Genetic Analysis of a Synaptic Calcium Channel in Drosophila: Intragenic Modifiers of a Temperature-Sensitive Paralytic Mutant of cacophony

Genetic Analysis of a Synaptic Calcium Channel in Drosophila: Intragenic Modifiers of a Temperature-Sensitive Paralytic Mutant of cacophony

I. M. Brooks^a, R. Felling^a, F. Kawasaki^a, and R. W. Ordway^a
^a Department of Biology, The Pennsylvania State University, University Park, Pennsylvania 16802

Corresponding author: R. W. Ordway, 208 Mueller Laboratory, Pennsylvania State University, University Park, PA 16802., rwo4{at}psu.edu (E-mail)

Communicating editor: T. C. KAUFMAN

ABSTRACT

TOP
ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

Our previous genetic analysis of synaptic mechanisms in Drosophilaidentified a temperature-sensitive paralytic mutant of the voltage-gatedcalcium channel ${alpha}$ 1 subunit gene, cacophony (cac). Electrophysiologicalstudies in this mutant, designated cac^TS2, indicated cac encodesa primary calcium channel ${alpha}$ 1 subunit functioning in neurotransmitterrelease. To further examine the functions and interactions ofcac-encoded calcium channels, a genetic screen was performedto isolate new mutations that modify the cac^TS2 paralytic phenotype.The screen recovered 10 mutations that enhance or suppress cac^TS2,including second-site mutations in cac (intragenic modifiers)as well as mutations mapping to other genes (extragenic modifiers).Here we report molecular characterization of three intragenicmodifiers and examine the consequences of these mutations fortemperature-sensitive behavior, synaptic function, and processingof cac pre-mRNAs. These mutations may further define the structuralbasis of calcium channel ${alpha}$ 1 subunit function in neurotransmitterrelease.

TRANSMISSION of electrical impulses among neurons is a fundamentalaspect of neural function. This occurs at chemical synapseswhen neurotransmitters are released from the presynaptic neuronand produce excitation or inhibition of the postsynaptic cell.Neurotransmitter release is evoked by calcium influx throughvoltage-gated calcium channels, which triggers rapid fusionof neurotransmitter-filled synaptic vesicles with the presynapticplasma membrane.

Calcium channels implicated in neurotransmitter release areheteromultimers composed of a primary structural subunit, ${alpha}$ 1,as well as accessory ß, ${alpha}$ 2- ${delta}$ , and possibly ${gamma}$ subunits(CATTERALL 1998 ). The ${alpha}$ 1 subunit consists of four homologousrepeats, each containing six transmembrane segments and an intramembranous"P loop" (Fig 1). The four repeats are joined by three majorcytoplasmic loops, which, together with the cytoplasmic N andC termini, include several protein interaction domains involvedin channel regulation (IKEDA and DUNLAP 1999 ; CATTERALL 2000). Certain structural features of the ${alpha}$ 1 subunit have been assignedspecific roles in channel function. Examples include the S4segments, which contain positively charged residues and arethought to serve as voltage sensors (HORN 2000 ), and the Ploop contributing to formation of the channel pore (Fig 1; VARADI et al. 1999 ). In vertebrates, the primary presynapticcalcium channels are of the P/Q and N types, for which the ${alpha}$ 1subunits are encoded by the ${alpha}$ 1A (Cav 2.1) and ${alpha}$ 1B (Cav 2.2) genes,respectively. Homologous calcium channel ${alpha}$ 1 subunit genes havenow been identified in a variety of organisms.

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Figure 1. Presynaptic voltage-gated calcium channel ${alpha}$ 1 subunit topology. The positively charged S4 voltage sensors (+) and the pore-forming P loops (P) are indicated. A calcium-dependent regulatory region within the C-terminal cytoplasmic tail contains consensus binding domains for calcium (EF hand) and calmodulin (IQ).

