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使用与生物素化DNA结构结合的链霉亲和素作为模型底物,用于分析解旋酶对核蛋白复合物的破坏作用。

Use of streptavidin bound to biotinylated DNA structures as model substrates for analysis of nucleoprotein complex disruption by helicases.

作者信息

Brüning Jan-Gert, Howard Jamieson A L, McGlynn Peter

机构信息

Department of Biology, University of York, Wentworth Way, York, YO10 5DD, United Kingdom.

Department of Biology, University of York, Wentworth Way, York, YO10 5DD, United Kingdom.

出版信息

Methods. 2016 Oct 1;108:48-55. doi: 10.1016/j.ymeth.2016.03.017. Epub 2016 Mar 24.

Abstract

Helicases are a subfamily of translocases that couple the directional translocation along a nucleic acid lattice to the separation of nucleic acid duplexes using the energy derived from nucleoside triphosphate hydrolysis. These enzymes perform essential functions in all aspects of nucleic acid metabolism by unwinding and remodelling DNA or RNA in DNA replication, repair, recombination, transcription and translation. Most classical biochemical studies assay the ability of these enzymes to separate naked nucleic acids. However, many different types of proteins form non-covalent interactions with nucleic acids in vivo and so the true substrates of helicases are protein-nucleic acid complexes rather than naked DNA and RNA. Studies over the last decade have revealed that bound proteins can have substantial inhibitory effects on the ability of helicases to unwind nucleic acids. Any analysis of helicase mechanisms in vitro must therefore consider helicase function within the context of nucleoprotein substrates rather than just DNA or RNA. Here we discuss how to analyse the impact of bound proteins on the ability of helicases to unwind DNA substrates in vitro.

摘要

解旋酶是转位酶的一个亚家族,它们利用核苷三磷酸水解产生的能量,将沿着核酸晶格的定向转位与核酸双链的分离耦合起来。这些酶通过在DNA复制、修复、重组、转录和翻译过程中解开和重塑DNA或RNA,在核酸代谢的各个方面发挥着重要作用。大多数经典的生化研究分析这些酶分离裸露核酸的能力。然而,许多不同类型的蛋白质在体内与核酸形成非共价相互作用,因此解旋酶的真正底物是蛋白质-核酸复合物,而不是裸露的DNA和RNA。过去十年的研究表明,结合的蛋白质对解旋酶解开核酸的能力可能有显著的抑制作用。因此,任何体外解旋酶机制的分析都必须在核蛋白底物的背景下考虑解旋酶的功能,而不仅仅是DNA或RNA。在这里,我们讨论如何分析结合的蛋白质对解旋酶在体外解开DNA底物能力的影响。

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