Ion channel genes and human neurological disease: Recent progress, prospects, and challenges

doi:10.1073/pnas.96.9.4759

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Ion channel genes and human neurological disease: Recent progress, prospects, and challenges

Edward C. Cooper^* and Lily Yeh Jan^,

Departments of ^* Neurology, and Physiology, Biochemistry, and Howard Hughes Medical Institute, University of California, San Francisco, CA 94143

Contributed by Lily Yeh Jan, December 31, 1998

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What do epilepsy, migraine headache, deafness, episodic ataxia, periodic paralysis, malignant hyperthermia, and generalizedmyotonia have in common? These human neurological disorders canbe caused by mutations in genes for ion channels. Many of thechannel diseases are "paroxysmal disorders" whose principal symptomsoccur intermittently in individuals who otherwise may be healthyand active. Some of the ion channels that cause human neurologicaldisease are old acquaintances previously cloned and extensivelystudied by channel specialists. In other cases, however, disease-genehunts have led the way to the identification of new channel genes.Progress in the study of ion channels has made it possible toanalyze the effects of human neurological disease-causing channelmutations at the level of the single channel, the subcellulardomain, the neuronal network, and the behavingorganism.

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Some of the most thrilling moments in science occur when workers from distinct disciplines converge on questions of newlyrecognized mutual interest. Recent publications build on one suchconvergence, between clinical neurology, human genetics, and ionchannel studies (1-11). Clinicians and geneticists seeking thecauses of neurological disorders have mapped chromosomal locifor hereditary diseases and have found at these loci both previouslyunknown channel genes and pathogenic mutations in known channelgenes. This work has proceeded rapidly. The first ion channeldisease mutations, associated with hyperkalemic periodic paralysis,were identified in 1991; now the list includes hundreds of diseasealleles responsible for more than 20 nerve and muscle disorders(Table 1). In the meantime, advances in many disciplines, includingelectrophysiology, cell biology, genomics, neuroanatomy, and structuralbiology have deepened our understanding of how ion channels functionat the molecular and cellular level. It is now possible to beginto understand how channel gene mutations cause particular typesof neurological symptoms. Here, we provide an update on some ofthe progress in ion channel studies. Then, because disorders causingabnormalities in skeletal muscle contraction remain the best understoodof the human ion channel diseases, we briefly will review whathas been learned about the biology and treatment of these disorders.This survey allows us to introduce concepts that are importantin considering some very recent discoveries linking channel mutationswith disorders of the central nervous system (1-11).

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Table 1. Nerve and muscle diseases caused by mutations in ion channel genes

Ion Channels and Cellular Excitability

All cells maintain concentration gradients for inorganic ions between their interior and exterior. Typically, potassium ionis at higher concentration in cytoplasm than in extracellularfluid; sodium, chloride, and calcium ions exhibit the oppositedistribution. These gradients make possible a system for electricalsignaling based on the activity of ion channel proteins embeddedin the cell membrane (35). Ion channels form pores that allowions to move rapidly through cell membranes down their electrochemicalgradients. Channels transport ions at rates of 1,000,000 to 100,000,000ions per sec. This flow of ions creates electrical current onthe order of 10¹² to 10¹⁰ amperes per channel. Such currents are large enough to producerapid changes in the membrane potential, the electrical potentialdifference between the cell interior and exterior. Because calciumand sodium ions are at higher concentration extracellularly thanintracellularly, openings of calcium and sodium channels causethese cations to enter the cell and depolarize the membrane potential.For analogous reasons, when potassium leaves or chloride entersthe cell through open channels, the cell interior becomes morenegative, orhyperpolarized.

Most ion channels are gated $---$ capable of making transitions between conducting and nonconducting conformations. Channel gatingcan be induced by extracellular ligands, intracellular secondmessengers and metabolites, protein-protein interactions, phosphorylation,and other factors. In addition, many ion channels are gated byanother regulatory signal $---$ the membrane potential itself. Voltage-gatedion channels respond to and modify the changes in membrane potentialproduced by the binding of neurotransmitters to ligand-gated ionchannels atsynapses.