Several studies have utilized genetic approaches to examinethe in vivo functions of specific calcium channel gene productsat native synapses. In addition to work in Drosophila (see below),analysis of presynaptic calcium channels has been pursued inseveral other genetic model systems. The unc-2 gene of Caenorhabditiselegans, originally identified in a screen for mutants exhibitingaltered adaptation to neuroactive substances, encodes a homologof vertebrate presynaptic calcium channel ${alpha}$ 1 subunits (SCHAFERand KENYON 1995 ). In the mouse and human, mutations in the ${alpha}$ 1A subunit gene are associated with several inherited disorderscharacterized by ataxia and migraine as well as by altered P/Q-typechannel activity (DOVE et al. 1998 ; LORENZON et al. 1998 ; WAKAMORI et al. 1998 ; LORENZON and BEAM 2000 ; MORI et al.2000 ; PIETROBON 2002 ). In addition, knockout mice have beengenerated for all of the ${alpha}$ 1 subunit genes implicated in neurotransmitterrelease, including ${alpha}$ 1A (JUN et al. 1999 ), ${alpha}$ 1B (INO et al. 2001), and ${alpha}$ 1E (SAEGUSA et al. 2000 ). Despite this progress, a majorremaining challenge in determining the physiological roles ofthese gene products is presented by long-term compensatory changesthat may occur in null or hypomorphic mutants (JUN et al. 1999; SAEGUSA et al. 2000 ; INO et al. 2001 ; MATSUSHITA et al.2002 ; ZHANG et al. 2002 ). Thus complementary approaches usingconditional mutants, such as temperature-sensitive (TS) paralyticmutants of Drosophila, will continue to make important contributions.

Previous studies in Drosophila identified cacophony (cac), alsoknown as nightblind A (nbA), as a neurally expressed homologof vertebrate presynaptic calcium channel ${alpha}$ 1 subunit genes (SMITHet al. 1996 ). In addition, electroretinogram recordings fromcac/nbA mutant flies suggested a role for cac-encoded channelsin synaptic transmission (HEISENBERG and GOTZ 1975 ; SMITHet al. 1998B ). Our laboratory subsequently isolated and characterizedcac^TS2, a cac mutant exhibiting rapid paralysis at elevatedtemperatures (DELLINGER et al. 2000 ). This conditional mutantallowed electrophysiological analysis of synaptic transmissionfollowing acute perturbation of a specific calcium channel geneproduct, revealing that cac encodes a primary calcium channelfunctioning in neurotransmitter release (KAWASAKI et al. 2000).

Recent work identified the molecular lesion in cac^TS2 and demonstratedtransformation rescue of cac mutants by neural expression ofa specific cac-encoded ${alpha}$ 1 subunit variant (KAWASAKI et al. 2002). Independent characterization of the cac^TS2 mutation and itsconsequences for male courtship behavior have also been reportedrecently (CHAN et al. 2002 ). The cac^TS2 mutation maps to acalcium regulatory domain within the C-terminal cytoplasmictail of the ${alpha}$ 1 subunit. This domain includes a binding site forcalmodulin (IQ in Fig 1) as well as an adjacent EF-hand calcium-bindingmotif (EF hand in Fig 1). Calmodulin bound to the IQ domainhas been shown to mediate calcium-dependent facilitation andinactivation (DEMARIA et al. 2001 ); the EF hand may participatein the latter process as well (PETERSON et al. 2000 ). The cac^TS2mutation maps adjacent to the EF-hand domain, raising the possibilitythat altered channel inactivation may be responsible for reducedneurotransmitter release at elevated temperatures (KAWASAKIet al. 2002 and see DISCUSSION).

cac^TS2 and other TS paralytic mutants provide powerful toolsfor analysis of molecular mechanisms underlying synaptic function.In addition, these mutants serve as excellent starting pointsfor broader genetic analysis (RAMASWAMI et al. 1993 ; DELLINGERet al. 2000 ). In fact, cac^TS2 was originally isolated as anenhancer of the N-ethylmaleimide-sensitive fusion protein mutant,comatose (DELLINGER et al. 2000 ), another TS paralytic mutantaffecting neurotransmitter release (KAWASAKI et al. 1998 ).In this study, we conducted a genetic screen for new mutationsthat enhance or suppress the cac^TS2 paralytic phenotype withthe goal of further defining the in vivo functions and interactionsof cac-encoded ${alpha}$ 1 subunits. Among 10 mutants recovered, 4 appearedto be second-site mutations within the cac gene (intragenicmodifiers) and 6 mapped to other genes (extragenic modifiers).Here we focus on behavioral, electrophysiological, and molecularcharacterization of the intragenic modifiers of cac^TS2. Thefindings are discussed in the context of previous work investigatingthe structural determinants of presynaptic calcium channel function.

MATERIALS AND METHODS

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ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

Drosophila stocks:
cac^TS2 and C(1)RM, y w f were from our laboratory stock collection.cac^TS2 was maintained as a homozygous stock. Meiotic mappingof X-linked mutants was carried out by conventional methodsusing a y m wy g f chromosome constructed in our laboratory.Wild-type flies were Canton-S.

