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首页> 外文期刊>Analytical Biochemistry: An International Journal of Analytical and Preparative Methods >A fluorescence-based assay for the apurinic/apyrimidinic-site cleavage activity of human tyrosyl-DNA phosphodiesterase 1
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A fluorescence-based assay for the apurinic/apyrimidinic-site cleavage activity of human tyrosyl-DNA phosphodiesterase 1

机译:基于荧光的人酪氨酰-DNA磷酸二酯酶1的嘌呤/嘧啶位点裂解活性测定

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摘要

Tyrosyl-DNA phosphodiesterase 1 (Tdp1) catalyzes the hydrolysis of phosphodiester bonds between the DNA 30-phosphate and tyrosine residues and plays a major role in the repair of stalled topoisomerase IDNA covalent complexes. Given this role, Tdp1 is of interest as a potential target for anticancer therapy. Inhibiting Tdp1 in combination with clinically used Top1 inhibitors may potentiate the effects of the latter and help to overcome some of the chemoresistance issues currently observed. In addition, Tdp1 can function during DNA repair to remove a variety of other 30 adducts from DNA such as phosphoglycolates and abasic or apurinic/apyrimidinic (AP) sites. Here we describe a new mix-and-read homogeneous fluorogenic assay for the measurement of the AP-site cleavage activity of Tdp1 that is compatible with highthroughput screening. The application of such an assay will open up further avenues for the discovery of novel Tdp1 inhibitors.
机译:酪氨酰-DNA磷酸二酯酶1(Tdp1)催化DNA 30-磷酸和酪氨酸残基之间的磷酸二酯键的水解,并在修复停滞的拓扑异构酶IDNA共价复合物中起主要作用。鉴于此作用,Tdp1作为抗癌治疗的潜在靶标受到关注。与临床使用的Top1抑制剂组合使用抑制Tdp1可以增强后者的作用,并有助于克服目前观察到的一些化学耐药性问题。此外,Tdp1可以在DNA修复过程中发挥作用,以从DNA中去除其他30种加合物,例如磷酸乙醇酸和无碱基或嘌呤/嘧啶(AP)位点。在这里,我们描述了一种与高通量筛选兼容的,用于测量Tdp1的AP位点裂解活性的新型混合读取均质荧光检测方法。这种测定法的应用将为发现新型Tdp1抑制剂开辟更多的途径。

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