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Mechanism of Exonuclease I stimulation by the single-stranded DNA-binding protein

机译:单链DNA结合蛋白刺激核酸外切酶I的机制

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Bacterial single-stranded (ss) DNA-binding proteins (SSBs) bind and protect ssDNA intermediates formed during cellular DNA replication, recombination and repair reactions. SSBs also form complexes with an array of genome maintenance enzymes via their conserved C-terminal tail (SSB-Ct) elements. In many cases, complex formation with SSB stimulates the biochemical activities of its protein partners. Here, we investigate the mechanism by which Escherichia coli SSB stimulates hydrolysis of ssDNA by Exonuclease I (ExoI). Steady-state kinetic experiments show that SSB stimulates ExoI activity through effects on both apparent k(cat) and K-m. SSB variant proteins with altered SSB-Ct sequences either stimulate more modestly or inhibit ExoI hydrolysis of ssDNA due to increases in the apparent Michaelis constant, highlighting a role for protein complex formation in ExoI substrate binding. Consistent with a model in which SSB stabilizes ExoI substrate binding and melts secondary structures that could impede ExoI processivity, the specific activity of a fusion protein in which ExoI is tethered to SSB is nearly equivalent to that of SSB-stimulated ExoI. Taken together, these studies delineate stimulatory roles for SSB in which protein interactions and ssDNA binding are both important for maximal activity of its protein partners.
机译:细菌单链(ss)DNA结合蛋白(SSB)结合并保护在细胞DNA复制,重组和修复反应过程中形成的ssDNA中间体。 SSB还通过其保守的C末端尾巴(SSB-Ct)元素与一系列基因组维持酶形成复合物。在许多情况下,与SSB形成复合物会刺激其蛋白质伴侣的生化活性。在这里,我们调查大肠埃希氏菌SSB通过核酸外切酶I(ExoI)刺激ssDNA水解的机制。稳态动力学实验表明,SSB通过对视在k(cat)和K-m的影响来刺激ExoI活性。由于表观米氏常数增加,SSB-Ct序列改变的SSB变体蛋白要么刺激性更小,要么抑制ssDNA的ExoI水解,从而突出了蛋白质复合物在ExoI底物结合中的作用。与其中SSB稳定ExoI底物结合并融化可能阻碍ExoI合成能力的二级结构的模型一致,其中ExoI束缚于SSB的融合蛋白的比活性几乎与SSB刺激的ExoI相当。综上所述,这些研究描述了SSB的刺激作用,其中蛋白质相互作用和ssDNA结合对于其蛋白质伴侣的最大活性都是重要的。

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