Mutagenesis and screening:
An F₂ screen was carried out essentially as described (DELLINGERet al. 2000 ). Briefly, male cac^TS2 flies were exposed for 24hr to a solution of 25 mM ethyl methanesulfonate (EMS) in 1.6%sucrose and then mated in groups of 30 to a similar number ofattached-X females [C(1)RM, y w f]. Mutagenized males were removedfrom these crosses after 5 days. Single F₁ male progeny weremated to attached-X females and F₂ progeny were screened at37° for any alteration of the cac^TS2 behavioral phenotype.Flies were observed for 3 min after placing them in a vial preheatedand maintained at 37° by immersion in a water bath. Crosseswere maintained at room temperature and F₂ progeny were collectedtwice from each cross, $~$ 14 and 21 days after mating. Althoughonly male progeny carry the cac^TS2 mutation, both males andfemales were examined at 37°.

Behavioral analysis:
TS behavior was analyzed in flies reared at 20° or as notedin the text and figure legends. Using the same apparatus describedfor screening, 2- to 3-day-old flies were tested in groups ofsix. Five groups were examined for each genotype (n = 5). Timefor 50% paralysis represents the time at which three flies wereno longer able to stand. In all tests exceeding 5 min in duration,the cotton plug sealing the vial was wet with water to preventdehydration.

Synaptic electrophysiology:
Synaptic current recordings at dorsal longitudinal flight muscle(DLM) neuromuscular synapses of the adult were obtained andanalyzed as described previously (KAWASAKI et al. 1998 ). Experimentswere performed on 2- to 5-day-old flies reared at 20°.

Sequence analysis:
First-strand cDNA synthesis was performed by conventional methods,using total RNA isolated from heads (KAWASAKI et al. 2002 ).The resulting cDNA preparations were used as template in PCRsto amplify the entire 6-kb cac coding sequence in three overlappingfragments. cac coding sequences from modifier mutants were generatedby direct sequencing of reverse transcriptase (RT)-PCR productsand compared directly to those obtained from the cac^TS2 parentchromosome used in the mutagenesis. For analysis of RNA editingat nucleotide position 4106, cDNA clones including this sitewere generated from RT-PCR products and sequenced. Automatedsequencing was carried out on an ABI Prism 377 DNA sequencer(ABI, Foster City, CA) or a CEQ 2000XL DNA analysis system (BeckmanCoulter, Fullerton, CA). Sequence alignments were generatedby the Clustal method, using the MegAlign feature of the Lasergenesoftware package (DNAstar, Madison, WI).

Data analysis:
Data are presented as the mean ± SEM. All graphing andstatistical analysis was carried out using Microsoft Excel (MicrosoftCorp., Seattle, WA). Statistical analysis of electrophysiologicaland behavioral data was performed using an unpaired Student'st-test, and significance was assigned to comparisons with Pvalues $<=$ 0.05. In the figures, values significantly differentfrom control are marked with an asterisk.

RESULTS

TOP
ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

A screen for genetic modifiers of cac^TS2:
The cac^TS2 paralytic phenotype is well suited for the isolationof genetic modifiers. At 36°, cac^TS2 exhibits moderate locomotordefects including spinning, uncoordinated walking, and tumbling,but is able to stand and walk for >50 min (DELLINGER et al.2000 ). In contrast, exposure to 38° results in rapid paralysiswithin $~$ 20 sec (DELLINGER et al. 2000 ). At an intermediate temperatureof 37°, cac^TS2 exhibits severe motor defects approachingparalysis but can remain standing. We anticipated that mutationsthat enhance the cac^TS2 phenotype would cause rapid paralysisat 37°, while suppressors would alleviate the severe motordefects observed at this temperature.

