Rescue of NBD2 Mutants N1303K and S1235R of CFTR by Small-Molecule Correctors and Transcomplementation

Rapino, Daniele; Sabirzhanova, Inna; Lopes‐Pacheco, Miquéias; Grover, Rahul; Guggino, William B.; Cebotaru, Liudmila

doi:10.1371/journal.pone.0119796

Cited by 41 publications

(55 citation statements)

References 49 publications

(63 reference statements)

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“…An increasing number of correctors have been evaluated for their ability to rescue CFTR bearing ΔF508, as well as other NBD mutations [18, 23, 24]. The impact of these small-molecules to restoring CFTR processing and trafficking in cells bearing the mutants G85E, E92K, L1077P, and M1101K has notyet been established.…”

Section: Resultsmentioning

confidence: 99%

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Combination of Correctors Rescues CFTR Transmembrane-Domain Mutants by Mitigating their Interactions with Proteostasis

Lopes‐Pacheco¹,

Boinot²,

Sabirzhanova³

et al. 2017

Cell Physiol Biochem

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Background/Aims: Premature degradation of mutated cystic fibrosis transmembrane conductance regulator (CFTR) protein causes cystic fibrosis (CF), the commonest Mendelian disease in Caucasians. Despite recent advances in precision medicines for CF patients, many CFTR mutants have not been characterized and the effects of these new therapeutic approaches are still unclear for those mutants. Methods: Cells transfected or stably expressing four CFTR transmembrane-domain mutants (G85E, E92K, L1077P, and M1101K) were used to: 1) characterize the mutants according to their protein expression, thermal sensitivity, and degradation pathways; 2) evaluate the effects of correctors in rescuing them; and 3) explore the effects of correctors on CFTR interactions with proteostasis components. Results: All four mutants exhibited lower protein expression than did wild type-CFTR, and they were degraded by proteasomes and aggresomes. At low temperature, only cells expressing the mutants L1077P and M1101K exhibited increased CFTR maturation. Co-administration of C4 and C18 showed the greatest effect, restoring functional expression and partial stability of CFTR bearing E92K, L1077P, or M1101K at the cell surface. However, this treatment was inefficient in rectifying the defect of CFTR bearing G85E. Correctors rescued CFTR mutants by reducing their interactions with proteostasis components associated with protein retention in the endoplasmic reticulum and ubiquitination. Conclusion: Co-administration of C4 and C18 rescued CFTR transmembrane-domain mutants by remodeling the CFTR interactome.

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Section: Resultsmentioning

confidence: 99%

“…To answer this question, we incubated the cells bearing these mutants for 16 h with several correctors (see supplementary material, Fig. S2-S5): C3 and C18, discovered by Vertex Pharmaceuticals [25]; C4, developed by the Verkman lab [21]; and the CFFT compounds 002 and 003 [19, 24]. …”

Section: Resultsmentioning

confidence: 99%

Combination of Correctors Rescues CFTR Transmembrane-Domain Mutants by Mitigating their Interactions with Proteostasis

Lopes‐Pacheco¹,

Boinot²,

Sabirzhanova³

et al. 2017

Cell Physiol Biochem

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“…Given that CFTR-mediated chloride secretion is positively regulated by cAMP, 31, 32 we added the adenylate cyclase activator forskolin (10 μM) and potentiated the CFTR-mediated chloride secretion with the tyrosine kinase inhibitor genistein (30 μM). Thiazolidonone, a specific CFTR inhibitor (CFTR inh 172), 33, 34 was added at 10 μM to inhibit the I SC , indicating that the measured current was indeed generated by the CFTR. Pretreatment with tubacin significantly reduced the CFTR-dependent I SC in MDCK.2 cells when compared to DMSO-treated cells (Fig.…”

Section: Resultsmentioning

confidence: 99%

Inhibition of histone deacetylase 6 activity reduces cyst growth in polycystic kidney disease

