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Previous Article | Next Article
The Journal of Neuroscience, April 1, 2003, 23(7):2696
Caenorhabditis elegans UNC-103 ERG-Like Potassium Channel Regulates Contractile Behaviors of Sex Muscles in Males before and during Mating
L. Rene Garcia1 and Paul W. Sternberg2 1 Department of Biology, Texas A&M University, College Station, Texas 77843-3258, and 2 Howard Hughes Medical Institute and Division of Biology, California Institute of Technology, Pasadena, California 91125
ABSTRACT
TOP
ABSTRACT
Introduction
During mating behavior the Caenorhabditis elegans male must regulate periodic and prolonged protractor muscle contractions to insert his copulatory spicules into his mate. The protractors undergo periodic contractions to allow the spicules to reattempt insertion if a previous thrust failed to breach the vulva. When the spicule tips penetrate the vulva, the protractors undergo prolonged contraction to keep the spicules inside the hermaphrodite until sperm transfer is complete. To understand how these contractions are regulated, we isolated EMS-induced mutations that cause males to execute prolonged contraction inappropriately. Loss-of-function mutations in the unc-103 ERG-like K+ channel gene cause the protractor muscles to contract in the absence of mating stimulation. unc-103-induced spicule protraction can be suppressed by killing the SPC motor neurons and the anal depressor muscle: cells that directly contact the protractors. Also, reduction in acetylcholine suppresses unc-103-induced protraction, suggesting that UNC-103 keeps cholinergic neurons from stimulating the protractors before mating behavior. UNC-103 also regulates the timing of spicule protraction during mating behavior. unc-103 males that do not display mating-independent spicule protraction show abnormal spicule insertion behavior during sex. In contrast to wild-type males, unc-103 mutants execute prolonged contractions spontaneously within sequences of periodic protractor contractions. The premature prolonged contractions cause the spicules to extend from the male tail before the spicule tips penetrate the vulva. These observations demonstrate that unc-103 controls various aspects of spicule function.
Key words: Caenorhabditis elegans; mating behavior; unc-103; ERG; K+ channel; L-type voltage-gated calcium channels
Introduction
Analysis of Drosophila behavioral mutants led to the first in vivo correlation among K+ channel genes such as shaker (Kamb et al., 1987
; Temple et al., 1987
In Caenorhabditis elegans genetic screens also have identified K+ channel genes that regulate different behaviors. Gain-of-function mutations in the K+ channel genes like unc-103 (the homolog of seizure/erg) (Reiner et al., 1999
C. elegans male mating behavior is a complex behavior that requires the coordination of different motor outputs (Ward and Carrel, 1979
To understand how distinct motor outputs are regulated, we isolated mutations that induce spontaneous spicule protraction. We find that mutations in unc-103, the worm homolog of Drosophila seizure/erg-encoded and the human h-erg-encoded delayed inward rectifying voltage-gated K+ channel, affect the spicule insertion step (Sanguinetti et al., 1995
h-erg encodes the cardiac IKr K+ channel that facilitates cardiac rhythms (Sanguinetti et al., 1995
Materials and Methods
Strains. All strains used in this study contain him-5(e1490) on LGV (Hodgkin et al., 1979
Isolation of sy557 and scoring mating-independent spicule protraction. To isolate sy557, we first mutagenized PS1395 hermaphrodites by using ethyl methanesulfonate (EMS) (Brenner, 1974
To isolate sy670, sy673, and sy674, we followed the procedure of Park and Horvitz (1986)
sy557 animals were out-crossed six times to N2 strains. We out-crossed sy670, sy673, and sy674 animals to non-mutagenized unc-103(e1597) two times before we assayed their behavior. To score mating-independent spicule protraction, we first removed L4 males away from hermaphrodites, putting 20-30 males together on a Petri plate. Then 24 hr later we used a Wild M5A microscope to count how many males had protruding spicules. We continued to score the males for 2 d additionally; however, permanent spicule protraction generally occurred within the first 24 hr of adulthood. Mating-independent spicule protraction is not dependent on population density. The frequency of spicule protraction did not change if individuals were isolated or 150 males were kept together (data not shown). However, if too few males were kept together, the males crawled off the agar and dried on the side of the Petri plate; if too many males were kept together, the males would aggregate, damage the agar surface, and burrow.
