TRPV4 and purinergic receptor signalling pathways are separately linked in airway epithelia to CFTR and TMEM16A chloride channels

Genovese, Michele; Borrelli, Anna; Venturini, Arianna; Guidone, Daniela; Caci, Emanuela; Viscido, Gaetano; Gambardella, Gennaro; Bernardo, Diego di; Scudieri, Paolo; Galietta, Luis J. V.

doi:10.1113/jp278784

Cited by 46 publications

(46 citation statements)

References 55 publications

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“…Similarly, Eact or GSK1016790 did not increase whole cell currents in patch clamp experiments ( Figure 2D,E). This may correspond to the results of a previous report, demonstrating Eact as an activator of Ca 2+ permeable TRPV4 channels, rather than a direct activator of TMEM16A [16]. Although TRPV4 is expressed in HT 29 cells, the rise in intracellular Ca 2+ induced by Eact was insignificant, particularly when compared with the effect of ATP on intracellular Ca 2+ ([Ca 2+ ] i ) ( Figure 2H,I).…”

Section: Ca 2+ -Dependent CL − Transport In Colonic Epithelial Cells supporting

confidence: 91%

“…Similar differential activation of endogenous vs. exogenous TMEM16A was observed for the compound Eact. Eact has been reported as an activator of TMEM16A [15], but was suggested recently to activate TMEM16A indirectly by inducing Ca 2+ influx through activation of TRPV1/4 [16,45]. Currently, Eact is one of the few accessible TMEM16A activators and therefore deserved further analysis: (i) Although TRPV4 is expressed in HT29 cells, Eact and the TRPV4-activator GSK1016790 did not activate TMEM16A.…”

Section: Discussionmentioning

confidence: 99%

“…Similarly, quite different molecules were reported to activate TMEM16A [2], with controversial reports on their efficacy and mechanism of action. Some molecules, such as the putative TMEM16A-activator Eact, were suspected to increase intracellular Ca 2+ rather than directly activating TMEM16A [15,16].…”

Section: Introductionmentioning

confidence: 99%

“…Thus, TMEM16A modulates its own local environment in a way so that it is activated through locally concentrated Ca 2+ release [24]. In many previous studies as well as ongoing work, inhibitors and activators of TMEM16A are used, although they may also affect other TMEM16 paralogs or may exert additional effects on Ca 2+ regulating proteins [16,25]. Here we confirm the role of TMEM16A for intracellular Ca 2+ signaling and show for a number of compounds that they also affect TMEM16F, a paralog of TMEM16A.…”

Section: Introductionmentioning

confidence: 99%

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Pharmacological Inhibition and Activation of the Ca2+ Activated Cl− Channel TMEM16A

Centeio

Cabrita

Benedetto

et al. 2020

IJMS

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TMEM16A is a Ca 2+ activated Cl − channel with important functions in airways, intestine, and other epithelial organs. Activation of TMEM16A is proposed as a therapy in cystic fibrosis (CF) to reinstall airway Cl − secretion and to enhance airway surface liquid (ASL). This CFTR-agnostic approach is thought to improve mucociliary clearance and lung function in CF. This could indeed improve ASL, however, mucus release and airway contraction may also be induced by activators of TMEM16A, particularly in inflamed airways of patients with asthma, COPD, or CF. Currently, both activators and inhibitors of TMEM16A are developed and examined in different types of tissues. Here we compare activation and inhibition of endogenous and overexpressed TMEM16A and analyze potential off-target effects. The three well-known blockers benzbromarone, niclosamide, and Ani9 inhibited both TMEM16A and ATP-induced Ca 2+ increase by variable degrees, depending on the cell type. Niclosamide, while blocking Ca 2+ activated TMEM16A, also induced a subtle but significant Ca 2+ store release and inhibited store-operated Ca 2+ influx. Niclosamide, benzbromarone and Ani9 also affected TMEM16F whole cell currents, indicating limited specificity for these inhibitors. The compounds Eact, cinnamaldehyde, and melittin, as well as the phosphatidylinositol diC8-PIP 2 are the reported activators of TMEM16A. However, the compounds were unable to activate endogenous TMEM16A in HT 29 colonic epithelial cells. In contrast, TMEM16A overexpressed in HEK293 cells was potently stimulated by these activators. We speculate that overexpressed TMEM16A might have a better accessibility to intracellular Ca 2+ , which causes spontaneous activity even at basal intracellular Ca 2+ concentrations. Small molecules may therefore potentiate pre-stimulated TMEM16A currents, but may otherwise fail to activate silent endogenous TMEM16A.

