K v 4.2

Kv4.2 (KCND2, Shal family) protein is strongly expressed across the somatodendritic axis of hippocampal CA1 pyramidal neurons [Sheng, 92; Maletic-Savatic, 95], and evidence suggests that the predominant A-type transient current throughout principal neurons of the CNS arises from channels formed by Kv4.2 [Serodio, 94]. By Northern blot analysis, [Zhu, 99; Isbrandt, 00] expression of a 6.8-kb transcript was detected only in brain, particularly in the amygdala, caudate nucleus, cerebellum, hippocampus, substantia nigra, and thalamus. Heterologous expression determined that KCND2 mediates the rapidly inactivating, A-type outward potassium current which is not under the control of the N-terminus as it is in Kv1 (Shaker) channels [Zhu, 99]. The somatodendritic A-type (Kv4.2) channels rapidly inactivate close to the action potential firing threshold and recover from inactivation in the millisecond time range [Pak, 91; Serodio, 94]. In 2001, Bähring and co-workers suggested that Kv4.2 channels in response to membrane depolarization accumulate in the closed-inactivated state, from which they directly recover, bypassing the open state [Bahring, 01]. These features distinguish somatodendritic from other A-type channels.

Pharmacologically, this channel is blocked in a dose-dependent manner by 4-amino pyridine (4-AP) and polyunsaturated fatty acids (PUFA), such as arachidonic acid (AA). The effectiveness of PUFAs, however, is dependent on the gene subfamily that encodes the channel. For example, AA is most efficient in blocking Shal (Kv4) channels, whereas for Shaker (Kv1) channels there are controversial findings [Villarroel, 96; Danthi, 03]. 

Kv1.4

Channels from Kv1 (KNCA, Shaker) subfamily, for instance Kv1.4, also contributes to somatic transient currents in hippocampal basket interneurons [Zhang, 95] and other neurons [Eder, 96; Pardo, 92]. Moreover, there is evidence for heteromultimerization of Kv α-subunits from the same subfamily. It has been shown that antibodies, specific to Kv1.4 co-immunoprecipitate Kv1.2 and Kv1.1 proteins in non-denaturated brain membrane extracts [Sheng, 93]. The co-expression of Kv1.4 and Kv1.2 in axons and terminals of many cells suggests the native A-type K⁺ current may result from Kv1.4/Kv1.2 heteromultimers within these compartments [Sheng, 93; Wang, 99]. Such heteromultimere channels will exhibit hybrid pharmacology, for example to TEA. Therefore, there are not enough high-affinity pharmacological tools available for Kv1.4 channels.

Kv1 transient currents inactivate with time constants that change with the voltage and recover from inactivation very slowly [Po, 93; Stuhmer, 89]. The inactivation mechanism of Kv1.4 is well understood and could be described as a ‘ball-and-chain’ interaction [Hoshi, 90; Hoshi, 91]. In case of Kv1.4 channel, inactivation domain of the N-terminal of the Kv-α subunit [Zagotta, 90] or of an accessory Kvβ subunit [Rettig, 94] binds to a ball receptor near the inner entrance of the pore [Isacoff, 91] thereby preventing ion flux through the open channel. The fast N-type inactivation of the Shaker channels is followed by a slower C-type inactivation, from which the channels recover slowly [Hoshi, 90].

A number of proteins have been discovered recently that have been shown to interact with and modify function of Kv-α proteins, including β-subunits (Kvβs), K⁺-channel Interacting Proteins (KChIPs), dipeptidyl aminopeptidase-like proteins (DPPX or DPP10), frequenin, postsynaptic density protein 95 (PSD95), filamin, etc. The physiological role of many of these proteins in native channels remains to be clarified.

