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TMEM16A chloride channel does not drive mucus production

View ORCID ProfileFilipa B Simões, Margarida C Quaresma, Luka A Clarke, View ORCID ProfileIris AL Silva, Ines Pankonien, Violeta Railean, View ORCID ProfileArthur Kmit, View ORCID ProfileMargarida D Amaral  Correspondence email
Filipa B Simões
University of Lisboa, Faculty of Sciences, BioISI–Biosystems & Integrative Sciences Institute, Lisboa, Portugal
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  • ORCID record for Filipa B Simões
Margarida C Quaresma
University of Lisboa, Faculty of Sciences, BioISI–Biosystems & Integrative Sciences Institute, Lisboa, Portugal
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Luka A Clarke
University of Lisboa, Faculty of Sciences, BioISI–Biosystems & Integrative Sciences Institute, Lisboa, Portugal
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Iris AL Silva
University of Lisboa, Faculty of Sciences, BioISI–Biosystems & Integrative Sciences Institute, Lisboa, Portugal
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  • ORCID record for Iris AL Silva
Ines Pankonien
University of Lisboa, Faculty of Sciences, BioISI–Biosystems & Integrative Sciences Institute, Lisboa, Portugal
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Violeta Railean
University of Lisboa, Faculty of Sciences, BioISI–Biosystems & Integrative Sciences Institute, Lisboa, Portugal
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Arthur Kmit
University of Lisboa, Faculty of Sciences, BioISI–Biosystems & Integrative Sciences Institute, Lisboa, Portugal
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  • ORCID record for Arthur Kmit
Margarida D Amaral
University of Lisboa, Faculty of Sciences, BioISI–Biosystems & Integrative Sciences Institute, Lisboa, Portugal
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  • For correspondence: mdamaral@fc.ul.pt
Published 15 November 2019. DOI: 10.26508/lsa.201900462
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Abstract

Airway mucus obstruction is the main cause of morbidity in cystic fibrosis, a disease caused by mutations in the CFTR Cl− channel. Activation of non-CFTR Cl− channels such as TMEM16A can likely compensate for defective CFTR. However, TMEM16A was recently described as a key driver in mucus production/secretion. Here, we have examined whether indeed there is a causal relationship between TMEM16A and MUC5AC production, the main component of respiratory mucus. Our data show that TMEM16A and MUC5AC are inversely correlated during differentiation of human airway cells. Furthermore, we show for the first time that the IL-4–induced TMEM16A up-regulation is proliferation-dependent, which is supported by the correlation found between TMEM16A and Ki-67 proliferation marker during wound healing. Consistently, the notch signaling activator DLL4 increases MUC5AC levels without inducing changes neither in TMEM16A nor in Ki-67 expression. Moreover, TMEM16A inhibition decreased airway surface liquid height. Altogether, our findings demonstrate that up-regulation of TMEM16A and MUC5AC is only circumstantial under cell proliferation, but with no causal relationship between them. Thus, although essential for airway hydration, TMEM16A is not required for MUC5AC production.

  • Received June 20, 2019.
  • Revision received October 29, 2019.
  • Accepted November 6, 2019.
  • © 2019 Simões et al.
Creative Commons logoCreative Commons logohttps://creativecommons.org/licenses/by/4.0/

This article is available under a Creative Commons License (Attribution 4.0 International, as described at https://creativecommons.org/licenses/by/4.0/).

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TMEM16A and mucus production
Filipa B Simões, Margarida C Quaresma, Luka A Clarke, Iris AL Silva, Ines Pankonien, Violeta Railean, Arthur Kmit, Margarida D Amaral
Life Science Alliance Nov 2019, 2 (6) e201900462; DOI: 10.26508/lsa.201900462

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TMEM16A and mucus production
Filipa B Simões, Margarida C Quaresma, Luka A Clarke, Iris AL Silva, Ines Pankonien, Violeta Railean, Arthur Kmit, Margarida D Amaral
Life Science Alliance Nov 2019, 2 (6) e201900462; DOI: 10.26508/lsa.201900462
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Volume 2, No. 6
December 2019
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