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Functional characteristics of two BK(Ca) channel variants differentially expressed in rat brain tissuesopen access

Authors
Ha, T.S.Jeong, S.Y.Cho, S.-W.Jeon, H.-K.Roh, G.S.Choi, W.S.Park, C.-S.
Issue Date
Feb-2000
Keywords
Ca<sup>2+</sup> co-operativity; Large-conductance Ca<sup>2+</sup>-activated K<sup>+</sup> channel; Rslo; Splice variants; Tissue-specific expression
Citation
European Journal of Biochemistry, v.267, no.3, pp 910 - 918
Pages
9
Indexed
SCOPUS
Journal Title
European Journal of Biochemistry
Volume
267
Number
3
Start Page
910
End Page
918
URI
https://scholarworks.gnu.ac.kr/handle/sw.gnu/77615
DOI
10.1046/j.1432-1327.2000.01076.x
ISSN
0014-2956
Abstract
cDNAs encoding large-conductance Ca2+-activated K+ channel α-subunit (rSlo) were obtained from rat brain. From the DNA sequence of multiple rslo clones, we identified a specific sequence variation of 81 nucleotides, which is either absent from or present at the N-terminal region of a putative Ca2+-sensing domain of the channel. Transcripts containing such variations were detected in different ratios from several brain regions, and their functional significance was further examined. When heterologously expressed in Xenopus oocytes, both rSlo variants, named rSlo0 and rSlo27, generated Ca2+-activated and voltage-activated K+ currents characteristic of neuronal large-conductance Ca2+-activated K+ (BK(Ca)) channels. Single- channel recordings of the two channels showed almost identical permeation characteristics and steady-state gating behavior. Noticeable differences between rSlo0 and rSlo27 were revealed when the macroscopic currents were measured at various voltages and intracellular Ca2+ concentrations. rSlo27 activated was more rapidly than rSlo0 in the presence of the same voltage stimulus, and the differences in these activation kinetics were dependent on the concentration of intracellular Ca2+. Despite their similar apparent affinities for Ca2+, rSlo0 and rSlo27 showed significant differences in their co-operative gating behavior. The Hill coefficient for intracellular Ca2+ was estimated to be about 3.7 for rSlo27 regardless of the membrane voltage, and that for rSlo0 was reduced from about 5 to 2 as the membrane voltage changed from 40 to 140 mV. As activation of BK(Ca) channels is involved in rapid hyperpolarization of action potentials, the differential processing of rslo transcripts, and the generation of channels with different activation kinetics and Ca2+ cooperativity may be a mechanism for tuning the excitability of neurons in different brain regions.
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