Mating efficiency. We adapted the mating efficiency assay from Hodgkin (1983)
Mapping of sy557. We used standard mapping procedures to three-factor map sy557 (Brenner, 1974
We also used standard SNP mapping procedure to three-factor map sy557 in relation to SNPs that are located between unc-93 and pal-1 (Wicks et al., 2001
The results from the SNP mapping experiments are as follows: from daf-2 sy557 dpy-17 (N2)/+ (CB4856) heterozygotes, 1 of 16 daf-2 sy557+ recombinants contained snp C28A5.2 from CB4856 and 4 of 16 recombinants contained both snp C28A5.2 and snp R10E4.1 from CB4856; from daf-2 sy557 dpy-17(N2)/+ (CB4856) heterozygotes, 23 of 24 daf-2++ recombinants contained the SNPs pkP3096, pkP3097, snp C30D11.4, snp R10E4.1, and snp C28A5.2 from CB4856, and 1 of 24 recombinants contained snp C30D11.4, snp R10E4.1, and snp C28A5.2 from CB4856. These data suggested that sy557 mapped in a region between snp C30D11.4 and snp R10E4.1
Pharmacology. We dissolved arecoline (purchased from Sigma-Aldrich, St. Louis, MO) in water to make a stock solution of 100 mM. We then serially diluted the stock solution in water as needed. We added 1 ml of the drug to a Pyrex round-bottom, three-well titer dish. Then 5-10 <24 hr adult virgin males were transferred to the drug bath. We observed the males for 5 min with a Wild M5A microscope. The males were considered responsive to the drug if they kept their spicules protracted for
10 sec.
Laser ablations. We used standard laser ablation protocols to kill cells in the male tail (Bargmann and Avery, 1995
unc-103 reporter construction. We PCR-amplified an 8.2 kb fragment of DNA that contains 5 kb upstream of the unc-103 start codon and includes part of the seventh exon of unc-103. We used N2 genomic DNA as the template for the PCR and the primers 5'-GGGCACGCCTGCCTAAGGGATGCCTTAGCTCGGCC-3' and 5'-CTGGTGAAA TCGGATAAATTCTCTG-3' to amplify the DNA fragment. We then blunt end-ligated the PCR fragment into the SmaI site of pPD95.79 (plasmid courtesy of A. Fire, Carnegie Institute of Washington, Baltimore, MD) to make the plasmid pR48. Green fluorescent protein (GFP) is fused ~20 amino acids after the S6 transmembrane domain. pR48 (30 ng/µl) and the wild-type pha-1-containing plasmid pBX-1 (100 ng/µl) were injected into the germline of pha-1;him-5 hermaphrodites (Mello et al., 1991
We noted that the fusion protein aggregates mostly on the cytoplasmic membrane of neuronal processes and in many, but not all, cases of cell bodies; however, we detected no deleterious effect of the fusion construct on the behavior of the transgenic animals. In larval hermaphrodites and males we were able to identify some of the cells that had cell body localization of UNC-103:: GFP; many neurons express the construct, but because of variability in cell position and cellular localization of the fusion protein in processes, our list of unc-103-expressing cells is far from complete. In the head region ALA, ADL, ASK, AVH, AVJ, AIN, AVA, ASJ, SMDD, SIA, ADE, and AVD express the construct. In the tail region PHA, DVC, ALN, and PVP express the construct. The unc-103 fusion protein accumulates extensively in the processes of many ventral cord neurons; however, we were able to identify only some cells in the AS class of excitatory neurons. In the adult hermaphrodite HSN expresses the unc-103:: gfp construct.
