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基于 FRET 的荧光探针筛选抗癌药物,抑制 p73 与 MDM2 的结合。

A FRET-Based Fluorescent Probe to Screen Anticancer Drugs, Inhibiting p73 Binding to MDM2.

机构信息

School of Pharmacy, Sungkyunkwan University, Suwon, 16419 (Republic of, Korea.

出版信息

Chembiochem. 2021 Mar 2;22(5):830-833. doi: 10.1002/cbic.202000660. Epub 2020 Nov 20.

Abstract

The protein p73 acts as a transcription factor, resulting in tumour suppression. MDM2, an oncogenic protein, can negatively influence p73-mediated apoptosis by binding to p73 transactivation domains (TAD). Inhibition of the protein-protein interaction between p73 and oncogenic proteins is an attractive strategy for promoting p73-mediated apoptosis. Herein, we describe the use of a modified p73-TAD peptide for the FRET-based assay of the binding of p73-TAD to MDM2. The FRET probe, equipped with 1-naphthylamine (λ =330 nm, λ =445 nm), serves as a FRET acceptor, and the tryptophan of the protein acts as FRET donor (λ =280 nm, λ =340 nm). Sensitized emission from the FRET probe was observed upon excitation of the protein-FRET-probe complex at the excitation wavelength of Trp. Furthermore, addition of the MDM2 inhibitor Nutiln-3 drastically reduced the FRET signal, thus indicating that the FRET probe competes with Nutiln-3 for MDM2 binding. The developed FRET binding assay might be applicable in high-throughput screening of novel drugs that inhibit interactions between p73 and MDM2.

摘要

p73 蛋白作为转录因子发挥作用,从而抑制肿瘤。癌蛋白 MDM2 可以通过与 p73 反式激活结构域(TAD)结合,对 p73 介导的细胞凋亡产生负向影响。抑制 p73 与致癌蛋白之间的蛋白-蛋白相互作用是促进 p73 介导的细胞凋亡的一种有吸引力的策略。在此,我们描述了使用修饰的 p73-TAD 肽进行 FRET 基础测定,以测定 p73-TAD 与 MDM2 的结合。FRET 探针带有 1-萘胺(λ =330nm,λ =445nm),作为 FRET 受体,蛋白质的色氨酸作为 FRET 供体(λ =280nm,λ =340nm)。在 Trp 的激发波长下激发蛋白质-FRET-探针复合物时,可以观察到 FRET 探针的敏化发射。此外,加入 MDM2 抑制剂 Nutiln-3 会大大降低 FRET 信号,表明 FRET 探针与 Nutiln-3 竞争与 MDM2 的结合。开发的 FRET 结合测定法可能适用于抑制 p73 和 MDM2 之间相互作用的新型药物的高通量筛选。

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