Redox regulation of KV7 channels through EF3 hand of calmodulin

被引:5
作者
Nunez, Eider [1 ]
Jones, Frederick [2 ]
Muguruza-Montero, Arantza [1 ]
Urrutia, Janire [1 ]
Aguado, Alejandra [1 ]
Malo, Covadonga [1 ]
Bernardo-Seisdedos, Ganeko [3 ]
Domene, Carmen [4 ,5 ]
Millet, Oscar [6 ]
Gamper, Nikita [2 ]
Villarroel, Alvaro [1 ]
Colecraft, Henry M.
机构
[1] Univ Basque Country, Inst Biofis, CSIC, Leioa, Spain
[2] Univ Leeds, Fac Biol Sci, Sch Biomed Sci, Leeds, England
[3] Atlas Mol Pharm SL, Derio, Spain
[4] Univ Bath, Dept Chem, Bath, England
[5] Univ Oxford, Dept Chem, Oxford, England
[6] CIC bioGUNE, Prot Stabil & Inherited Dis Lab, Derio, Spain
来源
ELIFE | 2023年 / 12卷
基金
英国惠康基金;
关键词
KCNQ; calmodulin; redox; calcium; EF-hand; signal transduction; E; coli; REACTIVE OXYGEN; STRUCTURAL BASIS; MOLECULAR-DYNAMICS; HYDROGEN-PEROXIDE; K+ CHANNELS; BINDING; MODULATION; COMPLEX; AUGMENTATION; PLASTICITY;
D O I
10.7554/eLife.81961
中图分类号
Q [生物科学];
学科分类号
07 ; 0710 ; 09 ;
摘要
Neuronal K(V)7 channels, important regulators of cell excitability, are among the most sensitive proteins to reactive oxygen species. The S2S3 linker of the voltage sensor was reported as a site-mediating redox modulation of the channels. Recent structural insights reveal potential interactions between this linker and the Ca2+-binding loop of the third EF-hand of calmodulin (CaM), which embraces an antiparallel fork formed by the C-terminal helices A and B, constituting the calcium responsive domain (CRD). We found that precluding Ca2+ binding to the EF3 hand, but not to EF1, EF2, or EF4 hands, abolishes oxidation-induced enhancement of K(V)7.4 currents. Monitoring FRET (Fluorescence Resonance Energy Transfer) between helices A and B using purified CRDs tagged with fluorescent proteins, we observed that S2S3 peptides cause a reversal of the signal in the presence of Ca2+ but have no effect in the absence of this cation or if the peptide is oxidized. The capacity of loading EF3 with Ca2+ is essential for this reversal of the FRET signal, whereas the consequences of obliterating Ca2+ binding to EF1, EF2, or EF4 are negligible. Furthermore, we show that EF3 is critical for translating Ca2+ signals to reorient the AB fork. Our data are consistent with the proposal that oxidation of cysteine residues in the S2S3 loop relieves K(V)7 channels from a constitutive inhibition imposed by interactions between the EF3 hand of CaM which is crucial for this signaling.
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页数:22
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