Allosteric folding correction of F508del and rare CFTR mutants by elexacaftor-tezacaftor-ivacaftor (Trikafta) combination
Guido Veit, Ariel Roldan, Mark A. Hancock, Dillon F. Da Fonte, Haijin Xu, Maytham Hussein, Saul Frenkiel, Elias Matouk, Tony Velkov, Gergely L. Lukacs
Guido Veit, Ariel Roldan, Mark A. Hancock, Dillon F. Da Fonte, Haijin Xu, Maytham Hussein, Saul Frenkiel, Elias Matouk, Tony Velkov, Gergely L. Lukacs
View: Text | PDF
Research Article Cell biology Pulmonology

Allosteric folding correction of F508del and rare CFTR mutants by elexacaftor-tezacaftor-ivacaftor (Trikafta) combination

Abstract

Based on its clinical benefits, Trikafta — the combination of folding correctors VX-661 (tezacaftor), VX-445 (elexacaftor), and the gating potentiator VX-770 (ivacaftor) — was FDA approved for treatment of patients with cystic fibrosis (CF) carrying deletion of phenylalanine at position 508 (F508del) of the CF transmembrane conductance regulator (CFTR) on at least 1 allele. Neither the mechanism of action of VX-445 nor the susceptibility of rare CF folding mutants to Trikafta are known. Here, we show that, in human bronchial epithelial cells, VX-445 synergistically restores F508del-CFTR processing in combination with type I or II correctors that target the nucleotide binding domain 1 (NBD1) membrane spanning domains (MSDs) interface and NBD2, respectively, consistent with a type III corrector mechanism. This inference was supported by the VX-445 binding to and unfolding suppression of the isolated F508del-NBD1 of CFTR. The VX-661 plus VX-445 treatment restored F508del-CFTR chloride channel function in the presence of VX-770 to approximately 62% of WT CFTR in homozygous nasal epithelia. Substantial rescue of rare misprocessing mutations (S13F, R31C, G85E, E92K, V520F, M1101K, and N1303K), confined to MSD1, MSD2, NBD1, and NBD2 of CFTR, was also observed in airway epithelia, suggesting an allosteric correction mechanism and the possible application of Trikafta for patients with rare misfolding mutants of CFTR.

Authors

Guido Veit, Ariel Roldan, Mark A. Hancock, Dillon F. Da Fonte, Haijin Xu, Maytham Hussein, Saul Frenkiel, Elias Matouk, Tony Velkov, Gergely L. Lukacs

×

Figure 3

Trikafta mediated correction of CFTRF508del/F508del in HNE.

Options: View larger image (or click on image) Download as PowerPoint
Trikafta mediated correction of CFTRF508del/F508del in HNE. (A) Effect o...
(A) Effect of indicated single correctors or corrector combinations on the Isc of human nasal epithelia with CFTRF508del/F508del genotype (CF-HNE). CFTR-mediated currents were induced by sequential acute addition of forskolin (Fsk, 20 μM, arrow) and VX-770 (770, 10 μM, filled arrowhead), followed by CFTR inhibition with CFTRinh-172 (Inh-172, 20 μM, open arrowhead) in intact monolayers with basolateral-to-apical chloride gradient. (B) Quantification of the CFTRinh-172 inhibited current, after stimulation as in A, in CF-HNE isolated from 5 different homozygous F508del CF patients after single correctors (VX-809 and VX-661, 3 μM; VX-445, 2 μM; 24 hours, 37°C), corrector plus chronic potentiator (cVX-770, 1 μM, 24 hours, 37°C) or corrector combination treatment expressed as percentage of WT-CFTR currents in WT-HNE from 10 donors. **P < 0.01 by paired 2-tailed Student’s t test. (C) The fraction of potentiator-independent (forskolin-induced) current in HNE treated with single corrector or corrector combination. **P < 0.01 by paired 2-tailed Student’s t test followed by Bonferroni’s FDR correction.