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Characterization of an ATP-dependent DNA ligase from the acidophilic archaeon “Ferroplasma acidarmanus” Fer1

机译:嗜酸性古细菌“费拉酸杆菌” Fer1的ATP依赖性DNA连接酶的表征

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Analysis of the genome of “Ferroplasma acidarmanus” Fer1, an archaeon that is an extreme acidophile, identified an open reading frame encoding a putative ATP-dependent DNA ligase, which we termed FaLig. The deduced amino acid sequence of FaLig contains 595 amino acids, with a predicted molecular mass of 67.8 kDa. “F. acidarmanus” Fer1 is classified as a Euryarchaeote, but phylogenetic analysis using amino acid sequences showed that FaLig is more similar to DNA ligases from Crenarchaeota, suggesting that lateral transfer of these genes has occurred among archaea. The gene sequence encoding FaLig was cloned into a bacterial expression vector harbouring an upstream His-tag to aid purification. Conditions for expression and purification from Escherichia coli were identified and recombinant FaLig was confirmed to be an ATP-dependent DNA ligase. Optimal conditions for nick-joining by the protein were pH 6–7, 0.5 mM ATP, in the presence of either Mg2+ or Mn2+. Using a range of nicked, double-stranded nucleic acids, ligation was detected with the same substrates as previously determined for other DNA ligases. Although FaLig is the DNA ligase from one of the most extreme acidophilic organism yet studied, this characterization suggests that its biochemical mechanism is analogous to that of enzymes from other cellular systems.
机译:对极端嗜酸菌古细菌“ Ferroplasma acidarmanus” Fer1的基因组进行分析,确定了一个开放阅读框,该框架编码一个假定的依赖于ATP的DNA连接酶,我们将其称为FaLig。 FaLig推导的氨基酸序列包含595个氨基酸,预测分子量为67.8 kDa。 “F。 Fer1被归类为Euryarchaeote,但是根据氨基酸序列进行的系统发育分析表明,FaLig与Crenarchaeota的DNA连接酶更为相似,这表明这些基因在古细菌之间发生了横向转移。将编码FaLig的基因序列克隆到带有上游His-tag的细菌表达载体中,以帮助纯化。鉴定了从大肠杆菌表达和纯化的条件,并确认重组FaLig是ATP依赖的DNA连接酶。在存在Mg2 + 或Mn2 + 的情况下,蛋白进行缺口连接的最佳条件是pH 6–7、0.5 mM ATP。使用一系列带切口的双链核酸,使用与先前确定的其他DNA连接酶相同的底物检测连接。尽管FaLig是迄今为止研究过的最极端的嗜酸生物之一的DNA连接酶,但此特征表明其生化机制与其他细胞系统的酶类似。

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