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核苷酸与三聚钽(III)-二锌(II)配合物的相互作用:单磷酸鸟苷对铽发光的高效敏化及其在实时监测磷酸二酯酶活性中的应用。

Interaction of Nucleotides with a Trinuclear Terbium(III)-Dizinc(II) Complex: Efficient Sensitization of Terbium Luminescence by Guanosine Monophosphate and Application to Real-Time Monitoring of Phosphodiesterase Activity.

机构信息

School of Chemistry , Monash University , Clayton , Victoria 3800 , Australia.

Department of Chemistry , Durham University , Durham DH1 3LE , U.K.

出版信息

Inorg Chem. 2019 Jan 7;58(1):495-505. doi: 10.1021/acs.inorgchem.8b02731. Epub 2018 Dec 18.

Abstract

An in-depth study of the interaction of a trinuclear terbium(III)-dizinc(II) complex with an array of nucleotides differing in the type of nucleobase and number of phosphate groups, as well as cyclic versus acyclic variants, is presented. The study examined the nature of the interaction and the efficiency at which guanine was able to sensitize terbium(III) luminescence. Competitive binding and titration studies were performed to help establish the nature/mode of the interactions. These established that (1) interaction occurs by the coordination of phosphate groups to zinc(II) (in addition to uridine in the case of uridine monophosphate), (2) acyclic nucleotides bind more strongly than cyclic counterparts because of their higher negative charge, (3) guanine-containing nucleotides are able to sensitize terbium(III) luminescence with the efficiency of sensitization following the order guanosine monophosphate (GMP) > guanosine diphosphate > guanosine triphosphate because of the mode of binding, and (4) nucleoside monophosphates bind to a single zinc(II) ion, whereas di- and triphosphates appear to bind in a bridging mode between two host molecules. Furthermore, it has been shown that guanine is a sensitizer of terbium(III) luminescence. On the basis of the ability of GMP to effectively sensitize terbium(III)-based luminescence while cyclic GMP (cGMP) does not, the complex has been utilized to monitor the catalytic conversion of cGMP to GMP by a phosphodiesterase enzyme in real time using time-gated luminescence on a benchtop fluorimeter. The complex has the potential to find broad application in monitoring the activity of enzymes that process nucleotides (co)substrates, including high-throughput drug-screening programs.

摘要

本文深入研究了三核铽(III)-二锌(II)配合物与一系列核苷酸的相互作用,这些核苷酸在碱基类型和磷酸基团数量上存在差异,以及环状和非环状变体。研究考察了相互作用的性质以及鸟嘌呤敏化铽(III)发光的效率。进行了竞争性结合和滴定研究,以帮助确定相互作用的性质/模式。这些研究结果表明:(1)通过磷酸基团与锌(II)配位发生相互作用(在尿苷单磷酸盐的情况下还有尿苷);(2)由于其更高的负电荷,非环状核苷酸的结合能力更强;(3)由于结合模式,含有鸟嘌呤的核苷酸能够敏化铽(III)的发光,敏化效率依次为鸟苷一磷酸(GMP)>鸟苷二磷酸>鸟苷三磷酸;(4)核苷单磷酸与单个锌(II)离子结合,而二磷酸和三磷酸似乎以桥联模式结合在两个主体分子之间。此外,已经表明鸟嘌呤是铽(III)发光的敏化剂。基于 GMP 有效敏化铽(III)发光而环状 GMP(cGMP)不能的能力,该配合物已被用于使用台式荧光计上的时间门控发光实时监测磷酸二酯酶酶对 cGMP 到 GMP 的催化转化。该配合物具有在监测处理核苷酸(共)底物的酶的活性方面找到广泛应用的潜力,包括高通量药物筛选计划。

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