Abstract
The Kv2.1 gene encodes a highly conserved delayed rectifier potassium channel that is widely expressed in neurons of the central nervous system. In the bag cell neurons of Aplysia, Kv2.1 channels contribute to the repolarization of action potentials during a prolonged afterdischarge that triggers a series of reproductive behaviors. Partial inactivation of Aplysia Kv2.1 during repetitive firing produces frequency-dependent broadening of action potentials during the afterdischarge. We have now found that, as in mammalian neurons, Kv2.1 channels in bag cell neurons are localized to ring-like clusters in the plasma membrane of the soma and proximal dendrites. Either elevation of cyclic AMP levels or direct electrical stimulation of afterdischarge rapidly enhanced formation of these clusters on the somata of these neurons. In contrast, injection of a 13-amino acid peptide corresponding to a region in the C terminus that is required for clustering of Kv2.1 channels produced disassociation of the clusters, resulting in a more uniform distribution over the somata. Voltage clamp recordings demonstrated that peptide-induced dissociation of the Kv2.1 clusters is associated with an increase in the amplitude of delayed rectifier current and a shift of activation toward more negative potentials. In current clamp recording, injection of the unclustering peptide reduced the width of action potentials and reduced frequency-dependent broadening of action potentials. Our results suggest that rapid redistribution of Kv2.1 channels occurs during physiological changes in neuronal excitability.
Highlights
A series of studies by Trimmer and co-workers [5] have demonstrated that Kv2.1 channels have an unusual distribution in the plasma membrane and that this localization can be modified by neuronal activity
The induction of seizure activity or the application of glutamate or muscarinic agonists to isolated neurons produces dissolution of the clusters leading to a more uniform distribution of Kv2.1 immunoreactivity in the plasma membrane [5]. This alteration in channel location can be attributed to stimulation-induced elevation of calcium levels, which activates a calcium-dependent phosphatase, leading to the dephosphorylation of Kv2.1 at sites located in its cytoplasmic C terminus [6]
Like mammalian Kv2.1, Aplysia Kv2.1 channels form clusters in the plasma membrane at the soma and proximal dendrites of bag cell neurons
Summary
Animals and Cell Culture—Adult A. californica weighing 100 –200 g were obtained from Marine Specimens Unlimited (San Francisco, CA) or Marinus Inc. (Long Beach, CA). The coverslips were washed extensively with PBS and incubated for 2 h at room temperature with fluorescein or Cy3-conjugated goat anti-chicken IgG secondary antibodies (FITC-G␣CigG or Cy3-G␣CigG, Molecular Probes). Injection of Anti-Aplysia Kv2.1 Peptide into Bag Cell Neurons— Bag cell neurons were isolated and maintained in primary culture according to the previously described method of Kaczmarek et al [19]. Where gK1 describes the value of the Aplysia Kv2.1 conductance This equation is similar to that used previously to describe the effects of Aplysia Kv2.1 on action potentials of bag cell neurons [8] except for the addition of a second voltage-dependent potassium conductance (gK2) governed by the gating variable p, which evolved according to equations identical in form to Equations. Microelectrodes were pulled from borosilicate glass capillaries (1.2-mm ID, TW 120F-4; World Precision Instruments, Sarasota, FL) and had tip diameters of Ͻ1 m and had resistances of ϳ2 M⍀ when the effects of altered voltage dependence, gK1 was 1.5 s, but Vm was changed from Ϫ10 to Ϫ20 mV
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