Males carrying the cac^TS2 mutation were exposed to the chemicalmutagen EMS and mated to attached-X (compound X) females (Fig 2).All F₁ male progeny of this cross inherit a mutagenizedpaternal X chromosome carrying cac^TS2 as well as mutagenizedpaternal autosomes. Although screens for TS paralytic mutationson the X chromosome have typically examined F₁ progeny for mutantphenotypes, we have found it advantageous to perform F₂ screensafter backcrossing individual F₁ males to attached-X females(DELLINGER et al. 2000 ). In this study, F₂ progeny from 1954lines were screened for alteration of the cac^TS2 paralytic phenotype.Of 10 modifier mutations recovered, all mapped to the X chromosome.Six were designated extragenic modifiers because they couldbe separated from cac^TS2 by recombination. All of these areenhancers, producing rapid paralysis at 36° in a cac^TS2genetic background. The four remaining mutations (Table 1) weredesignated putative intragenic modifiers because they were notseparated from cac^TS2 during recombinational mapping. Two ofthe intragenic modifiers are enhancers [cac^E(TS2)1 and cac^E(TS2)2]and two are suppressors [cac^su(TS2)1 and cac^su(TS2)2]. Sequenceanalysis of the cac open reading frame (ORF) identified missensemutations in three of these mutants (see below). In this studywe focus on the behavioral, electrophysiological, and molecularcharacterization of the three confirmed intragenic modifiersof cac^TS2.

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Figure 2. An F₂ genetic screen for modifiers of cac^TS2. *, mutagenized chromosome; , attached-X chromosome.

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Table 1. Intragenic modifiers of cac^TS2

TS paralytic behavior:
Initial characterization of the intragenic modifiers involvedexamination of TS behavior. Enhancers and suppressors were analyzedat 36° and 38°, respectively. Note that analysis ofthese mutations was necessarily performed in a cac^TS2 geneticbackground.

The intragenic enhancer, cac^E(TS2)1, caused enhanced paralysisin double-mutant combination with cac^TS2 [cac^TS2 cac^E(TS2)1].While cac^TS2 alone fails to paralyze at 36°, cac^TS2 cac^E(TS2)1is paralyzed rapidly, exhibiting a time for 50% paralysis of0.15 ± 0.01 min (n = 5; Fig 3A). Similarly, femaleshomozygous for cac^TS2 but heterozygous for cac^E(TS2)1 exhibiteda time for 50% paralysis of 0.31 ± 0.03 min (n = 5),indicating that this enhancer is dominant (Fig 3A). The suppressormutation, cac^su(TS2)1, greatly increased the time for 50% paralysisat 38° from 0.28 ± 0.04 min (n = 5) in cac^TS2 aloneto 20.43 ± 1.88 min (n = 5) in cac^TS2 cac^su(TS2)1 doublemutants (Fig 3B). Females homozygous for cac^TS2 but heterozygousfor cac^su(TS2)1 exhibited a time for 50% paralysis of 0.43 ±0.06 min (n = 5), indicating that this suppressor is recessive.

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Figure 3. TS behavior of intragenic modifiers. (A) cac^TS2 cac^E(TS2)1 double mutants exhibited rapid paralysis at 36°. Note that cac^TS2 behavioral tests were truncated after 50 min. (B) Both cac^su(TS2)1 and cac^su(TS2)2 markedly suppressed cac^TS2 paralytic behavior at 38°. Behavioral characterization of cac^su(TS2)2 was performed on flies reared at 23°, as indicated in parentheses following the genotype designations. Asterisks mark values significantly different from control values.

The above behavioral analysis was performed on flies rearedat 20°; however, characterization of the third intragenicmodifier, suppressor cac^su(TS2)2, indicated no suppression ofthe cac^TS2 paralytic phenotype under the same conditions (datanot shown). In contrast, flies reared at 23° (the approximateroom temperature at which crosses were maintained for the geneticscreen) showed strong suppression of cac^TS2 paralysis at 38°(Fig 3B). While cac^TS2 flies reared at 23° exhibited rapidparalysis at 38°, with a time for 50% paralysis of 0.33± 0.02 min (n = 5), the suppressor cac^su(TS2)2 dramaticallyincreased this value to 29.84 ± 1.76 min (n = 5) in cac^TS2cac^su(TS2)2 double mutants. Females homozygous for cac^TS2 andheterozygous for cac^su(TS2)2 exhibited a time for 50% paralysisof 0.39 ± 0.02 min (n = 5), indicating that this suppressoris recessive.

