人类端粒 G-四链体 DNA 结合药物的测定法。
An assay for human telomeric G-quadruplex DNA binding drugs.
机构信息
NUBAD LLC, 900 B West Faris Road, Greenville, SC 29630, United States.
出版信息
Bioorg Med Chem Lett. 2013 Dec 15;23(24):6695-9. doi: 10.1016/j.bmcl.2013.10.030. Epub 2013 Nov 1.
Abstract
Compounds that stabilize the G-quadruplexes formed by human telomeres can inhibit the telomerase activity and are potential cancer therapies. We have developed an assay for the screening of compounds with high affinity for human telomeric G-quadruplexes (HTG). The assay uses a thiazole orange fluorescent reporter molecule conjugated to the aminoglycoside, neomycin, as a probe in a fluorescence displacement assay. The conjugation of the planar base stacking thiazole orange with the groove binding neomycin results in high affinity probe that can determine the relative binding affinity of high affinity HTG binding drugs in a high throughput format. The robust assay is applicable for the determination of the binding affinity of HTG in the presence of K(+) or Na(+).
摘要
能够稳定人端粒形成的 G-四链体的化合物可以抑制端粒酶活性,是有潜力的癌症治疗方法。我们开发了一种用于筛选与人端粒 G-四链体(HTG)具有高亲和力的化合物的测定法。该测定法使用噻唑橙荧光报告分子与氨基糖苷类抗生素新霉素缀合作为荧光置换测定中的探针。平面碱基堆积噻唑橙与沟结合新霉素的缀合导致高亲和力探针,该探针可以以高通量格式确定高亲和力 HTG 结合药物的相对结合亲和力。该稳健的测定法适用于在存在 K(+) 或 Na(+) 的情况下测定 HTG 的结合亲和力。
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