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Plant Physiol, November 1999, Vol. 121, pp. 995-1002
Evaluation of Functional Interaction between K+
Channel - and -Subunits and Putative Inactivation Gating
by Co-Expression in Xenopus laevis
Oocytes1
Xiao
Zhang,2
Jiong
Ma,23 and
Gerald A.
Berkowitz*
Department of Plant Science, University of Connecticut, Storrs,
Connecticut 06269-4067
Animal K+ channel -
(pore-forming) subunits form native proteins by association with
-subunits, which are thought to affect channel function by modifying
electrophysiological parameters of currents (often by inducing fast
inactivation) or by stabilizing the protein complex. We evaluated the
functional association of KAT1, a plant K+ channel
-subunit, and KAB1 (a putative homolog of animal K+
channel -subunits) by co-expression in Xenopus laevis
oocytes. Oocytes expressing KAT1 displayed inward-rectifying,
non-inactivating K+ currents that were similar in magnitude
to those reported in prior studies. K+ currents recorded
from oocytes expressing both KAT1 and KAB1 had similar gating kinetics.
However, co-expression resulted in greater total current, consistent
with the possibility that KAB1 is a -subunit that stabilizes and
therefore enhances surface expression of K+ channel protein
complexes formed by -subunits such as KAT1. K+ channel
protein complexes formed by -subunits such as KAT1 that undergo
(voltage-dependent) inactivation do so by means of a "ball and
chain" mechanism; the ball portion of the protein complex (which can
be formed by the N terminus of either an - or -subunit) occludes
the channel pore. KAT1 was co-expressed in oocytes with an animal
K+ channel -subunit (hKv1.4) known to contain the
N-terminal ball and chain. Inward currents through heteromeric
hKv1.4:KAT1 channels did undergo typical voltage-dependent
inactivation. These results suggest that inward currents through
K+ channel proteins formed at least in part by KAT1
polypeptides are capable of inactivation, but the structural component
facilitating inactivation is not present when channel complexes are
formed by either KAT1 or KAB1 in the absence of additional subunits.
1
This material is based on work supported by the
National Science Foundation (grant nos. MCB-9513921 and BIR-9512977).
This is Storrs Agricultural Experiment Station publication no. 1,883.
2
These authors contributed equally to this manuscript.
3
Present address: Genetic Info Research
Institute, 1170 Morse Avenue, Sunnyvale, CA 94089.
*
Corresponding author; e-mail
gberkowi{at}canr1.cag.uconn.edu; fax 860-486-0682.
© 1999 American Society of Plant Physiologists
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