Abstract

Ca2+-activated Cl- channels (CaCCs) are ion channels that are opened by increases in cytosolic Ca2+ and selectively conduct Cl- and other anions down their electrochemical gradient. Their best known function is epithelial fluid secretion. CaCCs are encoded by members of two different gene families, Bestrophins and Anoctamins (also called TMEM16). Mutations in BEST1 cause a spectrum of retinal degenerations called bestrophinopthies. ANO1 and ANO2, while not yet linked directly to retinal disease, are expressed in a variety of cells in the retina including photoreceptors and RPE. Since their discovery in 2008, it has since become increasingly apparent that anoctamins are amazingly versatile: ANO1 has a very broad range of functions that encompass sensory transduction and adaptation, regulation of myoepithelial cell and smooth muscle tone, control of neuronal and cardiac excitability, and nociception. In addition, evidence is accumulating that ANO1 plays fundamental roles in cell biological processes like regulation of cell motility, proliferation, and primary ciliogenesis. Recently, we observed that ANO1, while spread over the cell surface in non-confluent cells, becomes concentrated in a distinctive apical torus (the nimbus) as cells become confluent and polarize. The nimbus becomes the site where the primary cilium emerges from the cell. The primary cilium, a non-motile cellular antenna that is packed with sensory receptors, plays a pivotal role in tissue morphogenesis and development and is closely linked to cell proliferation and migration. Mutations in various genes involved in ciliogenesis produce a diverse spectrum of human disorders called ciliopathies that are very frequently characterized by retinal degeneration. We have found that disrupting ANO1 function or expression has profound effects on the development of the primary cilium. The goal of this research is to elucidate the role of ANO1 in the genesis and function of the primary cilium. We hypothesize that ANO1 plays a key role in organizing a subdomain of the apical membrane to make it competent for ciliogenesis to occur. We imagine two mechanisms by which ANO1 may function in this context. (i) ANO1 may operate as a scaffold to organize and coordinate ciliogenic proteins at the apical membrane. This mechanism is supported by our proteomic data that ANO1 interacts with proteins essential for ciliogenesis and that these ciliary proteins regulate ANO1 currents. (ii) Alternatively, Cl- transport through ANO1 may play a role in ciliogenesis. This idea is supported by data that ANO1 channel blockers disrupt ciliogenesis and that the species of anion in the extracellular solution has profound effects on ciliogenesis. Because the primary cilium is a fundamental property of both photoreceptors and retinal pigment epithelial cells, understanding the role of ANO1 in primary ciliogenesis has important implications for retinal biology and therapy of retinal diseases.

Public Health Relevance

Primary cilia are unique sensory appendages present on most cells of the body. Disruption of genes encoding ciliary proteins produce a range of disorders called ciliopathies that often include retinal degeneration. This application explores th workings of a Ca2+-activated Chloride Channel called ANO1 that is present in the primary cilium of retinal pigment epithelial cells and that we propose plays an important role in primary ciliogenesis and/or maintenance

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Eye Institute (NEI)
Type
Research Project (R01)
Project #
5R01EY014852-13
Application #
9233115
Study Section
Neurotransporters, Receptors, and Calcium Signaling Study Section (NTRC)
Program Officer
Neuhold, Lisa
Project Start
2003-08-01
Project End
2021-02-28
Budget Start
2017-03-01
Budget End
2018-02-28
Support Year
13
Fiscal Year
2017
Total Cost
$348,233
Indirect Cost
$123,233

  Institution

Name
Emory University
Department
Anatomy/Cell Biology
Type
Schools of Medicine
DUNS #
066469933
City
Atlanta
State
GA
Country
United States
Zip Code
30322

  Publications

Omotade, Omotola F; Rui, Yanfang; Lei, Wenliang et al. (2018) Tropomodulin Isoform-Specific Regulation of Dendrite Development and Synapse Formation. J Neurosci 38:10271-10285
De Jesús-Pérez, José J; Cruz-Rangel, Silvia; Espino-Saldaña, Ángeles E et al. (2018) Phosphatidylinositol 4,5-bisphosphate, cholesterol, and fatty acids modulate the calcium-activated chloride channel TMEM16A (ANO1). Biochim Biophys Acta Mol Cell Biol Lipids 1863:299-312
Whitlock, Jarred M; Hartzell, H Criss (2017) Anoctamins/TMEM16 Proteins: Chloride Channels Flirting with Lipids and Extracellular Vesicles. Annu Rev Physiol 79:119-143
Jiang, Tao; Yu, Kuai; Hartzell, H Criss et al. (2017) Lipids and ions traverse the membrane by the same physical pathway in the nhTMEM16 scramblase. Elife 6:
Cruz-Rangel, Silvia; De Jesús-Pérez, José J; Aréchiga-Figueroa, Iván A et al. (2017) Extracellular protons enable activation of the calcium-dependent chloride channel TMEM16A. J Physiol 595:1515-1531
Fisher, Skylar Id; Hartzell, H Criss (2017) Poring over furrows. Elife 6:
Whitlock, Jarred M; Hartzell, H Criss (2016) A Pore Idea: the ion conduction pathway of TMEM16/ANO proteins is composed partly of lipid. Pflugers Arch 468:455-73
Hartzell, H Criss; Whitlock, Jarred M (2016) TMEM16 chloride channels are two-faced. J Gen Physiol 148:367-373
Griffin, Danielle A; Johnson, Ryan W; Whitlock, Jarred M et al. (2016) Defective membrane fusion and repair in Anoctamin5-deficient muscular dystrophy. Hum Mol Genet 25:1900-1911
Contreras-Vite, Juan A; Cruz-Rangel, Silvia; De Jesús-Pérez, José J et al. (2016) Revealing the activation pathway for TMEM16A chloride channels from macroscopic currents and kinetic models. Pflugers Arch 468:1241-57

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