Ion channels colocalized in discrete subcellular compartments function together as signaling elements in excitable cells.These elements amplify weak signals, determine thresholds, propagatesignals to other regions of the cell, and generate membrane potentialoscillations, among other functions. Physiologists study the channelsof tiny neuronal subcellular regions, such as dendrites, axons,and presynaptic terminals, by using refined methods that combinethe patch-clamp with sophisticated imaging techniques (36).Such experiments show, for example, that the membranes of dendritescontain unexpectedly high numbers of voltage-gated channels. Asa result, signal processing in dendrites now seems to be moredynamic and complex than previously thought (37-39). Potassiumchannels located in patches along the lengths of central axonsmay allow differential control of signal propagation into particularaxonal branches (40). Presynaptic terminals possess a varietyof voltage-gated channels and G-protein linked receptors regulatingthe last steps leading to neurotransmitter release (41, 42).Anatomists have found that the channels underlying these signalingfunctions are localized with extraordinary precision. It seemsthat axons, dendrites, presynaptic terminals, and postsynapticspines all contain a rather large number of distinct microdomains(e.g., subsynaptic, perisynaptic, nonsynaptic) and that the localizationof channels and other signaling proteins respects these borders(43-46). Protein-protein interactions between channels, multivalentscaffolding proteins, and the cytoskeleton appear to control thespatial organization of channels in these microdomains (47).

Molecular cloning has revealed a large number of channel genes. This expansion began early in evolution. The genome of thenematode Caenorhabditis elegans contains about 80 potassium channelgenes, 90 ligand-gated channel genes, five voltage-gated calciumchannel genes, six cyclic nucleotide-gated channel genes, andsix chloride channel genes (48). These statistics do not includethe many channel auxiliary subunits, that, though incapable offorming pores themselves, nonetheless make important contributionsto channel function (49, 50). Homologues of a large portionof the worm channel genes already have been found inmammals.

Why are there so many different channel genes? We suspect that the large number of channels reflects a diversity of specificsignaling needs. This point is illustrated by recent studies ofthe neurons in the inner ear. Sound vibrations cause specializedsensory neurons in the cochlea (called hair cells) to depolarizerepetitively and release their neurotransmitter. Hair cells thatrespond optimally to different sound frequencies are arrangedsequentially along the length of the cochlea, like piano keys.The optimal frequency of each hair cell depends largely on thekinetics of a calcium-activated potassium channel, Slo, that causeshyperpolarization and counters the depolarization caused by theopening of voltage-gated calcium channels (51). Alternativeexon usage in Slo genes allows expression of a large number ofdistinct Slo channels, with differing gating kinetics $---$ these channelsare differentially expressed along the length of the cochlea,resulting in cells that oscillate at varying frequencies (52-54).The rules governing signaling between and within neurons in thecentral nervous system, though poorly understood, are likely tobe as complex as within the cochlea, and also may rely on differentialexpression and localization of channels with distinctive properties.Analysis of mutations is an important approach for identifyingtheserules.

Ion Channel Disorders of the Motor Nerve and Skeletal Muscle

The importance of the specific properties of individual channel types for cellular excitability and behavior is best understoodfor the neuromuscular synapse that transmits signals from themotor nerve to the skeletal muscle. The axons of spinal motorneurons exit the spinal column and make their way to the muscle,where they form contacts with individual muscle fibers. Ion channelsplay crucial roles in the passage of signals along the nerve andfrom the muscle surface to the contractile machinery within (Fig.1). The signal that travels down the axon, the action potential,results from the sequential opening of voltage-gated sodium channels(that allow external sodium to enter and depolarize the membranepotential) and potassium channels (that allow potassium to exitthe cell, causing repolarization). Arrival of the action potentialat the nerve terminal activates voltage-gated calcium channels,allowing calcium to enter the terminal, causing neurotransmitterrelease into the synaptic cleft. The released neurotransmitter,acetylcholine, binds to nicotinic acetylcholine receptors, whichare ligand-gated cation channels, causing sodium to enter anddepolarize the muscle cell membrane at synaptic sites where theseacetylcholine receptors are clustered. This local depolarizationleads to the activation of nearby voltage-gated sodium channels,which spread action potentials across the surface of the musclefiber and into special invaginations of the plasma membrane, thetransverse tubules, where calcium channels are present at highdensity. T-tubule calcium channels are physically associated withthe calcium release channels embedded in the closely apposed membranesof the sarcoplasmic reticulum. The invading action potential causesthe T-tubule calcium channels to undergo conformational changesthat are relayed to the associated sarcoplasmic reticulum calciumchannels, causing them to open. Calcium ions from within the sarcoplasmicreticulum flow into the cytoplasm, leading to muscle contraction.Chloride channels located on the T-tubule and muscle surface thenreturn the muscle membrane potential to its resting level.