Synaptic physiology:
Our previous electrophysiological analysis at adult neuromuscularsynapses demonstrated that cac^TS2 produces a marked reductionin neurotransmitter release at restrictive temperatures (KAWASAKIet al. 2000 ). To examine whether intragenic modifiers alteredthe synaptic phenotype of cac^TS2, similar experiments were performedin flies carrying both cac^TS2 and the modifier mutations. Two-electrodevoltage clamp was employed at DLM synapses to record excitatorypostsynaptic currents (EPSCs) evoked by DLM motor axon stimulation.Recordings from double-mutant synapses were compared to thosefrom cac^TS2 at both 20° and 36°. As described previously,cac^TS2 exhibited a wild-type synaptic current at 20° anda marked reduction in the EPSC amplitude at 36° (Fig 4Aand Fig B). Both cac^su(TS2)1 and cac^su(TS2)2 produced strikingsuppression of the synaptic current reduction observed in cac^TS2(Fig 4A and Fig B). Synaptic current amplitudes recorded incac^TS2, cac^TS2 cac^su(TS2)1, and cac^TS2 cac^su(TS2)2 at 36°were 1.16 ± 0.21 µA (n = 6), 2.26 ± 0.35µA (n = 9), and 2.63 ± 0.31 µA (n = 6), respectively.These results indicate that each suppressor produces a second-sitelesion in the cac-encoded ${alpha}$ 1 subunit that counteracts the functionalconsequences of the cac^TS2 mutation at neuromuscular synapses.

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Figure 4. Synaptic physiology of intragenic modifiers. (A) Representative synaptic current recordings from DLM neuromuscular synapses of wild type (WT) and cac^TS2, as well as cac^TS2 cac^su(TS2)1 and cac^TS2 cac^su(TS2)2 double mutants. Both cac^su(TS2)1 and cac^su(TS2)2 markedly suppressed the synaptic current reduction observed in cac^TS2 alone at 36°. Arrows indicate stimulation of the DLM motor axon. Stimulation artifacts have been removed. The 36° traces were obtained after 7–12 min at 36°. All recordings were performed on flies reared at 20°. (B) Mean EPSC amplitudes relative to wild type at 36°. The synaptic currents in cac^TS2 cac^su(TS2)1 and cac^TS2 cac^su(TS2)2 were significantly different from those of cac^TS2 alone.

In contrast to the suppressors, cac^E(TS2)1 did not significantlyalter the cac^TS2 synaptic phenotype (Fig 4B). Synaptic currentvalues for cac^TS2 and cac^TS2 cac^E(TS2)1 at 36° were 1.16± 0.21 µA (n = 6) and 1.12 ± 0.19 µA(n = 4), respectively. Thus enhancement of the cac^TS2 behavioralphenotype in cac^TS2 cac^E(TS2)1 is not reflected in DLM neuromuscularsynaptic function, suggesting that enhanced paralysis may resultfrom perturbation of central synapses. In previous studies oftwo TS paralytic mutants affecting synaptic transmission, comatose(KAWASAKI and ORDWAY 1999 ; SANYAL et al. 1999 ) and shibire(SALKOFF and KELLY 1978 ), these mutants exhibited increasedCNS activity at elevated temperatures, suggesting that TS paralysisreflects complex interactions between central and peripheralsynapses. This issue was examined in cac^TS2 cac^E(TS2)1 by performingintracellular DLM recordings under conditions in which the motoraxons are not cut, but rather their connections with the CNSare left intact. In these experiments, the frequency of endogenousDLM action potentials reflects central activity. Unlike comatoseand shibire, cac^TS2 at restrictive temperature exhibits a lowfrequency of DLM action potentials closely resembling that ofwild type (Fig 5A; KAWASAKI and ORDWAY 1999 ). In contrast,the cac^TS2 cac^E(TS2)1 double mutant shows a striking increasein CNS activity at 36°. This activity occurs in bursts thatreach sustained frequencies exceeding 50 Hz and reduce DLM actionpotential amplitude (Fig 5B). Although the precise mechanismsunderlying the enhancement of cac^TS2 paralytic behavior by cac^E(TS2)1remain to be determined, the observed increase in CNS activityis likely to play an important role.

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Figure 5. Intracellular DLM recordings from cac^TS2 (A) and the cac^TS2 cac^E(TS2)1 double mutant (B) at 36°. The DLM motor axons were left intact. High-frequency bursts of action potentials driven by CNS neural activity were observed in cac^TS2 cac^E(TS2)1.

Molecular analysis:
To explore the mechanisms underlying the intragenic modifierphenotypes, the molecular lesions in these mutants were identified.The cac ORF from each mutant was analyzed by direct sequencingof RT-PCR products. To identify the induced mutation, the resultingsequence was compared to that of the parent cac^TS2 chromosomeused in the mutagenesis. Any sequence difference between themodifier mutant and parent cac^TS2 chromosomes was confirmedthrough analysis of at least three independent RNA preparations.Missense mutations were identified in three of the four putativeintragenic modifiers, confirming that these mutations are intragenicand defining the underlying molecular lesions.

