首页> 外文OA文献 >Cleavage of intron from the standard or non-standard position of the precursor tRNA by the splicing endonuclease of Aeropyrum pernix, a hyper-thermophilic Crenarchaeon, involves a novel RNA recognition site in the Crenarchaea specific loop
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Cleavage of intron from the standard or non-standard position of the precursor tRNA by the splicing endonuclease of Aeropyrum pernix, a hyper-thermophilic Crenarchaeon, involves a novel RNA recognition site in the Crenarchaea specific loop

机译:通过剪接Aeropyrum pernix的内切核酸酶从前体tRNA的标准或非标准位点切割内含子,这是一种超嗜热的克雷夏鱼,在克雷夏鱼特异性环中涉及一个新的RNA识别位点

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摘要

In Crenarchaea, several tRNA genes are predicted to express precursor-tRNAs (pre-tRNAs) with canonical or non-canonical introns at various positions. We initially focused on the tRNAThr species of hyperthermophilic crenarchaeon, Aeropyrum pernix (APE) and found that in the living APE cells three tRNAThr species were transcribed and subsequently matured to functional tRNAs. During maturation, introns in two of them were cleaved from standard and non-standard positions. Biochemical studies revealed that the APE splicing endonuclease (APE-EndA) removed both types of introns, including the non-canonical introns, without any nucleotide modification. To clarify the underlying reasons for broad substrate specificity of APE-EndA, we determined the crystal structure of wild-type APE-EndA and subsequently compared its structure with that of Archaeaoglobus fulgidus (AFU)-EndA, which has narrow substrate specificity. Remarkably, structural comparison revealed that APE-EndA possesses a Crenarchaea specific loop (CSL). Introduction of CSL into AFU-EndA enhanced its intron-cleaving activity irrespective of the position or motif of the intron. Thus, our biochemical and crystallographic analyses of the chimera-EndA demonstrated that the CSL is responsible for the broad substrate specificity of APE-EndA. Furthermore, mutagenesis studies revealed that Lys44 in CSL functions as the RNA recognition site.
机译:在Crenarchaea中,预计有几种tRNA基因会在不同位置表达具有规范或非规范内含子的前体tRNA(pre-tRNA)。我们最初将重点放在嗜热火球鱼的tRNAThr物种,即Aeropyrum pernix(APE),发现在活的APE细胞中转录了三种tRNAThr物种,并随后成熟为功能性tRNA。在成熟过程中,其中两个内含子从标准和非标准位置切割下来。生化研究表明,APE拼接核酸内切酶(APE-EndA)去除了两种类型的内含子,包括非规范内含子,而没有任何核苷酸修饰。为了弄清APE-EndA广泛底物特异性的根本原因,我们确定了野生型APE-EndA的晶体结构,然后将其结构与具有狭窄底物特异性的fulglodus fulgidus(AFU)-EndA的晶体结构进行了比较。值得注意的是,结构比较表明APE-EndA具有Crenarchaea特异环(CSL)。将CSL引入AFU-EndA可以增强其内含子切割活性,而与内含子的位置或基序无关。因此,我们对嵌合体EndA的生化和晶体学分析表明CSL负责APE-EndA的广泛底物特异性。此外,诱变研究表明CSL中的Lys44充当RNA识别位点。

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