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三磷酸腺苷连接嵌合核苷酸作为脱氧尿嘧啶三磷酸酶的特异性发光报告物。

ATP-Linked Chimeric Nucleotide as a Specific Luminescence Reporter of Deoxyuridine Triphosphatase.

机构信息

Department of Chemistry , Stanford University , Stanford , California 94305 , United States.

出版信息

Bioconjug Chem. 2018 May 16;29(5):1614-1621. doi: 10.1021/acs.bioconjchem.8b00124. Epub 2018 Mar 29.

Abstract

Nucleotide surveillance enzymes play important roles in human health, by monitoring damaged monomers in the nucleotide pool and deactivating them before they are incorporated into chromosomal DNA or disrupt nucleotide metabolism. In particular, deamination of cytosine, leading to uracil in DNA and in the nucleotide pool, can be deleterious, causing DNA damage. The enzyme deoxyuridine triphosphatase (dUTPase) is currently under study as a therapeutic and prognostic target for cancer. Measuring the activity of this enzyme is important both in basic research and in clinical applications involving this pathway, but current methods are nonselective, detecting pyrophosphate, which is produced by many enzymes. Here we describe the design and synthesis of a dUTPase enzyme-specific chimeric dinucleotide (DUAL) that replaces the pyrophosphate leaving group of the native substrate with ATP, enabling sensitive detection via luciferase luminescence signaling. The DUAL probe functions sensitively and selectively to quantify enzyme activities in vitro and in cell lysates. We further report the first measurements of dUTPase activities in eight different cell lines, which are found to vary by a factor of 7-fold. We expect that the new probe can be of considerable utility in research involving this clinically significant enzyme.

摘要

核苷酸监测酶在人类健康中起着重要作用,通过监测核苷酸池中的受损单体,并在它们被掺入染色体 DNA 或破坏核苷酸代谢之前使其失活。特别是,胞嘧啶的脱氨基作用会导致 DNA 和核苷酸池中的尿嘧啶,这可能是有害的,会导致 DNA 损伤。脱氧尿苷三磷酸酶 (dUTPase) 目前正在作为癌症的治疗和预后靶点进行研究。测量该酶的活性在基础研究和涉及该途径的临床应用中都很重要,但目前的方法是非选择性的,会检测到许多酶产生的焦磷酸。在这里,我们描述了一种 dUTPase 酶特异性嵌合二核苷酸 (DUAL) 的设计和合成,它用 ATP 取代了天然底物的焦磷酸离去基团,通过荧光素发光信号实现了灵敏检测。DUAL 探针在体外和细胞裂解物中灵敏且选择性地定量酶活性。我们进一步报告了在八种不同细胞系中首次测量 dUTPase 活性的结果,发现它们的活性差异可达 7 倍。我们预计,新探针在涉及这种具有临床意义的酶的研究中具有相当大的实用性。

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本文引用的文献

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