Molecular lesions in three intragenic modifiers:
The cac^E(TS2)1 mutation is an a $->$ t transversion at position2407, resulting in substitution of serine for a conserved threonine(T619S) in the P-loop region of the second repeat (Fig 6, bottomleft). A mutation at the analogous position in the human ${alpha}$ 1Agene (T666M) is associated with familial hemiplegic migraine(OPHOFF et al. 1996 ). cac^su(TS2)1 is a t $->$ c transition at position4112, substituting threonine for a conserved isoleucine (I1187T).This residue lies within the short extracellular loop betweenIVS3 and IVS4 (Fig 6, top right) in proximity to the S4 voltagesensor. As described below, cac^su(TS2)1 also alters RNA processingat an adjacent site. Finally, the molecular lesion in cac^su(TS2)2is a t $->$ a transversion at position 3300, substituting leucinefor a conserved phenylalanine (F916L) in IIIS5 (Fig 6, top left).As noted in the DISCUSSION, phenylalanine residues within S5have been proposed to interact with the S4 voltage sensor andplay an important role in voltage-dependent gating.

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Figure 6. Molecular lesions in the intragenic modifiers of cac^TS2. Alignment of CAC with related calcium channel ${alpha}$ 1 subunit polypeptide sequences is shown. Amino acid identities with CAC are shaded. Characteristic domains are indicated with horizontal bars below the alignments. The aligned sequences correspond to CAC (U55776), Mouse ${alpha}$ 1A (NM007578), and C. elegans UNC-2 (U25119).

A fourth putative intragenic modifier, cac^E(TS2)2, exhibiteda wild-type cac ORF sequence and thus was not confirmed to bean allele of cac. In meiotic mapping experiments examining >1000recombinant chromosomes, cac^E(TS2)2 was not separated from cac^TS2,indicating that this modifier is either intragenic or withina closely linked gene.

cac^su(TS2)1 alters pre-mRNA editing:
Despite the short length of the IVS3-IVS4 extracellular loop,the corresponding cac mRNA sequence is subject to both alternativesplicing and A-to-I RNA editing (SMITH et al. 1996 , SMITHet al. 1998A ; PEIXOTO et al. 1997 ). As reported previously,the IVS3-IVS4 loop varies from 9 to 12 amino acids in lengthdepending upon the inclusion or exclusion of a 3-, 6-, or 9-bpalternative exon (SMITH et al. 1996 ; PEIXOTO et al. 1997 ; KAWASAKI et al. 2002 ). The cac^su(TS2)1 mutation (t4112a) isnot within any of these alternative exons, and RT-PCR analysisof cac cDNAs suggests that alternative splicing in this regionis not perturbed in this mutant (data not shown). However, thecac^su(TS2)1 mutation does alter A-to-I RNA editing at an adjacentsite.

A-to-I editing is a form of pre-mRNA processing in which a genomicallyencoded adenosine is deaminated to inosine (reviewed in REENAN2001 ). Inosine is read as guanosine during translation andmay alter the amino acid sequence of the encoded protein. Editingof adenosine 4106, 1 of 12 previously characterized RNA editingsites in cac (SMITH et al. 1998A ; KAWASAKI et al. 2002 ),results in substitution of serine for a genomically encodedasparagine (Fig 7A). Consistent with previous work, our directsequencing of RT-PCR products derived from wild-type or cac^TS2head RNA indicates that the majority of cac transcripts areedited at this position. Sequence chromatographs (Fig 7B) showthat this editing site exhibits major and minor peaks correspondingto the edited and unedited forms, respectively. Interestingly,the cac^su(TS2)1 mutation at nucleotide 4112 appears to suppressediting at position 4106, resulting in similar and often superimposedpeaks corresponding to the edited and unedited sequences (Fig 7C).However, these sequence chromatograph peaks may not providea quantitative measure of the relative abundance of specificcDNA variants, and thus editing at this site was further examinedby generating and sequencing cloned cDNAs. RT-PCR was utilizedto generate cDNA clones including the region of interest fromwild type, cac^TS2, and cac^TS2 cac^su(TS2)1 double mutants. Sequencesfrom >20 clones for each genotype confirmed that editing atposition 4106 is reduced by the cac^su(TS2)1 mutation. The percentagesof clones edited at this site in WT, cac^TS2, and cac^TS2 cac^su(TS2)1were 91.7% (n = 24), 80.0% (n = 25), and 59.1% (n = 22), respectively,in agreement with the sequence chromatograph data. These resultsindicate that the cac^su(TS2)1 mutation acts on an adjacent editingsite to increase the fraction of ${alpha}$ 1 subunits containing a genomicallyencoded asparagine and raise the possibility that altered RNAediting may contribute to the suppressor phenotype.