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Fig. 1. Ion channels of the motor nerve and skeletal muscle involved in human disease. The drawing shows a myelinated axon branching to form synaptic contacts with a muscle fiber. (Upper) The outer surfaces of the axon and muscle. (Lower) The nerve presynaptic terminal and muscle fiber in cut section. (Inset) A magnified view of the nerve fiber, cut lengthwise near a node of Ranvier. Different channel types are identified by number and color, as indicated in the key below the drawing. The contractile proteins of the sarcomere are depicted schematically within the muscle. See text for additional details.

Remarkably, mutations of most of these key channel molecules have been found to cause human neuromuscular disorders. The distinctclinical syndromes can in many cases be understood based on thespecific alterations the mutations produce in channel activity[Fig. 1, see recent reviews (55-59) for additional details andreferences]. Reducing the activity of potassium channels in thenerve fiber delays action potential repolarization and lowersthe amount of excitation needed to produce action potentials.Potassium channel mutations with these effects underlie hereditaryforms of myokymia, a spontaneous, involuntary rippling movementof skeletal muscle based on abnormal spontaneous action potentialgeneration within the peripheral nerve. A large number of differentmutations in genes encoding subunits of the acetylcholine receptorcause congenital myesthenic syndromes, disorders associated withmuscle weakness and fatigue. Electrophysiological study has revealedthat some of these acetylcholine receptor mutations reduce thenumber of channels at the cell surface, whereas others alter therate channels open and close, cause spontaneous openings in theabsense of neurotransmitter, or reduce the affinity of receptorsforacetylcholine.

Mutations in the pore-forming subunits of sodium channels and chloride channels cause myotonia, a muscle abnormality in whichrelaxation after voluntary contraction is markedly delayed. Myotonicmuscles recorded in vivo exhibit abnormal spontaneous oscillationsin membrane potential, called myotonic discharges. What underliesthese spontaneous oscillations? In normal muscle, depolarizationof the postsynaptic membrane causes brief openings of sodium channelsthat take place within the first few msec after membrane depolarization.As these sodium channel openings subside, chloride enters thecell through more slowly opening chloride channels, promptly returningthe membrane potential to its resting level. Sodium channels harboringmutations causing myotonia exhibit an abnormal tendency to openlater or more persistently after membrane depolarization. Residualsodium entry through these abnormal channels repeatedly reinitiatesthe cycle of membrane depolarization. Chloride channel mutationscausing myotonia reduce the amount of chloride ion that can enterthe cell to repolarize the membrane, leading tooscillations.

Mutations in muscle sodium and calcium channels cause forms of periodic paralysis, disorders associated with episodes of weaknesslasting hours to days at a time. The sodium channel mutants exhibitabnormal, long-lasting currents. The resulting prolonged membranedepolarization causes a portion of the sodium channels to entera desensitized or inactivated state, leading to membrane inexcitability.The molecular mechanism underlying calcium channel-associatedperiodic paralysis is less clear and awaits additionalstudy.

Mutations in the sarcoplasmic calcium release channel cause malignant hyperthermia. Attacks often are provoked by generalanesthesia. During the attack, the calcium release channel openspersistently, causing sustained muscle contraction, fever, andmuscle injury. Mutations in T-tubule calcium channel and musclesodium channel are less common causes of malignanthyperthermia.

