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Characterization of Mg~(2+) Binding to the DNA Repair Protein Apurinic/Apyrimidic Endonuclease 1 via Solid-State ~(25)Mg NMR Spectroscopy

机译:通过固态〜(25)Mg NMR光谱表征Mg〜(2+)与DNA修复蛋白Apurinic / Apyrimidic核酸内切酶1的结合

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Apurinic/apyrimidinic endonuclease 1 (APE1), a member of the divalent cation-dependent phosphoesterase super-family of proteins that retain the conserved four-layered α/β-sandwich structural core, is an essential protein that functions as part of base excision repair to remove mutagenic and cytotoxic abasic sites from DNA. Using low-temperature solid-state ~(25)Mg NMR spectroscopy and various mutants of APE1, we demonstrate that Mg~(2+) binds to APE1 and a functional APE1-substrate DNA complex with an overall stoichiometry of one Mg~(2+) per mole of APE1 as predicted by the X-ray work of Tainer and co-workers (Mol, C. D.; Kuo, C. F.; Thayer, M. M.; Cunningham, R. P.; Tainer, J. A. Nature 1995, 374, 381 -386). However, the NMR spectra show that the single Mg~(2+) site is disordered. We discuss the probable reasons for the disorder at the Mg~(2+) binding site. The most likely source of this disorder is arrangement of the protein-ligands about the Mg~(2+) (cis and trans isomers). The existence of these isomers reinforces the notion of the plasticity of the metal binding site within APE1.
机译:Apurinic / apyrimidinic内切核酸酶1(APE1)是蛋白质的二价阳离子依赖性磷酸酯酶超家族的成员,该家族保留了保守的四层α/β-三明治结构核心,是一种必需的蛋白质,可作为碱基切除修复的一部分去除DNA的诱变和细胞毒性无碱基位点。使用低温固态〜(25)Mg NMR光谱和APE1的各种突变体,我们证明Mg〜(2+)与APE1和功能性APE1底物DNA复合物结合,总化学计量为一个Mg〜(2由Tainer及其同事(Mol,CD; Kuo,CF; Thayer,MM; Cunningham,RP; Tainer,JA Nature 1995,374,381 -386)的X射线工作预测,每摩尔APE1的+。然而,NMR光谱显示单个Mg〜(2+)位点是无序的。我们讨论了Mg〜(2+)结合位点的疾病的可能原因。该疾病最可能的原因是围绕Mg〜(2+)的蛋白质配体(顺式和反式异构体)的排列。这些异构体的存在加强了APE1中金属结合位点可塑性的概念。

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