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Figure 7. The cac^su(TS2)1 mutation alters RNA editing at an adjacent site. (A) A-to-I RNA editing of the cac transcript at position 4106 in effect produces a codon change from aac to agc, resulting in substitution of serine (S) for a genomically encoded asparagine (N). (B) Sequence from cac^TS2 shows major and minor peaks at position 4106, corresponding to the edited (G) and unedited (a) sequences, respectively. (C) The same region from cac^TS2 cac^su(TS2)1 mutant cDNA shows that edited (G) and unedited (A) peaks are of similar size. The adjacent cac^su(TS2)1 molecular lesion is indicated at position 4112.

DISCUSSION

TOP
ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

We have carried out a screen for genetic modifiers of cac^TS2,a calcium channel ${alpha}$ 1 subunit mutant exhibiting rapid paralysisand a marked reduction in neurotransmitter release at elevatedtemperatures. Here we report isolation and characterizationof three intragenic modifier mutations, including one enhancerand two suppressors. Analysis of these mutants has identifiedsecond-site molecular lesions in the cac coding sequence anddefined the resulting behavioral and electrophysiological phenotypes.These findings extend our knowledge of the structural determinantsgoverning the function of a specific presynaptic calcium channel ${alpha}$ 1 subunit at native synapses.

Intragenic modifiers of cac^TS2:
Prior to the isolation of cac^TS2 (DELLINGER et al. 2000 ), viablemutant alleles of cac were recovered in screens for mutationsaltering male courtship (VON SCHILCHER 1976 , VON SCHILCHER1977 ) and the optomotor response (HEISENBERG and GOTZ 1975). In contrast, no cac mutants were identified in previous screensfor X-linked TS paralytic mutants (SUZUKI et al. 1971 ; GRIGLIATTIet al. 1973 ; SIDDIQI and BENZER 1976 ). In this study, threeconfirmed alleles of cac were recovered in a screen of 1954X chromosomes. This relative abundance of cac mutations mayhave resulted from the sensitized background provided by thecac^TS2 behavioral phenotype at 37°.

The molecular lesion in cac^TS2 maps to the second proline ofa highly conserved proline pair located in a calcium regulatorydomain within the C-terminal cytoplasmic tail of the ${alpha}$ 1 subunit(KAWASAKI et al. 2002 ). Interestingly, this proline pair isadjacent to an EF-hand calcium-binding motif, which may participatein calcium-dependent regulation of channel gating (PETERSONet al. 2000 ). This study has begun to define the molecularbasis of functional interactions between cac^TS2 and the intragenicmodifiers through molecular characterization of the modifiermutations.

cac^E(TS2)1:
The cac^E(TS2)1 mutation enhanced the cac^TS2 phenotype, producingrapid paralysis at 36°. This behavioral phenotype was notassociated with enhancement of the cac^TS2 neuromuscular synapticphenotype at the same temperature. However, the marked increasein CNS activity observed by recording endogenous DLM actionpotential frequencies at 36° (Fig 5) likely enhances TSparalysis through fatigue or general disruption of neural function.

The cac^E(TS2)1 mutation results in substitution of serine fora highly conserved threonine within the P loop of repeat II(T619S). A mutation at the analogous position within the human ${alpha}$ 1A gene (T666M) is one of several ${alpha}$ 1A mutations associated withthe human autosomal dominant disorder, familial hemiplegic migraine(OPHOFF et al. 1996 ). Consistent with the position of T666Mwithin the P loop, a reduction in ion permeation has been observed(HANS et al. 1999 ); this mutation has also been shown to enhancechannel inactivation (KRAUS et al. 1998 ). At present the lackof a cac^E(TS2)1 phenotype at neuromuscular synapses remainsunexplained. Although one possibility is that neuromuscularsynapses express an ${alpha}$ 1 subunit variant lacking the mutant formof the P loop, to date no sequence variation has been observedwithin the P loop of repeat II.