Insight into the molecular basis of these disorders has allowed for a more rational approach to therapy. In forms of the myesthenicsyndrome where acetylcholine receptor openings are prolonged,receptor blockers are useful; where mutations cause reductionsin the opening probability of the receptors, acetylcholinesteraseinhibitors that increase the lifetime of released acetylcholineand potassium channel blockers that promote transmitter releaseare of benefit. Sodium channel myotonias can be treated with "use-dependent"blockers of these channels that selectively inhibit the abnormallate openings of these mutantchannels.

Ion Channel Disorders in the Central Nervous System

From this brief overview of channel mutations that affect signaling from motor nerve to muscle, a model system for synaptictransmission, we can appreciate how different ion channels workin a pathway to execute a command from the nervous system. Similarprinciples are used by neurons in the brain to process and integratesignals, although the network of neurons is far more complex.One lesson likely to be of general validity is that prolongedor excessive excitation may result from sodium channel mutationsthat cause recurrent channel openings, or potassium or chloridechannel mutations that reduce channelactivity.

We will discuss three areas where very recent progress has linked human central nervous system disorders with mutations involtage-gated sodium and potassium channels: (i) the associationof the epileptic syndrome, generalized epilepsy with febrile seizuresplus, with a mutation in a neuronal sodium channel, (ii) the identificationof genes causing benign neonatal familial convulsions, a generalizedepilepsy, as the genes underlying an extensively studied potassiumchannel (the M-channel), and (iii) the characterization of possiblecellular mechanisms underlying episodic ataxia with myokymia,another potassium channel disorder, by using animal models. Recentreviews (58, 60) and citations included in Table 1 provideadditional discussion and references concerning other centralnervous system channeldiseases.

Altered Sodium Channel Function Is a Cause of Epilepsy

Epileptic seizures are behavioral attacks resulting from the overly synchronized and excessive activity of large groups ofbrain neurons. Symptoms vary widely, depending on the region andextent of the brain that participates in the abnormal electricalactivity, but may include alterations or loss of consciousness,sustained or rhythmic muscle contraction, stereotyped gesturalmovements, and visual or somatosensory hallucinations. Epilepsyis present in about 1% of the general population and is more frequentduring childhood (61). About 5-7% of children will have a seizureduring the first 5 years of life; about half of these will beprovoked by acute febrile illness. It has remained unclear whyfever provokes seizures in some individuals during childhood,but not later in life. The febrile seizure trait exhibits a complexpattern of inheritance, suggesting the involvement of multiplegeneticfactors.

Sheaffer and Berkovic (4) recently described an extraordinary family in which numerous members experienced both febrileand nonfebrile seizures, a syndrome they termed generalized epilepsywith febrile seizures plus. In one branch of the family, consistingof 60 individuals in five generations, 23 were epileptic. Thefamily was descended from early English settlers of a remote areaof Australia. In the first years after immigration, marriage betweenclose relatives sometimes occurred. Among the direct ancestorsof this family, such consanguinous marriage occurred in threesuccessive generations. This unusually homogeneous genetic backgroundleft later generations at risk for disorders that may result fromthe activity of weakly penetrant disease alleles. Mulley and colleagues(5) obtained evidence linking epilepsy in this family to aregion on chromosome 19. They evaluated candidate genes previouslylocalized to this region, including SCN1B, the $beta$ 1 auxilliary subunitof the voltage-gated sodium channel (5). The SCN1B genes ofepileptic individuals in the family contained a single base- pairsubstitution, causing a single amino acid change in the proteinsequence.

