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Designer Fluorescent Adenines Enable Real-Time Monitoring of MUTYH Activity

机译:设计师荧光腺嘌呤能够实时监控Mutyh活动

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The human DNA base excision repair enzyme MUTYH (MutY homolog DNA glycosylase) excises undamaged adenine that has been misincorporated opposite the oxidatively damaged 8-oxoG, preventing transversion mutations and serving as an important defense against the deleterious effects of this damage. Mutations in the MUTYH gene predispose patients to MUTYH-associated polyposis and colorectal cancer, and MUTYH expression has been documented as a biomarker for pancreatic cancer. Measuring MUTYH activity is therefore critical for evaluating and diagnosing disease states as well as for testing this enzyme as a potential therapeutic target. However, current methods for measuring MUTYH activity rely on indirect electrophoresis and radioactivity assays, which are difficult to implement in biological and clinical settings. Herein, we synthesize and identify novel fluorescent adenine derivatives that can act as direct substrates for excision by MUTYH as well as bacterial MutY. When incorporated into synthetic DNAs, the resulting fluorescently modified adenine-release turn-on (FMART) probes report on enzymatic base excision activity in real time, both in vitro and in mammalian cells and human blood. We also employ the probes to identify several promising small-molecule modulators of MUTYH by employing FMART probes for in vitro screening.
机译:人DNA碱基切除修复酶mutyh(官Homolog DNA糖基糖酶)促使未造成的腺嘌呤在氧化损伤的8氧氧化物相对,防止横转化突变并作为对这种损害的有害影响的重要防御。 MutyH基因中的突变使患者达到umyh相关的息肉病和结肠直肠癌,并且具有蛋白表达被记录为胰腺癌的生物标志物。因此,测量MutyH活性对于评估和诊断疾病状态以及将该酶作为潜在的治疗目标进行测试至关重要。然而,目前测量mutyh活性的方法依赖于间接电泳和放射性测定,这难以在生物和临床环境中实施。在此,我们合成并鉴定新型荧光腺嘌呤衍生物,其可以通过mutyh和细菌突变作为直接底物。当掺入合成DNA中时,得到的荧光改性的腺嘌呤释放匝(FMART)探针在实时在体外和哺乳动物细胞和人血中实时存在酶促基本切除活性的报告。我们还采用探针通过使用用于体外筛选的FMART探针来识别MutyH的几个有前途的小分子调节剂。

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