Injections of pR48 at
Mating observation. We observed mating behavior with a compound microscope fit with a 40× objective. Mating behavior was recorded with an MTI CCD72 black-and-white video camera and a Panasonic AG-6740 time-lapse Super VHS videocassette recorder. We placed five 15-24 hr unc-38(sy576);egl-19(n582) adult hermaphrodites and one male on a 5-mm-diameter OP50 lawn made on a 1 cm block of agar. We then placed the agar block on a microscope slide for direct viewing. When the male tail touched the vulva, we started the video recording. Males have difficulty inserting their spicules into young hermaphrodites and will prod the vulva continuously for 10 min or longer. This allowed us to make long recordings of this behavior. To quantify the rate of spicule movements for wild type and unc-103 null, we slowed the recordings to 1/7 the original speed and manually counted the downstrokes of the spicules.
Results
unc-103 males protract their copulatory spicules independently of mating stimulation
The C. elegans male contains two copulatory spicules. Each spicule is attached to two protractor muscles (Fig. 1A). When these muscles contract, the attached spicules extrude from the male tail. To understand how specific motor behaviors are regulated during copulation, we screened for mutations that uncouple the spicule insertion step from other mating-specific motor and sensory behaviors. From a screen of 10,000 EMS-mutagenized gametes we isolated the sy557 allele. Wild-type males keep their spicules extended from their tails only during mating. In contrast, sy557 males spontaneously protract their spicules in the absence of mating stimulation.
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Figure 1. Mating-independent spicule protraction displayed by a sy557 mutant male. A depicts a diagram of the sex muscles that are associated with the spicules (right lateral view of the male tail). The drawing was adapted from Sulston et al. (1980)
Initially after the L4 molt sy557 adult males behave normally, but within 1-5 hr they spontaneously protract their spicules (Fig. 1B-D). Occasionally, mating-independent protraction is coupled with a dorsal or a ventral tail curl. Affected males sometimes can retract their spicules into their tails; however, their spicules will continue to protract inappropriately. Eventually, the spicules remain permanently protracted.
This mutant phenotype is similar to the protruding spicule phenotype of males that contain the gain-of-function egl-19(n2368gf) allele (Lee et al., 1997
1 subunit (Lee et al., 1997
In a population of virgin males kept isolated from hermaphrodites, ~60% of the males will protract their spicules permanently within 24 hr after they emerge from their L4 cuticle (Table 1). Once the spicules remain protracted, the sy557 male is incapable of siring progeny. Exceptional sy557 males that do not display mating-independent spicule protraction can sire progeny, albeit at an efficiency less than wild-type males (wild-type mating efficiency: 0.74 ± 0.11, mean ± SD, n = 3 trials; sy557 mating efficiency: 0.29 ± 0.12, n = 2 trials).
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Table 1. unc-103 mutants display mating-independent spicule protraction sy557 males and hermaphrodites do not show any gross abnormalities in other behaviors such as locomotion, pharyngeal pumping behavior, defecation, or chemotaxis. However, sy557 hermaphrodites sometimes lay eggs at a slightly higher rate than wild type (our unpublished observation).
We mapped sy557 to LGIII between daf-2 and dpy-17 (see Materials and Methods). Using single nucleotide polymorphisms as mapping markers (Wicks et al., 2001
We sequenced the predicted coding regions of unc-103 in our reference wild-type strain and in the sy557 mutant and found that the sy557 mutant contains two missense mutations in unc-103. The mutations change a histidine at amino acid 165 to an asparagine near the S3 transmembrane region and a tryptophan at position 244 to an arginine in the S5 region. Both of these substitutions are in amino acids that are conserved in the human, fly, and worm protein (Fig. 2).
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Figure 2. Locations of mutation-induced amino acid changes in UNC-103. Amino acid residues that are identical to human HERG are boxed; those that are identical to Drosophila ERG are identified by the thin underline. Approximate regions of UNC-103 that correspond to the six membrane-spanning (S1-S6), the pore (P), and the cyclic nucleotide-binding (CNBD) domains are identified by the thick underline. Downward-pointing arrowheads show amino acids that are changed in the mutant alleles isolated in this study. The amino acid changes are listed next to the mutant allele.