Previous structural and functional studies of the sodium channel are helpful in assessing the significance of this mutation(49, 62-65). Sodium channels in mammalian brain, heart, and skeletalmuscle contain pore-forming $alpha$ subunits and $beta$ 1 subunits associatedin 1:1 stoichiometry. The $beta$ 1 subunit has important effects onthe gating of the channel, hastening the rates at which it opensand closes (49, 62-64). The $beta$ 1 subunit is a membrane protein,with a small intracellular domain, a single transmembrane segment,and a large extracellular domain. The extracellular domain hasa structure that is homologous to members of the Ig fold superfamily.Mutant $beta$ 1 subunits with alanine substitutions at positions expectedto disrupt the Ig fold lack the ability to modify channel gatingproperties (65). The mutation discovered by Mulley and colleagues(5) substitutes a tryptophan residue for a conserved cysteinethat normally forms a disulfide bridge to stabilize the Ig folddomain. This mutation appears to result in loss of function $---$ cellsexpressing the mutant exhibited slow channel openings and closingsindistinguishable from those expressing $alpha$ subunits alone (5).

As discussed above, the mutations in skeletal muscle sodium channel $alpha$ subunits causing myotonia and periodic paralysis alsoresult in the expression of channels that exhibit delayed andprolonged openings (57). Furthermore, mutations in the $alpha$ subunitof the heart sodium channel gene, linked to the long QT syndromeand idiopathic ventricular fibrillation (forms of cardiac arrhythmiathat cause sudden death), are associated with similar changesin channel gating (33, 34). The basis for these gating abnormalitieshas been revealed by single channel studies. It appears that normalsodium channels possess two distinct gating modes. The predominantmode is associated with brief openings occurring within the firstfew milliseconds after the membrane is depolarized. In the other,rarely occupied mode, channel openings are prolonged and may occurafter many milliseconds of delay. In the sodium channel diseasesso far studied, channels exhibit an increased tendency to enterthe second gating mode associated with long, late openings. Thesodium channel diseases, of muscle, heart, and now, brain, suggestone way in which ion channel mutations may result in episodicsymptoms $---$ -through selective changes in the characteristics ofan infrequently occupied gatingmode.

An Epilepsy Gene Hunt Leads to Genes Encoding the M-Channel

As the year 1998 drew to its end, two independent, decades-long searches converged: one by geneticists seeking the cause ofanother remarkable epileptic syndrome, and the second by channelspecialists seeking to identify a key mechanism underlying cholinergicexcitation in the central and autonomic nervous system. In the1960s and 1970s, investigators reported several large familiesin which neonatal convulsions appeared to be dominantly inheritedwith high penetrance. This epileptic syndrome, benign neonatalfamilial convulsions (BNFC) (66) is an often-cited model forwhat neurologists term "idiopathic" epilepsy: affected individualsare epileptic, but have no other neurological deficits or otherorgan involvement. Recurrent, brief, generalized seizures beginon about the fourth day of life and cease after 1-3 months. Infantsotherwise grow and develop normally. However, affected personscarry a 10-16% risk of developing epilepsy again later in life.When seizures occur after infancy, they are in many instancesprovoked by sudden emotional stress or startle (66). In 1989,Leppert and colleagues (67) found linkage of the disease geneto chromosome 20. Later, Lewis et al. (68) and Steinlein andcolleagues (69) identified two families in which the BNFC syndromewas linked not to chromosome 20 but to chromosome8.

A score of years ago, electrophysiologists recording from sympathetic ganglion neurons discovered the M-channel, a voltage-gatedpotassium channel that is suppressed by muscarinic acetylcholinereceptor activity (70). M-channels open occasionally at theresting membrane potential and are slowly activated by membranedepolarization. Because of these slow kinetics, M-channel activationcauses a delayed membrane hyperpolarization after a cell receivesexcitatory input. As a result, sympathetic neurons expressinglarge amounts of M-channels tend to fire one action potentialafter receiving excitatory input, then become transiently quiescent.Inhibition of the M-channel causes these neurons to become slightlydepolarized and to fire multiple action potentials rhythmicallyafter receiving excitatoryinputs.

M-channels were later found in central neurons in the brain and the spinal cord (71). Besides acetylcholine, peptide transmitterssuch as luteinizing hormone-releasing hormone, substance P, andbradykinin also inhibit the M-channel, thereby increasing neuronalexcitability (71). Although receptors that mediate the actionof these transmitters are known to activate the GTP binding proteinG_q/11 (72), the intracellular second messenger mobilized bythe muscarinic acetylcholine receptor to suppress the M-channelhas remained elusive (73, 74).

