De Stefano S , Pusch M , Zifarelli G .

GGP12008 Telethon, TI_GGP12008 Telethon

	Figure 1. Location of the residue D76 mapped on the structure of ClC-ec1 (PDB entry: 1OTS)A, dimeric structure of ClC-ec1 viewed from the membrane plane (extracellular side above and cytoplasmic side below). The two subunits are shown in green and cyan. Residue E148 (corresponding to E211 in ClC-5) is coloured in blue, D54 (corresponding to D76 of ClC-5) is shown in red and E203 (corresponding to E268 of ClC-5) in orange. Cl− anions bound to Scen and Sint are shown in magenta. B, expanded representation of the anion permeation pathway for one of the subunits. The position of the three binding sites, Sext, Scen and Sint, is also indicated by horizontal dashed lines. C, same representation as in B with a top view perpendicular to the membrane. In B and C, some transmembrane helices were removed for clarity.
	Figure 2. pH dependence of D76H and WTRepresentative current recordings for D76H (upper traces) and WT ClC-5 (lower traces) at pH 7.3 and 5.3. Voltages of the test pulse ranged from 120 to –80 mV. Here and in all figures with current traces, the dashed line represents the zero current level.
	Figure 3. pH dependence of inward tail currentsRepresentative current recordings for D76H (upper traces) and WT ClC-5 (lower traces) at some of the pHext values tested (7.3, 6.3, 5.3, 4.3), obtained with a voltage protocol comprising a pre-pulse and a post-pulse to 100 mV.
	Figure 4. Chloride dependence of inward tail currentsRepresentative current recordings for D76H (upper traces) and WT ClC-5 (lower traces) at different [Cl−]ext (10, 30, 100 and 300 mm). pHext is 5.3.
	Figure 5. Dependence of the inward tail currents of D76H on pHext and [Cl−]extA, changes in the reversal potential as a function of pHext are presented as ΔVrev, obtained as the difference between the reversal potential value at each pH and the value obtained at pH 5.3. Data are presented for pH 4.3 (n= 7), 4.8 (n= 7), 5.3 (n= 12), 6.3 (n= 5), 6.8 (n= 5), 7.3 (n= 5) and 8 (n= 6). Measurements were performed at 100 mm[Cl−]ext. The full, dashed-dotted, dashed and dotted lines represent the theoretical expectation for the changes in the reversal potential for transporters with 2 : 1, 3 : 1 or 1 : 1 Cl−/H+ stoichiometry or a pure proton conductance, respectively, under the same pH conditions. ΔVrev values calculated do not depend on assumptions on [Cl−]int (eqn (3)). B, the reversal potential as a function of [Cl−]ext is presented as the difference between the reversal potential value at each Cl− concentration and the value obtained at 100 mm[Cl−]. Data are presented for [Cl−] of 10 mm (n= 8), 30 mm (n= 7), 100 mm (n= 7) and 300 mm (n= 6). Full, dashed-dotted, dashed and dotted lines have the same meaning as in A. ΔVrev values calculated do not depend on assumptions on pHint (eqn (3)). Error bars are mostly smaller than symbols.
	Figure 6. Dependence of the inward tail currents on pHintA, representative inward tail currents at the indicated pHint values (5.3, 7.3, 9.3) from three different oocytes. [Cl−]ext is 110 mm and pHext is 5.8. Currents shown are the average of five traces. B, mean values of the reversal potential at pHint 7.3 (n= 5) and 9.3 (n= 3). The full, dashed-dotted, dashed and dotted lines represent the theoretical expectation for the changes in the reversal potential for transporters with a 2 : 1, 3 : 1 or 1 : 1 Cl−/H+ stoichiometry or a pure proton conductance, respectively, derived from eqn (3).
	Figure 7. Dependence of the inward tail currents on [Cl−]intA, representative inward tail currents at the indicated [Cl−]int (104 and 21 mm). [Cl−]ext is 110 mm and pHext is 5.8. Currents shown are the average of five traces. B, mean values of the reversal potential at [Cl−]int = 104 (n= 5) and 21 mm (n= 4). The full, dashed-dotted, dashed and dotted lines represent the theoretical expectation for the changes in the reversal potential for transporters with a 2 : 1, 3 : 1 or 1 : 1 Cl−/H+ stoichiometry or a pure proton conductance, respectively, derived from eqn (3). Error bars are smaller than symbols.