Reduction of unc-103 causes spontaneous spicule protractor contraction
To determine how the two missense mutations in unc-103(sy557) cause mating-independent spicule protraction, we compared the phenotype induced by unc-103(sy557) with the phenotypes of loss-of-function, gain-of-function, and null alleles of unc-103. unc-103(sy557) is semidominant because heterozygous males protract their spicules (Table 1). To determine whether semidominance was attributable to sy557 conferring enhanced activity to UNC-103, we first compared unc-103(sy557) with the canonical gain-of-function unc-103(e1597gf) allele. unc-103 was defined first by the dominant gain-of-function mutations e1597 and n500 (Hodgkin, 1983
Work by others has shown that suppression of unc-103(e1597gf)-induced lethargy and defective egg-laying behaviors can be caused by intragenic mutations that reduce gene function (Park and Horvitz, 1986
In all, 20 and 37% of males containing unc-103(sy673, e1597gf) W85opal and unc-103(sy670, e1597gf) G306E, respectively, displayed seizures of their protractor muscles; in contrast, only 7% of unc-103(e1597gf, sy674) P426S showed the phenotype. We believe that both the W85opal and G306E lesions reduce K+ channel function of the gain-of-function protein. The stop mutation truncates the gain-of-function protein within the first transmembrane region, and others have demonstrated that mutating the equivalent glycine in the ion selectivity filter of the human HERG channel disrupts ion conduction (Sanguinetti et al., 1996
Although loss-of-function and null mutations in unc-103 caused mating-independent spicule protraction, the percentages of males showing the defect were lower compared with unc-103(sy557) H165N, W244R males. To test whether UNC-103 (H165N, W244R) also might interfere with wild-type UNC-103 function, we analyzed its genetic interaction with the gain-of-function unc-103 allele. Arecoline, an acetylcholine agonist, can induce the spicule protractor muscles to contract artificially (Garcia et al., 2001
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Figure 3. Arecoline-induced spicule protraction in unc-103 mutants. A, The sensitivities of unc-103(e1597gf) males to different concentrations of arecoline are compared with wild type. The numbers in the columns refer to the percentages of males that protract their spicules with drug exposure; n refers to the number of males assayed. B shows how different unc-103 genotypes affect the percentages of males that protract their spicules in 1 mM arecoline.
The SPC motor neurons and the anal depressor muscle facilitate unc-103(sy557)-induced spicule protraction
The SPC motor neurons and the anal depressor muscle are attached directly to the protractor muscles (Fig. 4A) (Sulston et al., 1980
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Figure 4. Cells involved in unc-103(sy557)-induced spicule protraction. A depicts the right lateral view of the male tail, highlighting cells that are associated with the spicules. The drawing was adapted from Sulston et al. (1980)
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Table 2. Ablations of protractor associated cells Because unc-103(sy557) does not act solely in the protractor muscles, we fused GFP to unc-103 sequences to determine which of the cells associated with the spicules express the gene. Our unc-103:: GFP construct expressed broadly in the head and ventral cord neurons in both males and hermaphrodites (see Materials and Methods). In the male tail the SPC motor neurons and the PCB postcloacal sensory neurons expressed the construct (Fig. 4B). The expression in SPC is consistent with those neurons contributing to unc-103(sy557)-induced spicule protraction. Irregular expression was seen in the PCA postcloacal sensory neurons; in other neurons that are associated with spicules, such as the PCC postcloacal sensory neurons and the SPD and SPV spicule sensory neurons, the fusion protein was not expressed.