The action of acetylcholine on central neurons is of considerable interest because of its importance in cognition. Cholinergicneurons in the mammalian brain integrate inputs from subcorticalregions such as the hypothalamus and midbrain and modulate neuronsin the cortex, hippocampus, and other brain regions. Lesion ofthese cholinergic neurons impairs attention, alertness, learning,and memory; these defects can be reduced by cholinergic drugs(75). The loss of cognitive function in Alzheimer's diseaseis correlated with a marked reduction of central cholinergic neurons.Acetylcholinesterase inhibitors, which increase the lifetime ofacetylcholine that is released from remaining cholinergic neurons,improve the cognitive performance of patients in early stagesof the disease (76). In the course of developing other pharmacologicalreagents as potential treatments of Alzheimer's disease, researchersin the DuPont Merck Research Laboratories found that linopirdineboth improves learning and memory in laboratory animals and enhancesacetylcholine release because of its action on a potassium channel(77, 78). The most potent action of this drug in hippocampaland sympathetic neurons is the inhibition of the M-channel (79,80).

The involvement of acetylcholine and the M-channel in controlling neuronal excitability is further underscored in an rodentmodel of epilepsy. Systemic administration of the muscarinic agonistpilocarpine potently causes acute status epilepticus and inducesa chronic seizure phenotype reminiscent of human temporal lobeepilepsy (81). These effects are abolished in heterozygous orhomozygous mutant mice lacking half or all of the forebrain m1muscarinic acetylcholine receptors (82). Mutant mice lackingm1 receptors also fail to exhibit suppression of the M-channelwhen their sympathetic neurons are exposed to cholinergic agoniststhat activate muscarinic acetylcholine receptors (82), raisingthe question whether excessive muscarinic acetylcholine receptor-mediatedsuppression of the M-channel in central neurons might be a causeof epileptic seizures. Because of the M-channel's key importancein controlling repetitive firing in many neurons (71), its extensiveand potentially novel mechanisms of regulation (72-74), and itspossible contributions to normal cognitive function, dementia,and epilepsy, the identification of genes for the M-channel hasbeen eagerlyawaited.

The searches for genes for benign neonatal familial convulsions (BNFC) and the M-channel ended with a surprise. The two BNFCgenes on chromosome 20 and 8 encode highly homologous potassiumchannel subunits, KCNQ2 and KCNQ3 (1-3). Expression of eithergene alone in Xenopus oocytes results in only small currents,but expression of the two genes together results in currents thatare 10-50 times larger (7, 83). The channels resulting fromKCNQ2 and KCNQ3 coexpression exhibit gating properties and linopirdinesensitivity similar to those of neuronal M-channels (6). Insitu hybridization and Northern blotting experiments show thatKCNQ2 and KCNQ3 mRNA are expressed in overlapping patterns inbrain and sympathetic ganglia (6, 7). These data suggestthat KCNQ2 and KCNQ3 coassemble in vivo to form the M-channel.Disease-causing missense mutations in KCNQ2 and KCNQ3 are associatedwith only modest reductions (20-30%) in current magnitude (7).This finding suggests that symptoms are not the result of toxicgain-of-function or dominant-negative activity, but rather, ofa critical dependence of neuronal excitability on the absolutemagnitude of KCNQ2/KCNQ3 potassium channelactivity.