cac^su(TS2)1:
The cac^su(TS2)1 mutation strongly suppressed both the TS paralyticand the neuromuscular synaptic phenotypes of cac^TS2. cac^su(TS2)1results in substitution of threonine for a conserved isoleucine(I1187T) within the short IVS3-S4 extracellular loop and alsoreduces A-to-I RNA editing at an adjacent site. Editing at asingle site within the region encoding the IVS3-S4 loop (a4106)leads to substitution of serine for a genomically encoded asparagine(N1185S; SMITH et al. 1996 , SMITH et al. 1998A ). This editingevent is disrupted by the nearby cac^su(TS2)1 mutation, resultingin a lower percentage of edited transcripts. During A-to-I editing,specific secondary structures are thought to form between theedited region and an editing site complementary sequence (ECS)often located in a 3' intron (SMITH et al. 1998A ). The closeproximity of the cac^su(TS2)1 mutation to the a4106 editing siteraises the possibility that the mutation disrupts pairing withthe ECS and thus the secondary structure required for efficientediting. Future studies will determine the relative contributionsof the cac^su(TS2)1 mutation and altered RNA editing to the observedsuppression of cac^TS2.

It is noteworthy that the cac^su(TS2)1 lesion(s) within an extracellularloop of the ${alpha}$ 1 subunit can suppress the phenotype produced bythe altered cytoplasmic tail in cac^TS2, despite the apparentinability of these domains to interact directly. The close proximityof the cac^su(TS2)1 mutation to the IVS4 segment raises the possibilitythat a change in the position or mobility of the voltage sensormay be involved. Such intramolecular functional interactionshave been observed, for example, in voltage-gated sodium channelswhere fast inactivation produces immobilization of the IIIS4and IVS4 voltage sensors (CHA et al. 1999 ; KUHN and GREEFF1999 ). Interestingly, suppressors cac^su(TS2)1 and cac^su(TS2)2(see below) map to repeat IV and III residues that may interactwith the respective S4 voltage sensors.

cac^su(TS2)2:
The cac^su(TS2)2 mutation produces strong suppression of boththe TS paralytic and neuromuscular synaptic phenotypes of cac^TS2.Surprisingly, suppression of the paralytic phenotype requiredrearing flies at 23°, whereas suppression of the neuromuscularsynaptic phenotype was observed in flies reared at 20°.The mechanism underlying this effect is not clear; however,it is likely that central and neuromuscular synapses differin their sensitivity to culture temperature. The suppressorphenotype suggests important intramolecular interactions betweenthe respective channel domains affected by the two mutations.cac^su(TS2)2 maps to one of several phenylalanine residues withinthe IIIS5 segment (F916L). Previously, a systematic analysisof S5 segment phenylalanines was initiated on the basis of anotherDrosophila ion channel mutation, Shaker⁵, which maps to an S5phenylalanine (F401I) of the Shaker-encoded potassium channel(GAUTAM and TANOUYE 1990 ; KANEVSKY and ALDRICH 1999 ). Substitutingphenylalanine 401 with leucine (F401L), but not isoleucine,valine, or alanine, appeared to dramatically stabilize the openstate of the channel, resulting in slowed deactivation and increasedopen probability over a wide range of membrane potentials (KANEVSKYand ALDRICH 1999 ). These effects were modeled in terms of stabilizinginteractions between S5 phenylalanines and positively chargedresidues within the S4 voltage sensor. We speculate that suchan interaction operating in the cac^su(TS2)2 mutant (F916L) mightcounteract inhibition of channel activity in cac^TS2.

The results reported here raise interesting questions aboutthe interactions of calcium channel ${alpha}$ 1 subunit domains in channelgating mechanisms underlying neurotransmitter release. It willbe of great interest to examine the TS behavior of cac^TS2 mutantchannels, as well as the interactions of cac^TS2 and the modifiermutations, through direct functional analysis of wild-type andmutant channels. Together with in vivo analysis examining thefunction of mutant channels at native synapses, these studiesmay provide new insights into the mechanisms underlying presynapticcalcium channel function.

ACKNOWLEDGMENTS

We thank S. Schaeffer (Penn State University) as well as thePenn State Nucleic Acids Facility for assistance with automatedsequencing. This work was supported by a predoctoral fellowshipfrom the American Heart Association (I.M.B.) and grants fromthe National Institutes of Health (NIH R01-NS38064), the NationalScience Foundation (NSF IBN-9986990), and the Penn State President'sFund for Undergraduate Research.

Manuscript received February 1, 2002; Accepted for publication January 3, 2003.

LITERATURE CITED

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ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
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