The unc-103(sy557) phenotype requires acetylcholine production and L-type voltage-gated calcium channels
To determine which molecular components are acting inappropriately when unc-103 is compromised, we surveyed mutations that affect general synaptic transmission and muscle contraction for suppression of the unc-103(sy557) phenotype. We found that mutations in cat-1 [vesicular monoamine transporter (Duerr et al., 1999
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Table 3. Mutant genes that affect unc-103(sy557)-induced protraction UNC-68 ryanodine receptor calcium channels are not essential for spicule insertion behavior, but they contribute to the frequency of periodic contractions. The unc-68(r1158) null allele reduced the unc-103(sy557)-induced protraction by one-half, suggesting that, in some animals, calcium efflux from sarcoplasmic stores can contribute to muscle seizures. However, because many unc-103(sy557);unc-68(r1158) males still had protracted spicules, intracellular calcium mobilization must not be essential.
Although mutations in unc-13, unc-31, and unc-64 reduce synaptic transmission, they had little effect on the unc-103(sy557) phenotype. This finding was unexpected because reducing ACh production with the cha-1 mutation affected mating-independent spicule protraction. The unc-13, unc-31, and unc-64 alleles used in this work might not reduce synaptic transmission enough to affect spontaneous protraction drastically; alternatively, unc-103(sy557) might allow the neurons to bypass the requirement for wild-type action of these three genes.
unc-103 males execute premature prolonged protractor contraction during mating
When wild-type males mate with 24 hr or younger adult hermaphrodites, they have difficulty inserting their spicules into the vulva. The tips of the spicules rapidly prod the vulval slit until eventually they penetrate the vulva. Prodding behavior is facilitated by UNC-68-mediated periodic protractor contractions. When the spicule tips penetrate the vulva, the SPC motor neurons have been proposed to trigger EGL-19-mediated prolonged contraction, causing the spicules to remain extended from the male tail (Garcia et al., 2001
Although the unc-103 mutant phenotype suggests that UNC-103 helps to keep the spicule muscles inactive before mating, the protein might function additionally during sex. To address this, we observed how nonprotracted unc-103 males try to insert their spicules into 24 hr adult hermaphrodites. We observed that, instead of consistently prodding the vulval slit with their spicule tips until penetration, all unc-103(sy557) H165N, W244R males (n = 2), unc-103(sy673, e1597gf) W85opal males (n = 10), and unc-103(n1213) null males (n = 10) repeatedly protract their spicules during prodding behavior. The prematurely extended spicules would depress the hermaphrodite vulva rather than penetrate it. After protraction the spicules retract into the male tail to resume prodding behavior. We ablated the SPC motor neurons in five unc-103(n1213) null animals and observed their spicule insertion behavior. All of the operated males prematurely protracted their spicules during prodding behavior, demonstrating that the SPC motor neuron is not essential for this abnormal behavior.
We analyzed four intact unc-103(n1213) null males and four wild-type males in greater detail by counting the movements of their spicules. Video recordings of spicule insertion behavior were played back at slower speeds to determine the number of spicule movements during prodding behavior and the frequency of spontaneous protraction (Fig. 5). In contrast to the steady rhythmic prodding of wild-type spicules, we found that the spicules of unc-103(n1213) null males arrhythmically prodded the vulval slit 1-9 times/sec. We also noted that complete spicule protraction punctuated every 1-12 sec of prodding behavior. Thus we conclude that unc-103 plays at least two roles in the male: to suppress protractor muscle contractions until proper mating signals are sensed and to regulate periodic and prolonged contractions during mating.
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Figure 5. Number of muscle contractions per second during prodding behavior. A shows the profiles of muscle contractions of four unc-103(n1213) males. The horizontal axis displays sequential seconds during the window of observation. Gray columns represent the number of spicule movements during each second of prodding behavior. The black in some of the gray columns refers to a prolonged contraction that occurred during that time interval. Time intervals that show no gray columns are attributable to the hermaphrodites shifting their position during the observation period. Males temporarily stop prodding behavior to reorient their tails over the vulva. B shows the profiles of muscle contractions of four wild-type males.
