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Site-directed mutagenesis reveals roles for conserved amino acid residues in the hexameric DNA helicase DnaB from Bacillus stearothermophilus

机译:定点诱变揭示了嗜热脂肪芽孢杆菌六聚体DNA解旋酶DnaB中保守氨基酸残基的作用

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摘要

Site-directed mutagenesis studies on conserved amino acid residues within motifs H1, H1a, H2 and H3 of the hexameric replicative helicase DnaB from Bacillus stearothermophilus revealed specific functions associated with these residues. In particular, residues that coordinate a bound Mg2+ in the active site (T217 and D320) are important for the function of the enzyme but are not required for the formation of stable hexamers. A conserved glutamic acid (E241) in motif H1a is likely to be involved in the activation of a water molecule for in line attack on the γ-phosphate of the bound nucleotide during catalysis. A conserved glutamine (Q362) in motif H3 acts as a γ-phosphate sensor and mediates the conformational coupling of nucleotide- and DNA-binding sites. The nature of the residue at this position is also important for the primase-mediated activation of DnaB, suggesting that primase uses the same conformational coupling pathway to induce its stimulatory effect on the activity of DnaB. Together, these mutations reveal a conservation of many aspects of biochemical activity in the active sites of monomeric and hexameric helicases.
机译:对来自嗜热脂肪芽孢杆菌的六聚体复制解旋酶DnaB的基序H1,H1a,H2和H3中保守氨基酸残基的定点诱变研究揭示了与这些残基相关的特定功能。尤其是,在活性位点(T217和D320)配位结合的Mg2 +的残基对于酶的功能很重要,但对于形成稳定的六聚体不是必需的。 H1a基序中的保守谷氨酸(E241)可能参与水分子的活化,从而在催化过程中对结合核苷酸的γ-磷酸进行在线攻击。 H3基序中的保守谷氨酰胺(Q362)充当γ-磷酸盐传感器,并介导核苷酸和DNA结合位点的构象偶联。此位置上残基的性质对于由DaseB介导的酶的激活也很重要,这表明该酶使用相同的构象偶联途径来诱导其对DnaB活性的刺激作用。这些突变一起揭示了单体和六聚解旋酶活性位点中许多生化活性方面的保守性。

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