β-s ubunits

Kvβ-subunits are proteins that are essential components of the Kv1 subfamily of voltage-gated potassium channels and are non-enzymatic homologues of aldo-keto reductases [Campomanes, 02; Gulbis, 99; McCormack, 94]. Transient K⁺ channels, formed by Kv1.4 proteins (and by other Kv1 α-subunits), complex with β-subunits that confer fast inactivation to otherwise non-inactivating Kv1 channels [Heinemann, 96; Rettig, 94]. Furthermore, in this case, interaction of Kv1 with beta subunits slows down the recovery from inactivation [Heinemann, 95; Heinemann, 96; Serodio, 96].

Another role assigned to the β-subunits is to act as chaperones during channel biosynthesis [Shi, 96] and thus to increase expression levels, an effect first described for the interaction of Kvβ2 with Kv1.4 [McCormack, 95]. 

K ⁺ -channel Interacting Proteins (KChIPs)

Potassium channel interacting proteins (KChIPs) were found to co-immunoprecipitate and co-immunolocalize with Kv4 α-subunits in brain and heart [An, 00]. All KChIP subunits possess a high sequence homology region to neuronal calcium sensor-1 (NCS-1; frequenin) and calsenilin/DREAM, which belong to the superfamily of EF-hand-containing proteins. Therefore, a role for cytoplasmic calcium in the regulation of Kv4 channel function has been suggested [An, 00; Weiss, 01].

 It has been demonstrated that frequenin itself is responsible for a Ca²⁺-dependent enhancement of Kv4 expression and modulation of kinetic behaviour [Nakamura, 01]. In agreement, KChIPs interact with NH₂ terminus of Kv4 proteins and enhance surface expression, thereby increasing I_A current densities when expressed in heterologous systems and in native tissues [Liss, 01; Hatano, 02; An, 00]. For example, KChIP4a delays channel opening, but when the channel opens, it favours its open state by disrupting fast inactivation and slowing channel closing [Holmqvist, 02]. In contrast, KChIP1 speeds up inactivation from closed state and accelerates channel closing [Beck, 02]. Coexpression of KChIP1 in oocytes and mammalian cells results in increased current densities, slowed onset of inactivation, and accelerated recovery from inactivation (Nakamura et al., 2001; Hatano et al, 2002). Moreover, it has been shown that a defect in the KChIP2 gene results in complete loss of transient outward current (I_to) in cardiac myocytes [Kuo, 01].

Postsynaptic density protein (PSD-95)

PSD-95, a scaffolding synapse-associated protein that possesses PDZ domains, associates with Kv4.2 and Kv1.4. It has been shown that PSD-95 influences Kv1.4 channel clustering [Hsueh, 98] and Kv4.2 channel surface expression without affecting total channel levels [Wong, 02].

Dipeptidyl peptidase-like protein (DPPX)

DPPX (also known as DPP6 or BSPL) is a glycoprotein that is structurally related to the dipeptidyl aminopeptidase and cell adhesion protein CD26, but with unknown function. DPPX is co-expressed with the principal subunits of I_A-Kv4 in a somatodendritic pattern in central nervous system (CNS) neurons. DPPX associates with the pore-forming subunit Kv4 and drastically increases their intracellular trafficking and membrane targeting [Nadal, 03].

Moreover, function reconstitution experiments in Xenopus oocytes and CHO cells demonstrated that DPPX increases the rate of inactivation of Kv4.2 currents, considerably decreases time to peak, shifts the voltage-dependence of both activation and steady-state inactivation to the left and also increases the rate of recovery from inactivation [Nadal, 03].

Molecular basis of I_K(V)

Several candidate genes exist for being the molecular determinants of the delayed rectifier potassium current in pyramidal neurons. Among them are Kv2.1, Kv2.2 and Kv1.1 [Blaine, 01]. This non-inactivating potassium current, known also as sustained potassium current, plays a major role in membrane repolarization during an action potential. Kv2 family is widespread throughout the CNS and in hippocampus, is localised on somata and dendrites of pyramidal cells and interneurones. Pharmacologically the delayed rectifier currents are sensitive to TEA and to high concentrations of 4-AP.