	Figure 8. Voltage dependence of gating of D76H as a function of pHextA, representative current traces at the indicated pHext from one oocyte. Red lines represent the mono-exponential fit of the tail currents elicited by a post-pulse to 100 mV. The amplitude of the tail currents at the onset of the post-pulse was extrapolated from the fit. These values were normalized with the parameter Imax derived from the fit with eqn (1) to obtain the current–voltage (I–V) relationships. B, I–V relationships for the oocyte shown in A. Full lines are the fit of the data with a Boltzmann function (eqn (1)) providing estimates for V1/2 and z of 21, 39, 89, 141 mV and 1.1, 1.0, 0.8 and 0.5, respectively, for pH 7.3, 6.3, 5.3 and 4.3. C. mean values of the difference between V1/2 calculated at pH 4.3 (n= 6), 6.3 (n= 5), 7.3 (n= 7) and that calculated at pH 5.3 (n= 10) as a function of pHext. The full line represents the fit of the data with a linear function with a slope of 30.7 ± 6.4 per pH unit.
	Figure 9. Comparison of the transient currents of E268A and D76H–E268A at different [Cl−]extA, representative current recordings from two oocytes, one expressing E268A (upper panel) and one expressing D76H–E268A (lower panel) at the indicated [Cl−]ext. B and C, average values for V1/2 and z, respectively, obtained from the Boltzmann fit of the Q–V relationship for [Cl−]ext of 0 mm (a contaminating concentration of 80 μm was assumed, see Zifarelli et al. 2012) (n= 6), 3 mm (n= 7), 10 mm (n= 6), 30 mm (n= 7) and 100 mm (n= 6) (eqn (3) and Supplemental material).
	Figure 10. Schematic model of the transport cycle of ClC-5 including a gating mechanismThe hypothetical model is based on the transport cycle suggested for ClC-Cm by Feng et al. (2010) with the addition of state (c). The model is not intended to provide a realistic description of the ClC-5 transport cycle, but rather to guide a mechanistic interpretation of the results. Circles represent Cl− ions; the shaded box represents the branch of the transport cycle that is accessible to the E268A mutant. From any of the states composing the transport cycle, indicated collectively by a brace, ClC-5 can transition to the inactive state I in which it is not able to transport. Forward and backward transitions to state I are voltage and pH dependent. In state (a), the side chain of E211 is unprotonated and the transporter has all the binding sites occupied by Cl− ions. In state (b), the side chain of E211 moves to occupy Sext and one Cl− ion moves intracellularly. In state (c), the side chain of E211 moves to occupy Scen and this is associated with the transport of another Cl− ion, whereas Sext is transiently empty but binds an extracellular Cl− ion in state (d). From this conformation E211 can be protonated by an intracellular proton (state e) and can move outwardly (state f), giving way to Cl− binding from the extracellular space (state g).

Accardi, Secondary active transport mediated by a prokaryotic homologue of ClC Cl- channels. 2004, Pubmed

Accardi, Secondary active transport mediated by a prokaryotic homologue of ClC Cl- channels. 2004, Pubmed
Accardi, Conformational changes in the pore of CLC-0. 2003, Pubmed , Xenbase
Accardi, Separate ion pathways in a Cl-/H+ exchanger. 2005, Pubmed
Accardi, Ionic currents mediated by a prokaryotic homologue of CLC Cl- channels. 2004, Pubmed
Alekov, Channel-like slippage modes in the human anion/proton exchanger ClC-4. 2009, Pubmed
Bennetts, Temperature dependence of human muscle ClC-1 chloride channel. 2001, Pubmed
Chen, Different fast-gate regulation by external Cl(-) and H(+) of the muscle-type ClC chloride channels. 2001, Pubmed , Xenbase
De Stefano, Extracellular determinants of anion discrimination of the Cl-/H+ antiporter protein CLC-5. 2011, Pubmed , Xenbase
Drummond, Reporting ethical matters in the Journal of Physiology: standards and advice. 2009, Pubmed
Dutzler, X-ray structure of a ClC chloride channel at 3.0 A reveals the molecular basis of anion selectivity. 2002, Pubmed
Dutzler, Gating the selectivity filter in ClC chloride channels. 2003, Pubmed , Xenbase
Engh, Cysteine accessibility in ClC-0 supports conservation of the ClC intracellular vestibule. 2005, Pubmed , Xenbase