Discussion
UNC-103 keeps the spicule protractor muscles inactive before mating
Male mating behavior consists of many stereotyped sub-behaviors that must be coordinated to insure efficient mating. To impregnate a hermaphrodite, the male moves backward along her body scanning for the vulva. If the male fails to locate the vulva on one side of the hermaphrodite, he will turn to her other side and resume vulva location behavior. When he locates her genitalia, he stops backward locomotion and adjusts the position of his tail over the vulva so that the spicule tips contact the vulval slit. The neurons used for vulva location behavior also signal the spicule protractor muscles to contract and relax rhythmically until the spicules penetrate the vulval barrier. When the spicules breach the vulva, the SPC motor neurons signal the protractor muscles to remain contracted until sperm transfer is completed.
To understand how different spicule muscle behaviors are regulated, we isolated mutations that cause males to protract their spicules in the absence of mating stimulation. From 10,000 mutagenized gametes we isolated unc-103(sy557). unc-103(sy557) causes ~60% of virgin males to protract their copulatory spicules within 24 hr of adulthood. UNC-103 encodes a putative voltage-gated K+ channel that is homologous to human h-erg and Drosophila seizure/erg. The sy557 lesion contains two mutations that create an H165N and W244R amino acid change in the K+ channel protein. Null and loss-of-function alleles of unc-103 also induce spontaneous spicule protraction, suggesting that before mating behavior UNC-103 keeps the spicule muscles from contracting. No other gross behavioral abnormalities are seen in unc-103(null) and unc-103(sy557) males, suggesting that cells in the spicule insertion behavioral circuit are more sensitive to changes in this K+ channel than other unc-103-expressing cells.
UNC-103 may act in parallel with other proteins to regulate protractor muscle activity
Although unc-103(sy557) and the other unc-103 alleles cause mating-independent spicule protraction, males that do not protract their spicules within 24 hr of adulthood will not display the abnormal phenotype later. Two scenarios can account for why some males do not show the defect: (1) buffering systems that act parallel to unc-103 can overcompensate for loss of unc-103 function or (2) unaffected males are not exposed to some environmental stimuli that normally activates an unc-103-regulated excitatory pathway.
We favor the hypothesis that, at some efficiency, compensating mechanisms can attenuate spontaneous protractor activity in these exceptional males. The sy557 allele induces mating-independent spicule protraction at a higher percentage than compared with other unc-103 alleles. This difference could be attributable to the sy557 protein interfering with these hypothetical compensating mechanisms. In our mutant screen we identified three additional mutations that cause premature spicule protraction similar to unc-103(sy557). These mutations are not in unc-103 and might affect components that act parallel to the K+ channel (our unpublished data).
Behavioral and pharmacological properties of unc-103(sy557)/+ and unc-103(sy557)/unc-103(gf) males suggest that unc-103(sy557) encodes a dominant-negative protein that also may interfere promiscuously with other proteins. The H165N and W244R changes in the sy557 protein affect amino acids that are conserved in the human, fly, and worm protein. The hydrophobic aromatic to a hydrophilic basic side chain change at position 244 in the S5 transmembrane domain of unc-103 may disrupt proper channel function. However, the consequence of the H165N substitution near the S3 transmembrane region is not obvious. UNC-103 shares ~40% amino acid identity to the ether-a-go-go-encoded (eag) K+ channels in humans, flies, and worms (Titus et al., 1997
Neuronal ACh input facilitates unc-103(sy557)-induced spicule protraction
