TY - JOUR
T1 - The S6 gate in regulatory Kv6 subunits restricts heteromeric K+ channel stoichiometry
AU - Pisupati, Aditya
AU - Mickolajczyk, Keith J.
AU - Horton, William
AU - van Rossum, Damian B.
AU - Anishkin, Andriy
AU - Chintapalli, Sree V.
AU - Li, Xiaofan
AU - Chu-Luo, Jose
AU - Busey, Gregory
AU - Hancock, William O.
AU - Jegla, Timothy
N1 - Funding Information:
W.O. Hancock and K.J. Mickolajczyk were supported by National Institutes of Health grant R01GM076476. K.J. Mickolajczyk was also supported by National Institutes of Health grant 1F99CA223018-01. X. Li and W. Horton were supported by National Institutes of Health grant R01NS069842. The authors declare no competing financial interests. Author contributions: A. Pisupati, K.J. Mickolajczyk, W. Horton, and X. Li designed experiments and analyzed data. J. Chu-Luo and G. Busey constructed molecular reagents. A. Anishkin, S.V. Chintapalli, and D.B. van Rossum performed molecular modeling. A. Pisupati and T. Jegla conceived the study and wrote the manuscript with contributions from A. Anishkin, D.B. Van Rossum, K.J. Mickolajczyk, and W.O. Hancock
Publisher Copyright:
© 2018 Pisupati et al.
PY - 2018/12/1
Y1 - 2018/12/1
N2 - The Shaker-like family of voltage-gated K+ channels comprises four functionally independent gene subfamilies, Shaker (Kv1), Shab (Kv2), Shaw (Kv3), and Shal (Kv4), each of which regulates distinct aspects of neuronal excitability. Subfamilyspecific assembly of tetrameric channels is mediated by the N-terminal T1 domain and segregates Kv1-4, allowing multiple channel types to function independently in the same cell. Typical Shaker-like Kv subunits can form functional channels as homotetramers, but a group of mammalian Kv2-related genes (Kv5.1, Kv6s, Kv8s, and Kv9s) encodes subunits that have a "silent" or "regulatory" phenotype characterized by T1 self-incompatibility. These channels are unable to form homotetramers, but instead heteromerize with Kv2.1 or Kv2.2 to diversify the functional properties of these delayed rectifiers. While T1 self-incompatibility predicts that these heterotetramers could contain up to two regulatory (R) subunits, experiments show a predominance of 3:1R stoichiometry in which heteromeric channels contain a single regulatory subunit. Substitution of the self-compatible Kv2.1 T1 domain into the regulatory subunit Kv6.4 does not alter the stoichiometry of Kv2.1:Kv6.4 heteromers. Here, to identify other channel structures that might be responsible for favoring the 3:1R stoichiometry, we compare the sequences of mammalian regulatory subunits to independently evolved regulatory subunits from cnidarians. The most widespread feature of regulatory subunits is the presence of atypical substitutions in the highly conserved consensus sequence of the intracellular S6 activation gate of the pore. We show that two amino acid substitutions in the S6 gate of the regulatory subunit Kv6.4 restrict the functional stoichiometry of Kv2.1:Kv6.4 to 3:1R by limiting the formation and function of 2:2R heteromers. We propose a two-step model for the evolution of the asymmetric 3:1R stoichiometry, which begins with evolution of self-incompatibility to establish the regulatory phenotype, followed by drift of the activation gate consensus sequence under relaxed selection to limit stoichiometry to 3:1R.
AB - The Shaker-like family of voltage-gated K+ channels comprises four functionally independent gene subfamilies, Shaker (Kv1), Shab (Kv2), Shaw (Kv3), and Shal (Kv4), each of which regulates distinct aspects of neuronal excitability. Subfamilyspecific assembly of tetrameric channels is mediated by the N-terminal T1 domain and segregates Kv1-4, allowing multiple channel types to function independently in the same cell. Typical Shaker-like Kv subunits can form functional channels as homotetramers, but a group of mammalian Kv2-related genes (Kv5.1, Kv6s, Kv8s, and Kv9s) encodes subunits that have a "silent" or "regulatory" phenotype characterized by T1 self-incompatibility. These channels are unable to form homotetramers, but instead heteromerize with Kv2.1 or Kv2.2 to diversify the functional properties of these delayed rectifiers. While T1 self-incompatibility predicts that these heterotetramers could contain up to two regulatory (R) subunits, experiments show a predominance of 3:1R stoichiometry in which heteromeric channels contain a single regulatory subunit. Substitution of the self-compatible Kv2.1 T1 domain into the regulatory subunit Kv6.4 does not alter the stoichiometry of Kv2.1:Kv6.4 heteromers. Here, to identify other channel structures that might be responsible for favoring the 3:1R stoichiometry, we compare the sequences of mammalian regulatory subunits to independently evolved regulatory subunits from cnidarians. The most widespread feature of regulatory subunits is the presence of atypical substitutions in the highly conserved consensus sequence of the intracellular S6 activation gate of the pore. We show that two amino acid substitutions in the S6 gate of the regulatory subunit Kv6.4 restrict the functional stoichiometry of Kv2.1:Kv6.4 to 3:1R by limiting the formation and function of 2:2R heteromers. We propose a two-step model for the evolution of the asymmetric 3:1R stoichiometry, which begins with evolution of self-incompatibility to establish the regulatory phenotype, followed by drift of the activation gate consensus sequence under relaxed selection to limit stoichiometry to 3:1R.
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U2 - 10.1085/jgp.201812121
DO - 10.1085/jgp.201812121
M3 - Article
C2 - 30322883
AN - SCOPUS:85057765627
SN - 0022-1295
VL - 150
SP - 1702
EP - 1721
JO - Journal of General Physiology
JF - Journal of General Physiology
IS - 12
ER -