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通过定点诱变和铁(II)介导的切割鉴定聚腺苷酸特异性核糖核酸酶的活性位点

Identification of the active site of poly(A)-specific ribonuclease by site-directed mutagenesis and Fe(2+)-mediated cleavage.

作者信息

Ren Yan-Guo, Martínez Javier, Virtanen Anders

机构信息

Department of Cell and Molecular Biology, Uppsala University, BMC, Box 596, SE-751 24 Uppsala, Sweden.

出版信息

J Biol Chem. 2002 Feb 22;277(8):5982-7. doi: 10.1074/jbc.M111515200. Epub 2001 Dec 12.

DOI:10.1074/jbc.M111515200
PMID:11742007
Abstract

Poly(A)-specific ribonuclease (PARN) is the only mammalian exoribonuclease characterized thus far with high specificity for degrading the mRNA poly(A) tail. PARN belongs to the RNase D family of nucleases, a family characterized by the presence of four conserved acidic amino acid residues. Here, we show by site-directed mutagenesis that these residues of human PARN, i.e. Asp(28), Glu(30), Asp(292), and Asp(382), are essential for catalysis but are not required for stabilization of the PARN x RNA substrate complex. We have used iron(II)-induced hydroxyl radical cleavage to map Fe(2+) binding sites in PARN. Two Fe(2+) binding sites were identified, and three of the conserved acidic amino acid residues were important for Fe(2+) binding at these sites. Furthermore, we show that the apparent dissociation constant ((app)K(d)) values for Fe(2+) binding at both sites were affected in PARN polypeptides in which the conserved acidic amino acid residues were substituted to alanine. This suggests that these residues coordinate divalent metal ions. We conclude that the four conserved acidic amino acids are essential residues of the PARN active site and that the active site of PARN functionally and structurally resembles the active site for 3'-exonuclease domain of Escherichia coli DNA polymerase I.

摘要

聚(A)特异性核糖核酸酶(PARN)是迄今为止唯一一种对降解mRNA聚(A)尾具有高特异性的哺乳动物外切核糖核酸酶。PARN属于核酸酶的RNase D家族,该家族的特征是存在四个保守的酸性氨基酸残基。在这里,我们通过定点诱变表明,人PARN的这些残基,即Asp(28)、Glu(30)、Asp(292)和Asp(382),对催化作用至关重要,但对PARN x RNA底物复合物的稳定不是必需的。我们使用铁(II)诱导的羟基自由基切割来绘制PARN中的Fe(2+)结合位点。确定了两个Fe(2+)结合位点,并且三个保守的酸性氨基酸残基对这些位点的Fe(2+)结合很重要。此外,我们表明,在保守酸性氨基酸残基被替换为丙氨酸的PARN多肽中,两个位点上Fe(2+)结合的表观解离常数((app)K(d))值受到影响。这表明这些残基配位二价金属离子。我们得出结论,四个保守的酸性氨基酸是PARN活性位点的必需残基,并且PARN的活性位点在功能和结构上类似于大肠杆菌DNA聚合酶I的3'-外切核酸酶结构域的活性位点。

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