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Crystal structure of RNase T, an exoribonuclease involved in tRNA maturation and end turnover

机译:核糖核酸酶T的晶体结构,核糖核酸外切核酸酶参与tRNA的成熟和最终转换

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摘要

The 31 processing of most bacterial precursor tRNAs involves exonucleolytic trimming to yield a mature CCA end. This step is carried out by RNase T, a member of the large DEDD family of exonucleases. We report the crystal structures of RNase T from Escherichia coli and Pseudomonas aeruginosa, which show that this enzyme adopts an opposing dimeric arrangement, with the catalytic DEDD residues from one monomer closely juxtaposed with a large basic patch on the other monomer. This arrangement suggests that RNase T has to be dimeric for substrate specificity, and agrees very well with prior site-directed mutagenesis studies. The dimeric architecture of RNase T is very similar to the arrangement seen in oligoribonuclease, another bacterial DEDD family exoribonuclease. The catalytic residues in these two enzymes are organized very similarly to the catalytic domain of the third DEDD family exoribonuclease in E. coli, RNase D, which is monomeric.
机译:大多数细菌前体tRNA的31种加工涉及核酸外切酶修饰,以产生成熟的CCA末端。此步骤由RNase T(大型DEDD核酸外切酶家族的成员)进行。我们报告了大肠杆菌和铜绿假单胞菌的RNase T的晶体结构,表明该酶采用相反的二聚体排列,其中一种单体的催化DEDD残基与另一单体上的大碱性贴片紧密并置。这种安排表明,RNA酶T必须是二聚体以用于底物特异性,并且与先前的定点诱变研究非常吻合。 RNase T的二聚体结构与另一种细菌DEDD家族外切核糖核酸酶寡核糖核酸酶中的排列非常相似。这两种酶中的催化残基的组成与大肠杆菌中第三个DEDD家族外切核糖核酸酶的RNase D的催化结构域非常相似,后者是单体。

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