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A real-time fluorescence method for enzymatic characterization of specialized human DNA polymerases

机译:一种实时荧光方法,用于酶促表征特殊的人类DNA聚合酶

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Specialized DNA polymerases are involved in DNA synthesis during base-excision repair and translesion synthesis across a wide range of chemically modified DNA templates. Notable features of these enzymes include low catalytic efficiency, low processivity and low fidelity. Traditionally, in vitro studies of these enzymes have utilized radiolabeled substrates and gel electrophoretic separation of products. We have developed a simple homogeneous fluorescence-based method to study the enzymology of specialized DNA polymerases in real time. The method is based on fluorescent reporter strand displacement from a tripartite substrate containing a quencher-labeled template strand, an unlabeled primer and a fluorophore-labeled reporter. With this method, we could follow the activity of human DNA polymerases β, η, ι and κ under different reaction conditions, and we investigated incorporation of the aberrant nucleotide, 8-oxodGTP, as well as bypass of an abasic site or 8-oxoG DNA template lesion in different configurations. Lastly, we demonstrate that the method can be used for small molecule inhibitor discovery and characterization in highly miniaturized settings, and we report the first nanomolar inhibitors of Y-family DNA polymerases ι and η. The fluorogenic method presented here should facilitate mechanistic and inhibitor investigations of these polymerases and is also applicable to the study of highly processive replicative polymerases.
机译:在广泛的化学修饰的DNA模板的碱基切除修复和跨病变合成过程中,专门的DNA聚合酶参与DNA合成。这些酶的显着特征包括低催化效率,低合成能力和低保真度。传统上,这些酶的体外研究利用放射性标记的底物和产物的凝胶电泳分离。我们已经开发了一种简单的基于均相荧光的方法来实时研究专用DNA聚合酶的酶学。该方法基于荧光报告子链从包含淬灭剂标记的模板链,未标记的引物和荧光团标记的报告子的三重底物上的位移。通过这种方法,我们可以在不同的反应条件下跟踪人类DNA聚合酶β,η,ι和κ的活性,并研究了异常核苷酸8-oxodGTP的掺入以及无碱基位点或8-oxoG的旁路DNA模板病变的结构不同。最后,我们证明了该方法可用于在高度小型化的环境中发现和表征小分子抑制剂,并且我们报道了Y家族DNA聚合酶η和η的首批纳摩尔抑制剂。本文介绍的荧光方法应有助于对这些聚合酶进行机理和抑制剂研究,也可用于研究高生产力复制性聚合酶。

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