suggest that MgR shares some properties of both EcR and EcII and can carry out a broad range of RNA processing and degradative functions.
机译:生殖支原体是一种具有最小基因组大小的小型细菌,仅具有一种已鉴定的外切核糖核酸酶RNase R(MgR)。我们已经纯化了MgR,使其具有同质性,并将其RNA降解特性与其大肠杆菌同系物RNase R(EcR)和RNase II(EcII)进行了比较。 MgR在许多底物上具有活性,包括寡核糖核苷酸,poly(A),rRNA和tRNA的前体。与EcR降解rRNA和pre-tRNA而不会形成中间产物不同,MgR似乎对某些RNA结构特征敏感,并从这些稳定的RNA底物形成特定的产物。通过RT-PCR将23S rRNA的两个MgR降解产物的3'末端定位到位置2499和2553,每个位置在2'-O-甲基化位点的下游1个核苷酸。 MgR对核糖甲基化的敏感性由16S rRNA和合成的甲基化寡核糖核苷酸的降解模式进一步证明。值得注意的是,MgR从pre-tRNA上去除了3'尾序列,比EcII更有效地产生了具有成熟3'末端的产物。相反,EcR降解了该pre-tRNA,而没有形成特异性产物。我们的结果表明,MgR具有EcR和EcII的某些特性,并且可以进行多种RNA加工和降解功能。

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