Pedemonte Nicoletta, Sonawane N D, Taddei Alessandro, Hu Jie, Zegarra-Moran Olga, Suen Yat Fan, Robins Lori I, Dicus Christopher W, Willenbring Dan, Nantz Michael H, Kurth Mark J, Galietta Luis J V, Verkman A S
Department of Medicine, University of California, San Francisco, 94143-0521, USA.
Mol Pharmacol. 2005 May;67(5):1797-807. doi: 10.1124/mol.105.010959. Epub 2005 Feb 18.
Mutations in the cystic fibrosis transmembrane conductance regulator (CFTR) chloride channel cause cystic fibrosis. The delta F508 mutation produces defects in channel gating and cellular processing, whereas the G551D mutation produces primarily a gating defect. To identify correctors of gating, 50,000 diverse small molecules were screened at 2.5 microM (with forskolin, 20 microM) by an iodide uptake assay in epithelial cells coexpressing delta F508-CFTR and a fluorescent halide indicator (yellow fluorescent protein-H148Q/I152L) after delta F508-CFTR rescue by 24-h culture at 27 degrees C. Secondary analysis and testing of >1000 structural analogs yielded two novel classes of correctors of defective delta F508-CFTR gating ("potentiators") with nanomolar potency that were active in human delta F508 and G551D cells. The most potent compound of the phenylglycine class, 2-[(2-1H-indol-3-yl-acetyl)-methylamino]-N-(4-isopropylphenyl)-2-phenylacetamide, reversibly activated delta F508-CFTR in the presence of forskolin with K(a) approximately 70 nM and also activated the CFTR gating mutants G551D and G1349D with K(a) values of approximately 1100 and 40 nM, respectively. The most potent sulfonamide, 6-(ethylphenylsulfamoyl)-4-oxo-1,4-dihydroquinoline-3-carboxylic acid cycloheptylamide, had K(a) approximately 20 nM for activation of delta F508-CFTR. In cell-attached patch-clamp experiments, phenylglycine-01 (PG-01) and sulfonamide-01 (SF-01) increased channel open probability >5-fold by the reduction of interburst closed time. An interesting property of these compounds was their ability to act in synergy with cAMP agonists. Microsome metabolism studies and rat pharmacokinetic analysis suggested significantly more rapid metabolism of PG-01 than SF-03. Phenylglycine and sulfonamide compounds may be useful for monotherapy of cystic fibrosis caused by gating mutants and possibly for a subset of delta F508 subjects with significant delta F508-CFTR plasma-membrane expression.
囊性纤维化跨膜传导调节因子(CFTR)氯离子通道的突变会导致囊性纤维化。ΔF508突变在通道门控和细胞加工过程中产生缺陷,而G551D突变主要产生门控缺陷。为了鉴定门控校正剂,在27℃下培养24小时使ΔF508 - CFTR得到挽救后,通过碘摄取试验在共表达ΔF508 - CFTR和荧光卤化物指示剂(黄色荧光蛋白 - H148Q/I152L)的上皮细胞中,以2.5μM(加入20μM福斯可林)的浓度筛选了50,000种不同的小分子。对1000多种结构类似物进行二次分析和测试,得到了两类新型的有缺陷的ΔF508 - CFTR门控校正剂(“增强剂”),其具有纳摩尔效力,在人ΔF508和G551D细胞中具有活性。苯甘氨酸类中最有效的化合物2 - [(2 - 1H - 吲哚 - 3 - 基 - 乙酰基) - 甲基氨基] - N - (4 - 异丙基苯基) - 2 - 苯基乙酰胺,在福斯可林存在下可逆地激活ΔF508 - CFTR,其解离常数(K(a))约为70 nM,还能激活CFTR门控突变体G551D和G1349D,其K(a)值分别约为1100 nM和40 nM。最有效的磺酰胺类化合物6 - (乙基苯基磺酰基) - 4 - 氧代 - 1,4 - 二氢喹啉 - 3 - 羧酸环庚基酰胺激活ΔF508 - CFTR的K(a)约为20 nM。在细胞贴附式膜片钳实验中,苯甘氨酸 - 01(PG - 01)和磺酰胺 - 01(SF - 01)通过减少爆发间期关闭时间使通道开放概率增加了5倍以上。这些化合物的一个有趣特性是它们能够与cAMP激动剂协同作用。微粒体代谢研究和大鼠药代动力学分析表明,PG - 01的代谢比SF - 03明显更快。苯甘氨酸和磺酰胺类化合物可能可用于门控突变体引起的囊性纤维化的单一疗法,并且可能对一部分具有显著ΔF508 - CFTR质膜表达的ΔF508患者有用。
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