Ablation of both the SPC cholinergic neuron and the anal depressor muscle is required to suppress spontaneous spicule protraction. Removing either one separately has little effect, suggesting that both cells are capable of triggering the protractor muscles to sustain contraction. During mating behavior only the SPC motor neurons are essential for prolonged contraction. However, under artificial conditions neither SPC nor the anal depressor is required because ACh agonists can activate protractor contraction directly even when both cell types are ablated (Garcia et al., 2001
unc-103 is expressed in the SPC neurons, consistent with the contribution of those cells to the mutant phenotype. In hermaphrodites and larval males the AVL and DVB GABAergic neurons activate anal depressor muscle contractions (McIntire et al., 1993
Similar to unc-103(sy557), aldicarb, an acetylcholine esterase inhibitor, can induce males to protract their spicules. Ablation of the SPC cholinergic motor neurons and the anal depressor muscle can attenuate aldicarb-induced protraction, demonstrating that ACh can act on or via these cells to induce the protractors to contract. Mutations in cha-1 choline acetyltransferase or unc-64 syntaxin also reduce aldicarb-induced protraction. Thus in the absence of mating stimulation low levels of cholinergic transmission to the protractor and anal depressor muscle occur (Garcia et al., 2001
Worms containing unc-64 syntaxin mutations are severely compromised for locomotion. Elimination of SLO-1 calcium-activated, voltage-gated K+ channels suppresses unc-64-induced lethargy. This observation suggests that unc-64 mutants express enough syntaxin proteins to promote locomotion, but not enough to overcome negative regulation of synaptic transmission by SLO-1 channels in ventral cord neurons (Wang et al., 2001
UNC-103 regulates prolonged contraction during mating
During mating behavior ACh initiates two types of protractor muscle contractions that use different calcium channels. UNC-68 ryanodine receptor calcium channels are used during periodic contractions, and EGL-19 L-type voltage-gated calcium channels are needed for prolonged contraction. These calcium channels also are differentially required for levamisole-induced (an ACh agonist) and arecoline-induced spicule protraction. The difference between levamisole and arecoline activity is that the former requires UNC-68, whereas the latter requires EGL-19 (Garcia et al., 2001
unc-103 mutants that do not protract their spicules permanently show a consistent abnormal spicule insertion behavior during mating. As unc-103 mutant males try to breach the vulva, the rhythm of periodic protractor contractions is abnormal and is disrupted by spurious prolonged contraction. In contrast to wild type, these premature prolonged contractions do not require the SPC motor neurons. Considering that the protractor muscles must distinguish between which types of cholinergic-induced contraction to use during spicule insertion behavior, UNC-103 might suppress EGL-19-used cholinergic pathways while the protractor muscles are undergoing ACh-stimulated periodic contractions.
FOOTNOTES Received Nov. 13, 2002; revised Jan. 9, 2003; accepted Jan. 13, 2003.
The Howard Hughes Medical Institute with which P.W.S. is an investigator and L.R.G. was an associate supported this research. L.R.G. was supported by a Department of Health and Human Services National Research Service Award (GM18857). Strains were provided by the Caenorhabditis Genetics Center, which is supported by National Institutes of Health National Center for Research Resources. We thank David Reiner and James Thomas for communicating to us the molecular lesions in unc-103(e1597gf) and unc-103(n1213). We also thank Karin Doerr for writing software used in this work and Gary Schindelman for comments on this manuscript.
Correspondence should be addressed to L. Rene Garcia, Department of Biology, Texas A&M University, 3258 TAMU, College Station, TX 77843-3258. E-mail: rgarcia{at}mail.bio.tamu.edu.
References
- Ahmed S, Maruyama IN, Kozma R, Lee JH, Brenner S, Lim L (1992) The Caenorhabditis elegans unc-13 gene product is a phospholipid-dependent high-affinity phorbol ester receptor. Biochem J 287:995-999.
- Alfonso A, Grundahl K, McManus JR, Rand JB (1994) Cloning and characterization of the choline acetyltransferase structural gene (cha-1) from C. elegans. J Neurosci 14:2290-2300[Abstract].
