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Dive into the research topics where Dominique Loffing-Cueni is active.

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Featured researches published by Dominique Loffing-Cueni.


Journal of Biological Chemistry | 1998

Membrane Trafficking of the Cystic Fibrosis Gene Product, Cystic Fibrosis Transmembrane Conductance Regulator, Tagged with Green Fluorescent Protein in Madin-Darby Canine Kidney Cells

Bryan D. Moyer; Johannes Loffing; Erik M. Schwiebert; Dominique Loffing-Cueni; Patricia A. Halpin; Katherine H. Karlson; Iskandar I. Ismailov; William B. Guggino; George M. Langford; Bruce A. Stanton

The mechanism by which cAMP stimulates cystic fibrosis transmembrane conductance regulator (CFTR)-mediated chloride (Cl−) secretion is cell type-specific. By using Madin-Darby canine kidney (MDCK) type I epithelial cells as a model, we tested the hypothesis that cAMP stimulates Cl− secretion by stimulating CFTR Cl− channel trafficking from an intracellular pool to the apical plasma membrane. To this end, we generated a green fluorescent protein (GFP)-CFTR expression vector in which GFP was linked to the N terminus of CFTR. GFP did not alter CFTR function in whole cell patch-clamp or planar lipid bilayer experiments. In stably transfected MDCK type I cells, GFP-CFTR localization was substratum-dependent. In cells grown on glass coverslips, GFP-CFTR was polarized to the basolateral membrane, whereas in cells grown on permeable supports, GFP-CFTR was polarized to the apical membrane. Quantitative confocal fluorescence microscopy and surface biotinylation experiments demonstrated that cAMP did not stimulate detectable GFP-CFTR translocation from an intracellular pool to the apical membrane or regulate GFP-CFTR endocytosis. Disruption of the microtubular cytoskeleton with colchicine did not affect cAMP-stimulated Cl− secretion or GFP-CFTR expression in the apical membrane. We conclude that cAMP stimulates CFTR-mediated Cl− secretion in MDCK type I cells by activating channels resident in the apical plasma membrane.


American Journal of Physiology-renal Physiology | 1999

Butyrate increases apical membrane CFTR but reduces chloride secretion in MDCK cells.

Bryan D. Moyer; Dominique Loffing-Cueni; Jan Loffing; Donna Reynolds; Bruce A. Stanton

Sodium butyrate and its derivatives are useful therapeutic agents for the treatment of genetic diseases including urea cycle disorders, sickle cell disease, thalassemias, and possibly cystic fibrosis (CF). Butyrate partially restores cAMP-activated Cl(-) secretion in CF epithelial cells by stimulating DeltaF508 cystic fibrosis transmembrane conductance regulator (DeltaF508-CFTR) gene expression and increasing the amount of DeltaF508-CFTR in the plasma membrane. Because the effect of butyrate on Cl(-) secretion by renal epithelial cells has not been reported, we examined the effects of chronic butyrate treatment (15-18 h) on the function, expression, and localization of CFTR fused to the green fluorescent protein (GFP-CFTR) in stably transfected MDCK cells. We report that sodium butyrate reduced Cl(-) secretion across MDCK cells, yet increased apical membrane GFP-CFTR expression 25-fold and increased apical membrane Cl(-) currents 30-fold. Although butyrate also increased Na-K-ATPase protein expression twofold, the drug reduced the activity of the Na-K-ATPase by 55%. Our findings suggest that butyrate inhibits cAMP-stimulated Cl(-) secretion across MDCK cells in part by reducing the activity of the Na-K-ATPase.


Biophysical Journal | 1998

Subunit Stoichiometry of a Core Conduction Element in a Cloned Epithelial Amiloride-Sensitive Na+ Channel

Bakhrom K. Berdiev; Katherine H. Karlson; Biljana Jovov; Pierre Jean Ripoll; Ryan Morris; Dominique Loffing-Cueni; Patricia A. Halpin; Bruce A. Stanton; Thomas R. Kleyman; Iskander I. Ismailov

The molecular composition of a core conduction element formed by the alpha-subunit of cloned epithelial Na+ channels (ENaC) was studied in planar lipid bilayers. Two pairs of in vitro translated proteins were employed in combinatorial experiments: 1) wild-type (WT) and an N-terminally truncated alphaDeltaN-rENaC that displays accelerated kinetics (tauo = 32 +/- 13 ms, tauc = 42 +/- 11 ms), as compared with the WT channel (tauc1 = 18 +/- 8 ms, tauc2 = 252 +/- 31 ms, and tauo = 157 +/- 43 ms); and 2) WT and an amiloride binding mutant, alphaDelta278-283-rENaC. The channels that formed in a alphaWT:alphaDeltaN mixture fell into two groups: one with tauo and tauc that corresponded to those exhibited by the alphaDeltaN-rENaC alone, and another with a double-exponentially distributed closed time and a single-exponentially distributed open time that corresponded to the alphaWT-rENaC alone. Five channel subtypes with distinct sensitivities to amiloride were found in a 1alphaWT:1alphaDelta278-283 protein mixture. Statistical analyses of the distributions of channel phenotypes observed for either set of the WT:mutant combinations suggest a tetrameric organization of alpha-subunits as a minimal model for the core conduction element in ENaCs.


American Journal of Physiology-cell Physiology | 2001

Trafficking of GFP-tagged ΔF508-CFTR to the plasma membrane in a polarized epithelial cell line

Dominique Loffing-Cueni; Jan Loffing; Collin M. Shaw; Amilyn M. Taplin; Malu Govindan; Caitlin R. Stanton; Bruce A. Stanton


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Marion Vallet; Nicolas Picard; Dominique Loffing-Cueni; Marinos Fysekidis; May Bloch-Faure; Georges Deschênes; Sylvie Breton; Pierre Meneton; Johannes Loffing; Peter S. Aronson; Régine Chambrey; Dominique Eladari


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Marion Vallet; Nicolas Picard; Dominique Loffing-Cueni; Marinos Fysekidis; May Bloch-Faure; Georges Deschênes; Sylvie Breton; Pierre Meneton; Johannes Loffing; Peter S. Aronson; Régine Chambrey; Dominique Eladari


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Marion Vallet; Nicolas Picard; Dominique Loffing-Cueni; Marinos Fysekidis; May Bloch-Faure; Georges Deschênes; Sylvie Breton; Pierre Meneton; Johannes Loffing; Peter S. Aronson; Régine Chambrey; Dominique Eladari


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Marion Vallet; Nicolas Picard; Dominique Loffing-Cueni; Marinos Fysekidis; May Bloch-Faure; Georges Deschênes; Sylvie Breton; Pierre Meneton; Johannes Loffing; Peter S. Aronson; Régine Chambrey; Dominique Eladari


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Marion Vallet; Nicolas Picard; Dominique Loffing-Cueni; Marinos Fysekidis; May Bloch-Faure; Georges Deschênes; Sylvie Breton; Pierre Meneton; Johannes Loffing; Peter S. Aronson; Régine Chambrey; Dominique Eladari


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Marion Vallet; Nicolas Picard; Dominique Loffing-Cueni; Marinos Fysekidis; May Bloch-Faure; Georges Deschênes; Sylvie Breton; Pierre Meneton; Johannes Loffing; Peter S. Aronson; Régine Chambrey; Dominique Eladari

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Georges Deschênes

Centre national de la recherche scientifique

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Erik M. Schwiebert

University of Alabama at Birmingham

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