Estévez, Conservation of chloride channel structure revealed by an inhibitor binding site in ClC-1. 2003, Pubmed , Xenbase
Fahlke, An aspartic acid residue important for voltage-dependent gating of human muscle chloride channels. 1995, Pubmed , Xenbase
Fahlke, Pore-forming segments in voltage-gated chloride channels. 1997, Pubmed
Feng, Structure of a eukaryotic CLC transporter defines an intermediate state in the transport cycle. 2010, Pubmed
Friedrich, Mutational analysis demonstrates that ClC-4 and ClC-5 directly mediate plasma membrane currents. 1999, Pubmed , Xenbase
Günther, ClC-5, the chloride channel mutated in Dent's disease, colocalizes with the proton pump in endocytotically active kidney cells. 1998, Pubmed
Günther, The ClC-5 chloride channel knock-out mouse - an animal model for Dent's disease. 2003, Pubmed
Hilgemann, Unitary cardiac Na+, Ca2+ exchange current magnitudes determined from channel-like noise and charge movements of ion transport. 1996, Pubmed , Xenbase
Ishida, A model of lysosomal pH regulation. 2013, Pubmed
Jentsch, CLC chloride channels and transporters: from genes to protein structure, pathology and physiology. 2008, Pubmed
Leisle, ClC-7 is a slowly voltage-gated 2Cl(-)/1H(+)-exchanger and requires Ostm1 for transport activity. 2011, Pubmed
Lin, Probing the pore of ClC-0 by substituted cysteine accessibility method using methane thiosulfonate reagents. 2003, Pubmed
Lippiat, The CLC-5 2Cl(-)/H(+) exchange transporter in endosomal function and Dent's disease. 2012, Pubmed
Lloyd, A common molecular basis for three inherited kidney stone diseases. 1996, Pubmed , Xenbase
Ludewig, Inward rectification in ClC-0 chloride channels caused by mutations in several protein regions. 1997, Pubmed
Ludwig, Common gating of both CLC transporter subunits underlies voltage-dependent activation of the 2Cl-/1H+ exchanger ClC-7/Ostm1. 2013, Pubmed , Xenbase
Nguitragool, Uncoupling of a CLC Cl-/H+ exchange transporter by polyatomic anions. 2006, Pubmed
Novarino, Endosomal chloride-proton exchange rather than chloride conductance is crucial for renal endocytosis. 2010, Pubmed
Orhan, Anion- and proton-dependent gating of ClC-4 anion/proton transporter under uncoupling conditions. 2011, Pubmed
Picollo, Molecular determinants of differential pore blocking of kidney CLC-K chloride channels. 2004, Pubmed
Picollo, Chloride/proton antiporter activity of mammalian CLC proteins ClC-4 and ClC-5. 2005, Pubmed
Picollo, Proton block of the CLC-5 Cl-/H+ exchanger. 2010, Pubmed , Xenbase
Piwon, ClC-5 Cl- -channel disruption impairs endocytosis in a mouse model for Dent's disease. 2000, Pubmed
Pusch, Temperature dependence of fast and slow gating relaxations of ClC-0 chloride channels. 1997, Pubmed , Xenbase
Rychkov, Concentration and pH dependence of skeletal muscle chloride channel ClC-1. 1996, Pubmed , Xenbase
Smith, Voltage-dependent charge movement associated with activation of the CLC-5 2Cl-/1H+ exchanger. 2010, Pubmed
Stauber, Cell biology and physiology of CLC chloride channels and transporters. 2012, Pubmed
Stauber, Chloride in vesicular trafficking and function. 2013, Pubmed
Steinmeyer, Cloning and functional expression of rat CLC-5, a chloride channel related to kidney disease. 1995, Pubmed , Xenbase
Traverso, Gating competence of constitutively open CLC-0 mutants revealed by the interaction with a small organic Inhibitor. 2003, Pubmed , Xenbase
Wang, Mice lacking renal chloride channel, CLC-5, are a model for Dent's disease, a nephrolithiasis disorder associated with defective receptor-mediated endocytosis. 2000, Pubmed
Weinert, Lysosomal pathology and osteopetrosis upon loss of H+-driven lysosomal Cl- accumulation. 2010, Pubmed
Zdebik, Determinants of anion-proton coupling in mammalian endosomal CLC proteins. 2008, Pubmed
Zifarelli, The role of protons in fast and slow gating of the Torpedo chloride channel ClC-0. 2010, Pubmed
Zifarelli, On the mechanism of gating charge movement of ClC-5, a human Cl(-)/H(+) antiporter. 2012, Pubmed
Zifarelli, Conversion of the 2 Cl(-)/1 H+ antiporter ClC-5 in a NO3(-)/H+ antiporter by a single point mutation. 2009, Pubmed , Xenbase
Zifarelli, CLC chloride channels and transporters: a biophysical and physiological perspective. 2007, Pubmed