KCNQ2 and KCNQ3 are relatives of another channel, KCNQ1, which previously was shown to be mutated in long QT syndrome andin Jervell and Lange-Neilson syndrome, a recessive disorder characterizedby a congenital bilateral deafness associated with the long QTsyndrome (18, 31, 84). Recently, another member of the KCNQpotassium channel subfamily, KCNQ4, was identified as a causeof a dominantly inherited form of childhood-onset deafness (8).KCNQ1 and KCNQ4 both are expressed in the inner ear, but in differentcell types. KCNQ1 is expressed, as a complex with a small auxiliarysubunit called KCNE1, in the cells of a specialized endothelium,the stria vascularis. The stria is responsible for secretion ofendolymph, the potassium-rich fluid that fills the middle chamberof the cochlea and baths the sound-receptive hair cells. In Jervelland Lange-Neilson syndrome, endolymph secretion does not occurnormally, the middle chamber of the cochlea collapses, and haircells degenerate. In contrast, KCNQ4 is expressed in outer haircells. The outer hair cells function to increase the sensitivityof sound perception by mechanically amplifying sound vibrationswithin the cochlea. The specific cellular roles of KCNQ1 and KCNQ4channels in the stria and the outer hair cells remain to be determined.It is noteworthy that KCNQ4 appears to form heterooligomeric channelswhen coexpressed with KCNQ3, but not with KCNQ2, KCNQ1, or KCNE1.Thus, three different heterooligomeric KCNQ channels are likelyexpressed in different cell types. Mutations in each of the genescontributing to these channels have been shown to cause humandisease (Fig. 2).

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Fig. 2. The KCNQ family of voltage-gated potassium channels. Four pore-forming subunit genes (KCNQ1-4) and one small auxiliary subunit gene (KCNE1) are known.

Episodic Ataxia Type 1 (EA-1), Shaker Flies, and Epileptic Mice

How might the identification of culprit channel genes bearing mutations lead to mechanistic understanding of the resultingneurological diseases? Recent studies related to the pathogenesisof EA-1 are instructive. EA-1 is a dominantly inherited disorderinvolving both the brain and peripheral nerves (85, 86). Patientsexperience recurrent attacks of unsteady gait and loss of limbcoordination lasting minutes to hours. This phenotype suggestsan intermittent derangement of cerebellar function. In some cases,transient cognitive deficits accompany the motor symptoms. Attacksmay be provoked by a sudden stress or startle. Myokymia, discussedabove, is continuously present in many EA-1 patients. This myokymiais unaffected by pharmacological block at the proximal portionof peripheral nerves, but is reduced by distal nerve block andabolished by inhibition of neuromuscular transmission. This observationsuggests that, unlike myotonia or epilepsy, myokymia results fromabnormal hyperactivity in the peripheralnerve.

In 1994, Litt and colleagues (12) linked EA-1 to missense mutations in KCNA1, a voltage-gated potassium channel gene. KCNA1is a mammalian homologue of the fly gene Shaker. Adult Shakerflies exhibit abnormal limb shaking when anesthetized with ether.Shaker larvae showed abnormal hyperexcitability of the motor nerveterminals (87). Shaker and its mammalian homologues are amongthe most extensively studied of cloned ion channels (88).

Extensive further work, including physiological studies of the mutant channels, anatomical studies of KCNA channel localizationin the central nervous system and peripheral nerve, and studiesof kcna1 knockout mice, gives useful clues for understanding thebasis of the EA-1 phenotype. By using specific antibodies, researchersfound that kcna1 is localized to a key site regulating cerebellaroutput $---$ the axons and nerve terminals of the basket cells thatmake inhibitory synaptic contacts on the proximal segment of thepurkinje cell axon (44, 89). Patch-clamp recordings of basketcell terminals made in cerebellar slices revealed an extraordinarilyhigh potassium channel density, in excess of 1,000 channels perµm² (90). Block of these kcna channels with $alpha$ -dendrotoxin causesdramatic increases in the spontaneous inhibitory postsynapticpotentials recorded in purkinje cells, suggesting that kcna regulatesthe excitability of the basket cell presynaptic terminals (90).Kcna channels also are concentrated at the juxtaparanodal regionsof myelinated axons. In these regions that flank the nodes ofRanvier (see Fig. 1, Inset) the kcna channel appears to stabilizethe resting membrane potential, possibly preventing aberrant actionpotential generation that may result in myokymia (89, 91,92).

