Department of Chemistry, Scripps Florida, 130 Scripps Way, Jupiter, FL 33458, USA.
ACS Chem Biol. 2012 Dec 21;7(12):1984-93. doi: 10.1021/cb3001606. Epub 2012 Nov 7.
Myotonic dystrophy type 1 (DM1) is caused when an expanded r(CUG) repeat (r(CUG)(exp)) binds the RNA splicing regulator muscleblind-like 1 protein (MBNL1) as well as other proteins. Previously, we reported that modularly assembled small molecules displaying a 6'-N-5-hexynoate kanamycin A RNA-binding module (K) on a peptoid backbone potently inhibit the binding of MBNL1 to r(CUG)(exp). However, these parent compounds are not appreciably active in cell-based models of DM1. The lack of potency was traced to suboptimal cellular permeability and localization. To improve these properties, second-generation compounds that are conjugated to a d-Arg(9) molecular transporter were synthesized. These modified compounds enter cells in higher concentrations than the parent compounds and are efficacious in cell-based DM1 model systems at low micromolar concentrations. In particular, they improve three defects that are the hallmarks of DM1: a translational defect due to nuclear retention of transcripts containing r(CUG)(exp); pre-mRNA splicing defects due to inactivation of MBNL1; and the formation of nuclear foci. The best compound in cell-based studies was tested in a mouse model of DM1. Modest improvement of pre-mRNA splicing defects was observed. These studies suggest that a modular assembly approach can afford bioactive compounds that target RNA.
肌强直性营养不良 1 型(DM1)是由扩展的 r(CUG)重复序列(r(CUG)(exp))与 RNA 剪接调节蛋白肌肉盲样蛋白 1(MBNL1)以及其他蛋白结合引起的。先前,我们报道了具有肽聚糖骨架上的 6'-N-5-己炔酸卡那霉素 A RNA 结合模块(K)的模块化组装小分子强烈抑制 MBNL1 与 r(CUG)(exp)的结合。然而,这些母体化合物在 DM1 的基于细胞的模型中没有明显的活性。缺乏效力可归因于细胞通透性和定位不佳。为了改善这些特性,合成了与 d-Arg(9)分子转运体缀合的第二代化合物。这些修饰的化合物以比母体化合物更高的浓度进入细胞,并且在低微摩尔浓度的基于细胞的 DM1 模型系统中有效。特别是,它们改善了 DM1 的三个特征缺陷:由于包含 r(CUG)(exp)的转录物的核保留导致的翻译缺陷;由于 MBNL1 失活导致的前体 mRNA 剪接缺陷;以及核焦点的形成。在基于细胞的研究中,对最佳化合物在 DM1 小鼠模型中进行了测试。观察到前体 mRNA 剪接缺陷的适度改善。这些研究表明,模块化组装方法可以提供针对 RNA 的生物活性化合物。
