NMR Structure and Functional Characteristics of the Hydrophilic N Terminus of the Potassium Channel β-Subunit Kvβ1.1

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The auxiliary ␤-subunit KCNMB2 (␤ 2 ) endows the noninactivating large conductance Ca 2؉ -and voltagedependent potassium (BK) channel with fast inactivation. This process is mediated by the N terminus of KCNMB2 and closely resembles the "ball-and-chain"-type inactivation observed in voltage-gated potassium channels. Here we investigated the solution structure and function of the KCNMB2 N terminus (amino acids 1-45, BK␤ 2 N) using NMR spectroscopy and patch clamp recordings. BK␤ 2 N completely inactivated BK channels when applied to the cytoplasmic side; its interaction with the BK ␣-subunit is characterized by a particularly slow dissociation rate and an affinity in the upper nanomolar range. The BK␤ 2 N structure comprises two domains connected by a flexible linker: the pore-blocking "ball domain" (formed by residues 1-17) and the "chain domain" (between residues 20 -45) linking it to the membrane segment of KCNMB2. The ball domain is made up of a flexible N terminus anchored at a well ordered loop-helix motif. The chain domain consists of a 4-turn helix with an unfolded linker at its C terminus. These structural properties explain the functional characteristics of BK␤ 2 N-mediated inactivation.Large conductance K ϩ channels (BK 1 or MaxiK channels) are key modulators of excitability in many types of cell (1, 2).They are formed from four identical ␣-subunits encoded by the Slo gene and are activated by membrane depolarization and/or increase in intracellular Ca 2ϩ concentration ([Ca 2ϩ ] i (3-8)). This dual activation is unique among the large family of K ϩ channels and provides a direct feedback mechanism to regulate Ca 2ϩ influx. In many tissues, the activation gating of BK channels is modulated by accessory ␤-subunits, a family of membrane proteins (KCNMB) closely associated with the ␣-subunit (7). Four KCNMB proteins have been identified (KCNMB1-4), and they all share a prototypic topology of two transmembrane domains with intracellular N and C termini (9 -13). Functionally, each of these KCNMB proteins distinctly changes the rates of channel activation and deactivation as well as the apparent sensitivity of the channel for Ca 2ϩ (9). In addition, one of the ␤-subunits, KCNMB2 (␤ 2 ), was found to confer rapid and complete inactivation to the BK channel complex (11, 12) in a manner similar to that observed in chromaffin cells of the adrenal gland or in hippocampal CA1 neurons (14, 15). Analysis of this KCNMB2-mediated inactivation gating showed that it closely resembled the famous ball-andchain-type inactivation of voltage-gated K ϩ channels (Kv): (i) it is determined by the N terminus of KCNMB2; (ii) it occludes the open channel pore and competes with the pore-blocking agent tetraethylammonium (11, 12); (iii) recovery from inactivation is speeded up by an increase of the extracellular K ϩ concentration (11).Moreover, the N-terminal stretch of the KCNMB2 N terminus (19 amino acids) was shown to be a functional entity, i.e. its fusion to the N terminus of KCNMB1 (␤ 1 ) conferred rapid inactivation to this ...

Section: Bk␤ 2 N Inactivated Bk Channels In a Ball-like Manner-supporting

confidence: 80%

Section: Bk␤ 2 N Inactivated Bk Channels In a Ball-like Manner-supporting

confidence: 48%

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NMR Structure of the “Ball-and-chain” Domain of KCNMB2, the β2-Subunit of Large Conductance Ca2+- and Voltage-activated Potassium Channels

Bentrop

Beyermann

Wissmann

et al. 2001

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“…The structure of the isolated Kv␤1 N terminus (amino acids 1-62) was solved using NMR spectroscopy (17). The N terminus of Kv␤1.1 does not exhibit a well defined, unique, threedimensional structure, indicating a fast conformational equilibrium between weakly structured substrates.…”

Section: Structure and Redox Properties Of Kv ␤-Subunitmentioning

confidence: 99%

A Marriage of Convenience: β-Subunits and Voltage-dependent K+ Channels

Torres

Morera

Carvacho

et al. 2007

107

103

The movement of ions across cell membranes is essential for a wide variety of fundamental physiological processes, including secretion, muscle contraction, and neuronal excitation. This movement is possible because of the presence in the cell membrane of a class of integral membrane proteins dubbed ion channels. Ion channels, thanks to the presence of aqueous pores in their structure, catalyze the passage of ions across the otherwise ion-impermeable lipid bilayer. Ion conduction across ion channels is highly regulated, and in the case of voltage-dependent K

“…This classical gating process is brought about by a "plugin" mechanism in which a protein domain termed "inactivation ball" occludes the ion pathway through interaction with a receptor site in the pore of the channel (6). Structure-function analysis showed: (i) that inactivation domains (ID) are formed by the first 20 -40 amino acids at the N terminus of certain Kv␣ (7)(8)(9)(10) and Kv␤ subunits (11,12); (ii) that IDs inactivate channels independent of whether they are tethered to the protein or offered to the channel as a synthetic peptide (8,9,13,14); (iii) that IDs enter the channel pore and compete with open pore blockers such as tetraethylammonium (TEA) (11,(15)(16)(17); and finally (iv) that NMR-derived solution structures of the known IDs vary from a well ordered and compact folding as in Kv3.4 ID (18) to the disordered and highly flexible ID from ShakerB (19). Different from other ␣/␤ subunits that harbor one ID in their N terminus, Kv1.4 was found to be equipped with two IDs with the ability to endow the channel with rapid inactivation (Fig.…”

mentioning

confidence: 99%

Solution Structure and Function of the “Tandem Inactivation Domain” of the Neuronal A-type Potassium Channel Kv1.4

Wissmann

Bildl

Oliver

et al. 2003

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Cumulative inactivation of voltage-gated (Kv) K؉ channels shapes the presynaptic action potential and determines timing and strength of synaptic transmission. Kv1.4 channels exhibit rapid "ball-and-chain"-type inactivation gating. Different from all other Kv␣ subunits, Kv1.4 harbors two inactivation domains at its N terminus. Here we report the solution structure and function of this "tandem inactivation domain" using NMR spectroscopy and patch clamp recordings. Inactivation domain 1 (ID1, residues 1-38) consists of a flexible N terminus anchored at a 5-turn helix, whereas ID2 (residues 40 -50) is a 2.5-turn helix made up of small hydrophobic amino acids. Functional analysis suggests that only ID1 may work as a pore-occluding ball domain, whereas ID2 most likely acts as a "docking domain" that attaches ID1 to the cytoplasmic face of the channel. Deletion of ID2 slows inactivation considerably and largely impairs cumulative inactivation. Together, the concerted action of ID1 and ID2 may promote rapid inactivation of Kv1.4 that is crucial for the channel function in short term plasticity.