Because studies in Xenopus oocytes indicate that the mutations causing EA-1 result in reductions in KCNA1 expression and currentmagnitude (93, 94), knockout mice lacking the murine homologueof KCNA1 may provide a useful animal model for EA-1. Tempel andcolleagues (11) have generated kcna1 knockout mice. Interestingly,mice heterozygous for the null allele appear normal; homozygousmutants have very frequent generalized epileptic seizures (11).The homozygous mutant mice also exhibit a mild loss of coordinationunder normal conditions and attacks of tremulousness and markedataxia after cold-temperature stress (9). Physiological studiesof these mice reveal presynaptic hyperexcitability at both theneuromuscular and cerebellar basket cell synapses (9, 10).

Prospects

Molecular studies of ion channels, begun a generation ago, have revealed a remarkable diversity of channel genes. The impendingcompletion of genome projects in several model organisms as wellas humans probably signals the end of the cloning era as previouslypracticed. However, the characterization of the products of thechannel genes, and of the channel mutations that cause brain diseases,has in many ways only begun. As we have discussed, the channeldisorders of the neuromuscular synapse illustrate how a largevariety of disease phenotypes may result from mutations in channelsfunctioning together at a single anatomical site. In the brain,a far greater variety of channels are expressed, and the rolesplayed by specific channels are, for the most part, poorly understood.Yet, studies of the first few brain channel disorders indicatethat subtle changes in the electrophysiological properties ofa single channel type can have important effects onbehavior.

A challenge that awaits us is to more comprehensively analyze the contributions made by a large number of the channel genesat the cellular and neuronal network level. The importance ofmouse genetic models for this work is widely appreciated and willgrow. It is noteworthy that studies of inbred lines of mice withepilepsy, cerebellar deficits, and other neurological abnormalities,also have resulted in the cloning of channel alleles (60, 95).Besides these spontaneous mutations, targeted mutation of severaldifferent channel genes also have been shown to cause neurologicalphenotypes, including epilepsy (96). As illustrated by the studiesof kcna1 knockout mice already completed, these animal modelsmake possible efforts to unravel the functions of particular channelgenes through parallel studies at the molecular, cellular, neuronalnetwork, and behaviorallevels.

While neurobiologists illuminate the links between individual channel genes and behavior, structural biologists and pharmacologistswill characterize in new detail the molecular contours of thedifferent channel proteins and identify compounds that modifythe activity of individual channel types with greater specificity.In 1998, this effort entered a period of accelerating progress.The structure of a bacterial potassium channel was solved by x-raycrystallography (97), and the structures of components of eukaryoticchannels responsible for inactivation and deactivation gating(98, 99), subunit association (100), and ligand binding (101)also weredetermined.

As genomic tools become more powerful, it also may be possible to identify the important channel gene polymorphisms in humanpopulations and to correlate particular alleles with more common,genetically complex forms of epilepsy and other traits. In thenematode C. elegans, a naturally occurring polymorphism in a Gprotein-coupled receptor has been shown to underlie the preferenceof different individuals for solitary or social living (102).A comprehensive analysis of the properties of naturally occurringhuman channel variants and their influence over behavior likelywill deepen our understanding of nervous systemfunction.

	ACKNOWLEDGEMENTS

We thank members of the Jan laboratory, PNAS reviewers, and Drs. B. Schwappach, R. B. Layzer and J. C. Jen for helpful comments,and Wendy Hiller Gee for illustrations. E.C.C. was supported byThe Parke-Davis Young Investigator Award in Epilepsy Researchfrom the American Academy of Neurology Education and ResearchFoundation and by the National Institutes of Health. L.Y.J. wassupported by the National Institutes of Health and is an Investigatorof the Howard Hughes MedicalInstitute.

	ABBREVIATION

EA-1, episodic ataxia type 1.

	FOOTNOTES

To whom reprint requests should be addressed at: Box 0725, Howard Hughes Medical Institute, University of California, SanFrancisco, CA 94143. e-mail: gkw{at}itsa.ucsf.edu.

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Review Ion channel genes and human neurological disease: Recent progress, prospects, and challenges

Review
Ion channel genes and human neurological disease: Recent progress, prospects, and challenges