The Role of Distal S6 Hydrophobic Residues in the Voltage-dependent Gating of CaV2.3 Channels

Raybaud, Alexandra; Baspinar, Ebru-Eylem; Dionne, François; Dodier, Yolaine; Sauvé, Rémy; Parent, Lucie

doi:10.1074/jbc.m703895200

Cited by 22 publications

(42 citation statements)

References 53 publications

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“…Mutations within IIS6 were found to impact most significantly on the activation gating of Ca V 2.3. In particular, I701G shifted by Ϫ35 mV the voltage dependence of activation while slowing down inactivation and deactivation kinetics (20). These data indicated that IIS6 plays a unique role in the channel equilibrium between the closed and the open state(s) in Ca V 2.3.…”

Section: ؊1mentioning

confidence: 74%

“…In contrast to K V channels, Ca V channels are structurally asymmetrical with four distinct albeit homologous S4S5 linkers and four distinct S6 helices. We have already shown that glycine substitutions in the distal S6 regions of domains I, II, III, and IV altered the relative stability between the open and closed states (20). Mutations within IIS6 were found to impact most significantly on the activation gating of Ca V 2.3.…”

Section: ؊1mentioning

confidence: 99%

“…Point mutations were produced with the QuikChange XL-mutagenesis kit (Strategene, La Jolla, CA) using 39-mer primers on the full-length Ca V 2.3 clone as described elsewhere (20). Constructs were verified by automated double-stranded sequence analysis (Genomics Platform, IRIC, Université de Montréal, QC, Canada).…”

Section: Methodsmentioning

confidence: 99%

“…Whole Cell Recording and Data Acquisition in OocytesWild-type and mutant channels were screened at room temperature for macroscopic Ba 2ϩ currents, 2 to 4 days after RNA injection, using a two-electrode voltage-clamp amplifier (OC-725C, Warner Instruments) as described earlier (20,29,34). Oocytes were routinely injected with 23 nl of a 50 mM EGTA (Sigma) solution 0.5 to 2 h before the experiments.…”

Section: Methodsmentioning

confidence: 99%

“…Functional Expression of Ca V 2.3-Oocytes were obtained from female Xenopus laevis clawed frogs as described previously (20,29). Oocytes were injected with 46 or 4.6 nl of a solution containing cRNA coding for the Ca V ␣1, Ca V ␣2b␦, and Ca V ␤3 subunits in a 6:2:3 weight ratio.…”

Section: Methodsmentioning

confidence: 99%

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Double Mutant Cycle Analysis Identified a Critical Leucine Residue in the IIS4S5 Linker for the Activation of the CaV2.3 Calcium Channel

Wall-Lacelle

Hossain

Sauvé

et al. 2011

Journal of Biological Chemistry

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Voltage-dependent Ca 2ϩ channels are membrane proteins that play a critical role in promoting Ca 2ϩ influx in response to membrane depolarization in excitable cells (1-6). The Ca V ␣1 subunits of voltage-dependent Ca 2ϩ channels are evolutionarily related to the ␣ subunit of K V channels with a single polypeptidic chain carrying four domains of six transmembrane segments (S1-S6). Although the overall identity at the primary sequence level is quite low between Ca V and K V channels, it improves significantly for transmembrane segments. By homology with the three-dimensional structures of KcsA, MthK, K V AP, KirBac, and K V 1.2 channels (7-11), the four S4 transmembrane segments are thus believed to act as the voltage sensor, whereas the S6 helices line the channel pore of Ca V ␣1.Both in K V and Ca V channels, the question as to how the S4 motion is transmitted to the S6 helix to open the gate upon depolarization remains heavily studied. In the electromechanical coupling model based upon the K V 1.2 crystal structure (12), the S4S5 linker, which is located within atomic proximity (4 -5 Å) of the S6 helix, interacts with the latter in the closed state of the channel. The movement of the S4 voltage sensor is likely to induce a conformational change that pulls the S4S5 linker away from the S6 inner helix ultimately resulting in ions flowing through the pore. The closed conformation of the channel is postulated to be stabilized by hydrophobic interactions at the level of the "closed bundle" in S6 (13-15).Experimental evidence supporting a role for the S4S5 linker in the voltage dependence of activation of K V channels is steadily mounting. Introduction of the S4S5 linker from KcsA disrupts the voltage-dependent activation of K V 2.1 (16, 17). In hERG, cross-linking studies have shown that residues located in the S4S5 linker and in the S6 helix are in atomic proximity and that gating currents were greatly affected as a result of disulfide bridge formation (18). Furthermore, mutations of a unique glycine residue (Gly-546) within the N-terminal end of the S4S5 linker were shown to stabilize the closed state by ϳ1.6 -4.3 kcal/mol and restricted the voltage sensor movement (19).The potential coupling mechanism between the S4S5 linker and the S6 helix has yet to be explored in Ca V channels. In contrast to K V channels, Ca V channels are structurally asymmetrical with four distinct albeit homologous S4S5 linkers and four distinct S6 helices. We have already shown that glycine substitutions in the distal S6 regions of domains I, II, III, and IV altered the relative stability between the open and closed states (20). Mutations within IIS6 were found to impact most significantly on the activation gating of Ca V 2.3. In particular, I701G shifted by Ϫ35 mV the voltage dependence of activation while slowing down inactivation and deactivation kinetics (20). These data indicated that IIS6 plays a unique role in the channel equilibrium between the closed and the open state(s) in Ca V 2.3.To determine whether the S4S5 linker of Domai...

