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    Effect of an autism-associated variant, G124R, on BK channel properties.

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    Author
    Moldenhauer, Hans J
    Dinsdale, Ria L
    Alvarez, Sara
    Fernández-Jaén, Alberto
    Meredith, Andrea L
    Date
    2022-09-25
    Journal
    Current research in physiology
    Type
    Article
    
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    See at
    https://doi.org/10.1016/j.crphys.2022.09.001
    Abstract
    BK K+ channels are critical regulators of neuron and muscle excitability, comprised of a tetramer of pore-forming αsubunits from the KCNMA1 gene and cell- and tissue-selective β subunits (KCNMB1-4). Mutations in KCNMA1 are associated with neurological disorders, including autism. However, little is known about the role of neuronal BK channel β subunits in human neuropathology. The β2 subunit is expressed in central neurons and imparts inactivation to BK channels, as well as altering activation and deactivation gating. In this study, we report the functional effect of G124R, a novel KCNMB2 mutation obtained from whole-exome sequencing of a patient diagnosed with autism spectrum disorder. Residue G124, located in the extracellular loop between TM1 and TM2, is conserved across species, and the G124R missense mutation is predicted deleterious with computational tools. To investigate the pathogenicity potential, BK channels were co-expressed with β2WT and β2G124R subunits in HEK293T cells. BK/β2 currents were assessed from inside-out patches under physiological K+ conditions (140/6 mM K+ and 10 μM Ca2+) during activation and inactivation (voltage-dependence and kinetics). Using β2 subunits lacking inactivation (β2IR) revealed that currents from BK/β2IRG124R channels activated 2-fold faster and deactivated 2-fold slower compared with currents from BK/β2IRWT channels, with no change in the voltage-dependence of activation (V1/2). Despite the changes in the BK channel opening and closing, BK/β2G124R inactivation rates (τinact and τrecovery), and the V1/2 of inactivation, were unaltered compared with BK/β2WT channels under standard steady-state voltage protocols. Action potential-evoked current was also unchanged. Thus, the mutant phenotype suggests the β2G124R TM1-TM2 extracellular loop could regulate BK channel activation and deactivation kinetics. However, additional evidence is needed to validate pathogenicity for this patient-associated variant in KCNMB2.
    Rights/Terms
    © 2022 The Authors.
    Keyword
    Autism
    BK channel
    Calcium-activated potassium channel
    Channelopathy
    Inactivation
    Intellectual disability
    KCNMA1
    KCNMB2
    KCa1.1
    MaxiK
    Potassium channel
    Slo
    Slowpoke
    beta2
    Show allShow less
    Identifier to cite or link to this item
    http://hdl.handle.net/10713/19945
    ae974a485f413a2113503eed53cd6c53
    10.1016/j.crphys.2022.09.001
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