低游离药物浓度可防止增强剂VX-770(依伐卡托)对F508del囊性纤维化跨膜传导调节因子功能表达的抑制作用。
Low free drug concentration prevents inhibition of F508del CFTR functional expression by the potentiator VX-770 (ivacaftor).
作者信息
Matthes Elizabeth, Goepp Julie, Carlile Graeme W, Luo Yishan, Dejgaard Kurt, Billet Arnaud, Robert Renaud, Thomas David Y, Hanrahan John W
机构信息
Department of Physiology, McGill University, Montréal, QC, Canada.
CF Translational Research Centre, McGill University, Montréal, QC, Canada.
出版信息
Br J Pharmacol. 2016 Feb;173(3):459-70. doi: 10.1111/bph.13365. Epub 2016 Jan 13.
BACKGROUND AND PURPOSE
The most common cystic fibrosis (CF) mutation F508del inhibits the gating and surface expression of CFTR, a plasma membrane anion channel. Optimal pharmacotherapies will probably require both a 'potentiator' to increase channel open probability and a 'corrector' that improves folding and trafficking of the mutant protein and its stability at the cell surface. Interaction between CF drugs has been reported but remains poorly understood.
EXPERIMENTAL APPROACH
CF bronchial epithelial cells were exposed to the corrector VX-809 (lumacaftor) and potentiator VX-770 (ivacaftor) individually or in combination. Functional expression of CFTR was assayed as the forskolin-stimulated short-circuit current (Isc ) across airway epithelial monolayers expressing F508del CFTR.
KEY RESULTS
The potentiated Isc response during forskolin stimulation was increased sixfold after pretreatment with VX-809 alone and reached ~11% that measured across non-CF monolayers. VX-770 (100 nM) and genistein (50 μM) caused similar levels of potentiation, which were not additive and were abolished by the CFTR inhibitor CFTRinh -172. The unbound fraction of VX-770 in plasma was 0.13 ± 0.04%, which together with previous measurements in patients given 250 mg p.o. twice daily, suggests a peak free plasma concentration of 1.5-8.5 nM. Chronic exposure to high VX-770 concentrations (>1 μM) inhibited functional correction by VX-809 but not in the presence of physiological protein levels (20-40 mg·mL(-1) ). Chronic exposure to a low concentration of VX-770 (100 nM) together with VX-809 (1 μM) also did not reduce the forskolin-stimulated Isc , relative to cells chronically exposed to VX-809 alone, provided it was assayed acutely using the same, clinically relevant concentration of potentiator.
CONCLUSIONS AND IMPLICATIONS
Chronic exposure to clinically relevant concentrations of VX-770 did not reduce F508del CFTR function. Therapeutic benefit of VX-770 + VX-809 (Orkambi) is probably limited by the efficacy of VX-809 rather than by inhibition by VX-770.
背景与目的
最常见的囊性纤维化(CF)突变F508del会抑制CFTR(一种质膜阴离子通道)的门控和表面表达。最佳药物治疗可能既需要一种“增强剂”来增加通道开放概率,又需要一种“校正剂”来改善突变蛋白的折叠、转运及其在细胞表面的稳定性。已报道CF药物之间存在相互作用,但仍了解甚少。
实验方法
将CF支气管上皮细胞单独或联合暴露于校正剂VX - 809(鲁马卡托)和增强剂VX - 770(依伐卡托)。CFTR的功能表达通过测定佛司可林刺激的跨表达F508del CFTR的气道上皮单层的短路电流(Isc)来评估。
主要结果
单独用VX - 809预处理后,佛司可林刺激期间增强的Isc反应增加了6倍,达到非CF单层测定值的约11%。VX - 770(100 nM)和染料木黄酮(50 μM)引起相似程度的增强,二者无相加作用,且被CFTR抑制剂CFTRinh - 172消除。VX - 770在血浆中的未结合分数为0.13±0.04%,结合之前对每日口服250 mg两次的患者的测量结果,提示游离血浆峰值浓度为1.5 - 8.5 nM。长期暴露于高浓度的VX - 770(>1 μM)会抑制VX - 809的功能校正,但在生理蛋白水平(20 - 40 mg·mL⁻¹)存在时则不会。相对于仅长期暴露于VX - 809的细胞,长期暴露于低浓度的VX - 770(100 nM)与VX - 809(1 μM)一起也不会降低佛司可林刺激的Isc,前提是使用相同的临床相关浓度的增强剂进行急性测定。
结论与启示
长期暴露于临床相关浓度的VX - 770不会降低F508del CFTR功能。VX - 770 + VX - 809(奥卡姆比)的治疗益处可能受VX - 809的疗效限制,而非受VX - 770的抑制作用限制。
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