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Section: ؊1mentioning

confidence: 74%

Section: ؊1mentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

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Double Mutant Cycle Analysis Identified a Critical Leucine Residue in the IIS4S5 Linker for the Activation of the CaV2.3 Calcium Channel

Wall-Lacelle

Hossain

Sauvé

et al. 2011

Journal of Biological Chemistry

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Protein Interaction Partners of Cav2.3 R-Type Voltage-Gated Calcium Channels

Dibué

Tevoufouet

Neumaier

et al. 2013

Modulation of Presynaptic Calcium Channels

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Physicochemical properties of pore residues predict activation gating of CaV1.2: A correlation mutation analysis

Beyl

Depil

Hohaus

et al. 2010

Pflugers Arch - Eur J Physiol

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Single point mutations in pore-forming S6 segments of calcium channels may transform a high-voltage-activated into a low-voltage-activated channel, and resulting disturbances in calcium entry may cause channelopathies (Hemara-Wahanui et al., Proc Natl Acad Sci U S A 102(21):7553–7558, 16). Here we ask the question how physicochemical properties of amino acid residues in gating-sensitive positions on S6 segments determine the threshold of channel activation of CaV1.2. Leucine in segment IS6 (L434) and a newly identified activation determinant in segment IIIS6 (G1193) were mutated to a variety of amino acids. The induced leftward shifts of the activation curves and decelerated current activation and deactivation suggest a destabilization of the closed and a stabilisation of the open channel state by most mutations. A selection of 17 physicochemical parameters (descriptors) was calculated for these residues and examined for correlation with the shifts of the midpoints of the activation curve (ΔVact). ΔVact correlated with local side-chain flexibility in position L434 (IS6), with the polar accessible surface area of the side chain in position G1193 (IIIS6) and with hydrophobicity in position I781 (IIS6). Combined descriptor analysis for positions I781 and G1193 revealed that additional amino acid properties may contribute to conformational changes during the gating process. The identified physicochemical properties in the analysed gating-sensitive positions (accessible surface area, side-chain flexibility, and hydrophobicity) predict the shifts of the activation curves of CaV1.2.Electronic supplementary materialThe online version of this article (doi:10.1007/s00424-010-0885-2) contains supplementary material, which is available to authorized users.

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The Role of Distal S6 Hydrophobic Residues in the Voltage-dependent Gating of CaV2.3 Channels

Cited by 22 publications

References 53 publications

Double Mutant Cycle Analysis Identified a Critical Leucine Residue in the IIS4S5 Linker for the Activation of the CaV2.3 Calcium Channel

Double Mutant Cycle Analysis Identified a Critical Leucine Residue in the IIS4S5 Linker for the Activation of the CaV2.3 Calcium Channel

Protein Interaction Partners of Cav2.3 R-Type Voltage-Gated Calcium Channels

Physicochemical properties of pore residues predict activation gating of CaV1.2: A correlation mutation analysis

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