Yu Ying-Chun, Sohma Yoshiro, Hwang Tzyh-Chang
Dalton Cardiovascular Research Center, University of Missouri-Columbia, MO, 65211, USA.
Department of Medical Pharmacology and Physiology, University of Missouri-Columbia, MO, 65211, USA.
J Physiol. 2016 Jun 15;594(12):3227-44. doi: 10.1113/JP271723. Epub 2016 Mar 23.
Two functional abnormalities of cystic fibrosis transmembrane conductance regulator (CFTR), a 25% reduction of the single-channel conductance (g) and a ∼13-fold lower open probability (Po ), were found with the R117H mutation that is associated with mild forms of cystic fibrosis. Characterizations of the gating defects of R117H-CFTR led to the conclusion that the mutation decreases Po by perturbing the gating conformational changes in CFTR's transmembrane domains (TMDs) without altering the function of the nucleotide binding domains (NBDs). Nonetheless, gating of the R117H-CFTR can be improved by a variety of pharmacological reagents supposedly acting on NBDs such as ATP analogues, or TMDs (e.g. VX-770 or nitrate). These reagents potentiate synergistically R117H-CFTR gating to a level that allows accurate assessments of its gating deficits. Our studies not only elucidate the mechanism underpinning gating dysfunction of R117H-CFTR, but also provide a mechanistic understanding of how VX-770 ameliorates the gating defects in the R117H mutant.
Cystic fibrosis (CF) is caused by loss-of-function mutations of the cystic fibrosis transmembrane conductance regulator (CFTR) gene encoding a phosphorylation-activated, but ATP-gated chloride channel. In the current study, we investigated the mechanism responsible for the gating defects manifested in R117H-CFTR, an arginine-to-histidine substitution at position 117 of CFTR that is associated with mild forms of CF. We confirmed previous findings of a 25% decrease of the single-channel conductance (g) in R117H-CFTR, but found a ∼13-fold lower open probability (Po ). This dramatic gating deficit is not due to dysfunctional nucleotide binding domains (NBDs) as the mutation does not alter the apparent affinity for ATP, and the mutant channels respond to ATP analogues in a similar manner as wild-type CFTR. Furthermore, once ATP hydrolysis is abolished, the R117H mutant can be trapped in a prolonged 'burst opening' conformation that is proposed to be equipped with a stable NBD dimer. On the other hand, our results support the conclusion that the R117H mutation decreases Po by perturbing the gating conformational changes in CFTR's transmembrane domains as even when NBDs are kept at a dimerized configuration, Po is reduced by ∼10-fold. Moreover, our data demonstrate that a synergistic improvement of R117H-CFTR function can be accomplished with a combined regiment of VX-770 (Ivacaftor), nitrate ion (NO3 (-) ) and N(6) -(2-phenylethyl)-2'-deoxy-ATP (d-PATP), which almost completely rectifies the gating defect of R117H-CFTR. Clinical implications of our results are discussed.
在与轻度囊性纤维化相关的R117H突变中,发现囊性纤维化跨膜传导调节因子(CFTR)存在两种功能异常,即单通道电导(g)降低25%,开放概率(Po)降低约13倍。对R117H-CFTR门控缺陷的表征得出结论,该突变通过干扰CFTR跨膜结构域(TMDs)中的门控构象变化来降低Po,而不改变核苷酸结合结构域(NBDs)的功能。尽管如此,R117H-CFTR的门控可通过多种推测作用于NBDs的药理试剂(如ATP类似物)或TMDs(如VX-770或硝酸盐)得到改善。这些试剂协同增强R117H-CFTR门控,使其达到能够准确评估其门控缺陷的水平。我们的研究不仅阐明了R117H-CFTR门控功能障碍的机制,还提供了关于VX-770如何改善R117H突变体门控缺陷的机制性理解。
囊性纤维化(CF)由编码磷酸化激活但ATP门控氯离子通道的囊性纤维化跨膜传导调节因子(CFTR)基因突变导致功能丧失引起。在本研究中,我们调查了R117H-CFTR(CFTR第117位精氨酸被组氨酸取代,与轻度CF相关)中表现出门控缺陷的机制。我们证实了之前关于R117H-CFTR单通道电导(g)降低25%的发现,但发现开放概率(Po)降低约13倍。这种显著的门控缺陷并非由于核苷酸结合结构域(NBDs)功能失调,因为该突变不会改变对ATP的表观亲和力,且突变通道对ATP类似物的反应与野生型CFTR相似。此外,一旦ATP水解被消除,R117H突变体可被困在延长的“爆发开放”构象中,该构象被认为具有稳定的NBD二聚体。另一方面,我们的结果支持以下结论:R117H突变通过干扰CFTR跨膜结构域中的门控构象变化来降低Po,因为即使NBDs保持二聚化构型,Po仍降低约10倍。此外,我们的数据表明,联合使用VX-770(依伐卡托)、硝酸根离子(NO3 (-) )和N(6) -(2-苯乙基)-2'-脱氧-ATP(d-PATP)可协同改善R117H-CFTR功能,几乎完全纠正R117H-CFTR的门控缺陷。我们讨论了研究结果的临床意义。
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