Structure of a Kv channel

After the cloning and expression of Kv-channel proteins it became possible to study the structure of Kv channels after cristallization and x-ray crystallography of the channel proteins. Kv potassium channels are tetramers and their monomers contain six transmembrane α-helical segments (S1-S6). An intramembrane loop between S5 and S6 (P-loop) possess specific sequence of amino acids that are responsible for potassium ions selectivity. Four subunits of voltage-gated potassium channel form the pore surrounded by integral membrane domains that can "sense" membrane voltage and open the pore in response to its change.

The "voltage sensor" (S4) features positively charged arginine residues, that enable it to move at the protein-lipid interface, within the membrane electric field, thereby allowing membrane voltage to drive the pore between closed and opened states (MacKinnon, 2003). Both, N- and C-termini are in the cytosol and play an essential role in inactivation of the channels, as well as in regulatory subunits binding.

Fig. 1 Membrane topology of a voltage gated potassium channel.

Scheme of a Kv monomer. The six tansmembrane segments are shown in yellow (S1-6). A T1 recognition domain is indicated in green. Charges (+ and -) are indicated for some of the residues in the transmembrane domains of the voltage sensor (S1-4). The pore region includes S5-S6 intermembrane loop (Deutsch, 2003). Inset: Macrocomplex of Kv channel assemble with auxiliary subunits (dark blue). T1 domains associate with beta subunits. For simplicity the C termini are not shown. (Gulbis et al., 2000).

In neurons, a receptor-dependent event, leading to Ca²⁺-influx or release of Ca²⁺ from intracellular stores, is required for the brain lipases to release arachidonate from the phospholipids of the cell membrane. Several neuromodulators stimulate the deacylation of membrane phospholipids, causing release of free arachidonate. These include excitatory amino acids (e.g. glutamate), biogenic amines (e.g. serotonin and histamine), and peptides (e.g. bradykinin). Even though the final effect of these various substances on arachidonate turnover is similar, they may use different mechanisms to achieve it.

At least three distinct phospholipases are thought to generate free arachidonic acid, either directly (PLA₂) or indirectly (PLC and PLD). A number of studies have shown that all phospholipases are activated by neurotransmitters. Previous reports indicate that the key enzyme responsible for agonist-induced AA release is cytosolic PLA₂ (cPLA₂) [Lin, 92; Roshak, 94]. cPLA₂ is a cytosolic 85-kDa Ca^{2+ -}dependent phospholipase and is activated by both an increase in intracellular free Ca^{2+ -}concentration ([Ca^{2+ -}]i) and Ser-505 phosphorylation by mitogen-activated protein kinase (MAPK) or protein kinase C [Leslie, 97]. Hormones and growth factors also regulate PLA₂ activity [Loo, 97], [Trevisi, 02; Leslie, 04]. In addition, H₂O₂ dose-dependently enhances cell membrane associated PLA₂ activity and stimulates AA-release [Chakraborti, 93; Yasuda, 99]. It was also suggested that H₂O₂ stimulates PLA₂ through PKC [Chakraborti, 93].

Fig. 3 Simplified scheme of arachidonic acid release events.

IP3, inositol triphosphate, PLC, phospholipase C, PLA2 phospholipase A2, MAG, monoacyl glycerol DAG, diacylglycerol G, GTP-coupled protein, PIP2, phosphoinositol biphosphate

Most researchers believe that a G protein ensures the coupling of receptors with PLA₂. Jelsema and Axelrod [Jelsema, 87], have first to demonstrate inhibition of PLA₂ by G proteins.

