Functional and structural characterization of interactions between opposite subunits in HCN pacemaker channels

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DATA_SOURCE_MDsimulation_Modelling.xlsx (34.15 KB)
Data Source Electrophysiology.xlsx (35.21 KB)
Data Source Patch-Clamp-Fluorometry.xlsx (9.29 KB)

Date

2021-08-05

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Abstract

Hyperpolarization-activated and cyclic nucleotide (HCN) modulated channels are tetrameric cation channels. In each of the four subunits, the intracellular cyclic nucleotide-binding domain (CNBD) is coupled to the transmembrane domain via a helical structure, the C-linker. High-resolution channel structures suggest that the C-linker enables functionally relevant interactions with the opposite subunit, which might be critical for coupling the conformational changes in the CNBD to the channel pore. We combined mutagenesis, patch-clamp technique, confocal patch-clamp fluorometry, and molecular dynamics simulations to show that residue K464 of the C-linker is essential for stabilizing the closed state of the mHCN2 channel by forming interactions with the opposite subunit. MD simulations revealed that both cAMP and K464E induce a rotation of the intracellular domain relative to the channel pore, weakening the autoinhibitory effect of the unoccupied CL-CNBD region. The adopted poses are in excellent agreement with structural results.

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HCN channel, molecular dynamics simulations, subunit interaction, patch-clamp technique, confocal patch-clamp fluorometry

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https://researchdata.hhu.de/handle/entry/98
 http://dx.doi.org/10.25838/d5p-27

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Computational Pharmaceutical Chemistry and Molecular Informatics Group