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RNase P: role of distinct protein cofactors in tRNA substrate recognition and RNA-based catalysis

机译:RNase P:不同的蛋白质辅助因子在tRNA底物识别和基于RNA的催化中的作用

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摘要

The Escherichia coli ribonuclease P (RNase P) has a protein component, termed C5, which acts as a cofactor for the catalytic M1 RNA subunit that processes the 5' leader sequence of precursor tRNA. Rpp29, a conserved protein subunit of human RNase P, can substitute for C5 protein in reconstitution assays of M1 RNA activity. To better understand the role of the former protein, we compare the mode of action of Rpp29 to that of the C5 protein in activation of M1 RNA. Enzyme kinetic analyses reveal that complexes of M1 RNA-Rpp29 and M1 RNA-C5 exhibit comparable binding affinities to precursor tRNA but different catalytic efficiencies. High concentrations of substrate impede the activity of the former complex. Rpp29 itself exhibits high affinity in substrate binding, which seems to reduce the catalytic efficiency of the reconstituted ribonucleoprotein. Rpp29 has a conserved C-terminal domain with an Sm-like fold that mediates interaction with M1 RNA and precursor tRNA and can activate M1 RNA. The results suggest that distinct protein folds in two unrelated protein cofactors can facilitate transition from RNA- to ribonucleoprotein-based catalysis by RNase P.
机译:大肠杆菌核糖核酸酶P(RNase P)具有蛋白质成分,称为C5,它充当催化M1 RNA亚基的辅因子,该亚基处理前体tRNA的5'前导序列。 Rpp29是人RNase P的保守蛋白亚基,可以在M1 RNA活性的重组测定中替代C5蛋白。为了更好地了解前一种蛋白的作用,我们比较了Rpp29与C5蛋白在M1 RNA激活中的作用方式。酶动力学分析表明,M1 RNA-Rpp29和M1 RNA-C5的复合物表现出与前体tRNA相当的结合亲和力,但催化效率不同。高浓度的底物阻碍了前复合物的活性。 Rpp29本身对底物结合表现出高亲和力,这似乎降低了重组核糖核蛋白的催化效率。 Rpp29具有一个保守的C末端结构域,具有Sm样折叠,可介导与M1 RNA和前体tRNA的相互作用,并可以激活M1 RNA。结果表明,两个不相关的蛋白质辅因子中独特的蛋白质折叠可以促进RNase P从RNA过渡到基于核糖核蛋白的催化。

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