Arachidonic acid metabolism 

The major pathways of arachidonic acid metabolism have been discovered in most animal tissues, including brain. This pathways are controlled by lipoxygenase (LOX), cyclooxygenase (COX), and cytochrome (Cyt) P450 [Nishiyama, 92; Nishiyama, 93]. AA is converted into a large number of biologically active metabolites such as leukotrienes, lipoxins, prostaglandins, and thromboxanes, termed with the common name eicosanoids . These metabolites seem to play significant roles in several important processes, including vascular contraction and cell growth [Gong, 95; Anderson, 97].

In the brain, for example, 12-lipoxygenase products were shown to inhibit glutamate release from hippocampal mossy fiber nerve endings [Freeman, 91], whereas 5-lipoxygenase metabolites were found to increase the activity of muscarine-inactivated M-K⁺ channels in rat hippocampal CA1 neurons [Schweitzer, 90]. Some lipoxygenase metabolites of AA also activate the cardiac, muscarinic-activated K⁺ channel, stimulate BK_Ca channels in rat pituitary tumor cells [Duerson, 96], and modulate S-type K⁺ channels in Aplysia [Piomelli, 87]. K⁺ channel modulation by lipoxygenase products has also been reported in a number of non-neural cells, including heart myocytes [Kim, 90]. 12-Hydroxyeicosatetraenoic acid (12-HETE) is a neuromodulator that is synthesized during ischemia. Its neuronal effects include attenuation of calcium influx and glutamate release as well as inhibition of AMPA receptor (AMPA-R) activation. 12-HETE reduces ischemic injury in the heart, but it can also reduce neuronal excitotoxicity. 12-HETE could protect neurons from excitotoxicity by activating a G_i/o-protein-coupled receptor, which limits calcium influx through voltage-gated channels [Hampson, 02]. 

Fig. 4 Simplified scheme of arachidonic acid metabolism. 

LOX, lipooxigenase; COX, cyclo-oxigenase; CytP450, cytochrome; HPETE, hydroperoxyeicosatrienols, HETE, hydroxyleicosatrienols; EETs, epoxyeicosatrienoics

The eicosanoids produce a wide range of biological effects on inflammatory responses, on the intensity and duration of pain and fever [Samad, 01; Vane, 76], and on reproductive function [Zahradnik, 92]. Eicosanoids also play important roles in acid secretion [Eberhart, 95], regulating blood pressure through vasodilation [Pomposiello, 01] or vasoconstriction [Yu, 03], and inhibiting [Petroni, 95] or activating [Davi, 99] platelet aggregation and thrombosis. 

Modulation of voltage-gated potassium channels by arachidonic acid

AA and its metabolic products have been shown to modulate a large number of ligand- and voltage-gated ion channels in a variety of systems [Bevan, 87; Ordway, 91]. The potential role of arachidonic acid in mediating K⁺-channel modulation and presynaptic inhibition of neurotransmitter release-one example of a second messenger role for the eicosanoids-was first suggested by J. Schwartz , based on experiments with Aplysia. AA has been shown to activate a large conductance (160 pS) K⁺-channel directly in cardiac atrial muscle [Kim, 89] and a small conductance (23 pS) K⁺-channel in smooth muscle [Ordway, 91]. In central neurons, AA either depresses or enhances K⁺-currents through lipoxygenase or cyclooxygenase metabolites [Keyser, 90; Schweitzer, 90; Zona, 93]. With respect to K⁺-channels in expression systems, AA has been shown to inhibit currents directly through channels formed by members of the Kv4 (Shal) subfamily of voltage-dependent potassium channels, whereas other members of Kv1 (Shaker) subfamilies were relatively insensitive to AA [Villarroel, 96].

High concentrations of arachidonic acid (#SYMBOL#1µM) directly modulate I_A in CA1 hippocampal neurons [Colbert, 99; Keros, 97]. Bittner and Müller showed that intracellular AA is highly potent in selectively inhibiting the A-current in cultured hippocampal neurons. Our group recently demonstrated, that extremely low concentration of AA (1 pM) attenuates I_A, but not the delayed rectifier, in CA1 pyramidal neurons from acute brain slices [Angelova, 06].