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Section: Ca 2+ -Dependent CL − Transport In Colonic Epithelial Cells supporting

confidence: 91%

Section: Discussionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

See 2 more Smart Citations

Pharmacological Inhibition and Activation of the Ca2+ Activated Cl− Channel TMEM16A

Centeio

Cabrita

Benedetto

et al. 2020

IJMS

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“…To our knowledge, this is the first report of the discovery and efficacy of TMEM16A potentiator compounds. Compounds initially reported to be direct modulators of the channel (e.g., E act ) (38) have subsequently been shown to act indirectly via elevation of [Ca 21 ] i (39,40), negating their utility for validating CaCC function due to the numerous other cellular effects elevation of [Ca 21 ] i will trigger (e.g., goblet cell exocytosis and bronchospasm). In contrast, ETX001 potentiates the opening of the TMEM16A channel (i.e., it enhances the magnitude of the current in the presence of physiologically regulated [Ca 21 ] i ), but ETX001 does not…”

Section: Discussionmentioning

confidence: 99%

TMEM16A Potentiation: A Novel Therapeutic Approach for the Treatment of Cystic Fibrosis

Danahay

Lilley

Fox

et al. 2020

Am J Respir Crit Care Med

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Rationale: Enhancing non-CFTR (cystic fibrosis transmembrane conductance regulator)-mediated anion secretion is an attractive therapeutic approach for the treatment of cystic fibrosis (CF) and other mucoobstructive diseases. Objectives: To determine the effects of TMEM16A potentiation on epithelial fluid secretion and mucociliary clearance. Methods: The effects of a novel low-molecular-weight TMEM16A potentiator (ETX001) were evaluated in human cell and animal models of airway epithelial function and mucus transport. Measurements and Main Results: Potentiating the activity of TMEM16A with ETX001 increased the Ca 21-activated Cl 2 channel activity and anion secretion in human bronchial epithelial (HBE) cells from patients with CF without impacting calcium signaling. ETX001 rapidly increased fluid secretion and airway surface liquid height in CF-HBE cells under both static conditions and conditions designed to mimic the shear stress associated with tidal breathing. In ovine models of mucus clearance (tracheal mucus velocity and mucociliary clearance), inhaled ETX001 was able to accelerate clearance both when CFTR function was reduced by administration of a pharmacological blocker and when CFTR was fully functional. Conclusions: Enhancing the activity of TMEM16A increases epithelial fluid secretion and enhances mucus clearance independent of CFTR function. TMEM16A potentiation is a novel approach for the treatment of patients with CF and non-CF mucoobstructive diseases.

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Validation of TMEM16A Modulation as a Therapeutic Approach for the Treatment of Cystic Fibrosis: The Discovery of Novel TMEM16A Potentiators

Danahay,

Gosling

2024

Ion Channels as Targets in Drug Discovery

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TRPV4 and purinergic receptor signalling pathways are separately linked in airway epithelia to CFTR and TMEM16A chloride channels

Cited by 46 publications

References 55 publications

Pharmacological Inhibition and Activation of the Ca2+ Activated Cl− Channel TMEM16A

Pharmacological Inhibition and Activation of the Ca2+ Activated Cl− Channel TMEM16A

TMEM16A Potentiation: A Novel Therapeutic Approach for the Treatment of Cystic Fibrosis

Validation of TMEM16A Modulation as a Therapeutic Approach for the Treatment of Cystic Fibrosis: The Discovery of Novel TMEM16A Potentiators

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