Cebotaru

Liu

Yanda

et al. 2016

Kidney International

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Abnormal proliferation of cyst-lining epithelium and increased intra-cystic fluid secretion via the cystic fibrosis transmembrane conductance regulator (CFTR) are thought to contribute to cyst growth in autosomal dominant polycystic kidney disease (ADPKD). Histone deacetylase 6 (HDAC6) expression and activity are increased in certain cancers, and neurodegenerative diseases, and in Pkd1-mutant renal epithelial cells. Inhibition of HDAC6 activity with specific inhibitors slows cancer growth. Here we studied the effect of tubacin, a specific HDAC6 inhibitor, on cyst growth in polycystic kidney disease. Treatment with tubacin prevented cyst formation in MDCK cells, an in vitro model of cystogenesis. Cyclic AMP stimulates cell proliferation and activates intra-cystic CFTR-mediated chloride secretion in ADPKD. Treatment with tubacin down-regulated cyclic AMP levels, inhibited cell proliferation, and inhibited cyclic AMP-activated CFTR chloride currents in MDCK cells. We also found that tubacin reduced cyst growth by inhibiting proliferation of cyst-lining epithelial cells, down-regulated cyclic AMP levels, and improved renal function in a Pkd1-conditional mouse model of ADPKD. Thus, HDAC6 could play a role in cyst formation and could serve as a potential therapeutic target in ADPKD.

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“…To test the hypothesis that TRADD regulation might be mediated by a proteolytic mechanism, we treated cells with MG132, or E64 to inhibit proteosomal or lysosomal degradation, respectively (see [40] for a description of both inhibitors). Figure 10 C & D shows that in cells transfected with Wt CFTR, there is a significant increase in TRADD protein in response to either MG132 or E64; the greater increase was noted with MG132.…”

Section: Functional Cftr Regulates the Degradation Of Traddmentioning

confidence: 99%

CFTR Controls the Activity of NF-κB by Enhancing the Degradation of TRADD

Wang

Cebotaru

Lee

et al. 2016

Cell Physiol Biochem

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Background/Aims: Chronic lung infection in cystic fibrosis leads to an inflammatory response that persists because of the chronic presence of bacteria and ultimately leads to a catastrophic failure of lung function. Methods: We use a combination of biochemistry, cell and molecular biology to study the interaction of TRADD, a key adaptor molecule in TNFα signaling, with CFTR in the regulation of NFκB. Results: We show that Wt CFTR binds to and colocalizes with TRADD. TRADD is a key signaling intermediate connecting TNFα with activation of NFκB. By contrast, ΔF508 CFTR does not bind to TRADD. NF-κB activation is higher in CFBE expressing ΔF508 CFTR than in cells expressing Wt CFTR. However, this differential effect is abolished when TRADD levels are knocked down. Transfecting Wt CFTR into CFBE cells reduces NF-κB activity. However the reduction is abolished by the CFTR chloride transport inhibitor-172. Consistently, transfecting in the correctly trafficked CFTR conduction mutants G551D or S341A also fail to reduce NFκB activity. Thus CFTR must be functional if it is to regulate NF-κB activity. We also found that TNFα produced a greater increase in NF-κB activity in CFBE cells than in the same cell when Wt CFTR-corrected. Consistently, the effect is also abolished when TRADD is knocked down by shRNA. Thus, Wt CFTR control of TRADD modulates the physiological activation of NF-κB by TNFα. Based on studies with proteosomal and lysosomal inhibitors, the mechanism by which Wt CFTR, but not ΔF508 CFTR, suppresses TRADD is by lysosomal degradation. Conclusion: We have uncovered a novel mechanism whereby Wt CFTR regulates TNFα signaling by enhancing TRADD degradation. Thus by reducing the levels of TRADD, Wt CFTR suppresses downstream proinflammatory NFκB signaling. By contrast, suppression of NF-κB activation fails in CF cells expressing ΔF508 CFTR.

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Rescue of NBD2 Mutants N1303K and S1235R of CFTR by Small-Molecule Correctors and Transcomplementation

Cited by 41 publications

References 49 publications

Combination of Correctors Rescues CFTR Transmembrane-Domain Mutants by Mitigating their Interactions with Proteostasis

Combination of Correctors Rescues CFTR Transmembrane-Domain Mutants by Mitigating their Interactions with Proteostasis

Inhibition of histone deacetylase 6 activity reduces cyst growth in polycystic kidney disease

CFTR Controls the Activity of NF-κB by Enhancing the Degradation of TRADD

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