- Ann K, Kowalchyk JA, Loyet KM, Martin TF (1997) Novel Ca2+ binding protein (CAPS) related to UNC-31 required for Ca2+-activated exocytosis. J Biol Chem 272:19637-19640
[Abstract/Free Full Text] .- Atkinson NS, Robertson GA, Ganetzky B (1991) A component of calcium-activated potassium channels encoded by the Drosophila slo locus. Science 253:551-555
[Abstract/Free Full Text] .- Bamber BA, Beg AA, Twyman RE, Jorgensen EM (1999) The Caenorhabditis elegans unc-49 locus encodes multiple subunits of a heteromultimeric GABA receptor. J Neurosci 19:5348-5359
[Abstract/Free Full Text] .- Bargmann CI, Avery L (1995) Laser killing of cells in Caenorhabditis elegans. In: Methods of cell biology, Vol 48, Caenorhabditis elegans: modern biological analysis of an organism (Epstein HF, Shakes DC, eds), pp 225-250. New York: Academic.
- Barker DM (1994) Copulatory plugs and paternity assurance in the nematode Caenorhabditis elegans. Anim Behav 48:147-156.
- Barr MM, Sternberg PW (1999) A polycystic kidney-disease gene homologue required for male mating behaviour in C. elegans. Nature 401:386-389[Medline].
- Brenner S (1974) The genetics of Caenorhabditis elegans. Genetics 77:71-94
[Abstract/Free Full Text] .- Cowan TM, Siegel RW (1986) Drosophila mutations that alter ionic conduction disrupt acquisition and retention of a conditioned odor avoidance response. J Neurogenet 3:187-201[Web of Science][Medline].
- Curran ME, Splawski I, Timothy KW, Vincent GM, Green ED, Keating MT (1995) A molecular basis for cardiac arrhythmia: HERG mutations cause long QT syndrome. Cell 80:795-803[Web of Science][Medline].
- Davis MW, Fleischhauer R, Dent JA, Joho RH, Avery L (1999) A mutation in the C. elegans EXP-2 potassium channel that alters feeding behavior. Science 286:2501-2504
[Abstract/Free Full Text] .- Doyle DA, Morais Cabral J, Pfuetzner RA, Kuo A, Gulbis JM, Cohen SL, Chait BT, MacKinnon R (1998) The structure of the potassium channel: molecular basis of K+ conduction and selectivity. Science 280:69-77
[Abstract/Free Full Text] .- Duerr JS, Frisby DL, Gaskin J, Duke A, Asermely K, Huddleston D, Eiden LE, Rand JB (1999) The cat-1 gene of Caenorhabditis elegans encodes a vesicular monoamine transporter required for specific monoamine-dependent behaviors. J Neurosci 19:72-84
[Abstract/Free Full Text] .- Elkes DA, Cardozo DL, Madison J, Kaplan JM (1997) EGL-36 shaw channels regulate C. elegans egg-laying muscle activity. Neuron 19:165-174[Web of Science][Medline].
- Elkins T, Ganetzky B (1990) Conduction in the giant nerve fiber pathway in temperature-sensitive paralytic mutants of Drosophila. J Neurogenet 6:207-219[Web of Science][Medline].
- Engel JE, Wu C-F (1998) Genetic dissection of functional contributions of specific potassium channel subunits in habituation of an escape circuit in Drosophila. J Neurosci 18:2254-2267
[Abstract/Free Full Text] .- Fleming JT, Squire MD, Barnes TM, Tornoe C, Matsuda K, Ahnn J, Fire A, Sulston JE, Barnard EA, Sattelle DB, Lewis JA (1997) Caenorhabditis elegans levamisole resistance genes lev-1, unc-29, and unc-38 encode functional nicotinic acetylcholine receptor subunits. J Neurosci 17:5843-5857
[Abstract/Free Full Text] .- Garcia LR, Mehta P, Sternberg PW (2001) Regulation of distinct muscle behaviors controls the C. elegans male's copulatory spicules during mating. Cell 107:777-788[Web of Science][Medline].
- Granato M, Schnabel H, Schnabel R (1994) pha-1, a selectable marker for gene transfer in C. elegans. Nucleic Acids Res 22:1762-1763
[Free Full Text] .- Greenwald IS, Horvitz HR (1980) unc-93(e1500): a behavioral mutant of C. elegans that defines a gene with a wild-type null phenotype. Genetics 96:147-164
[Abstract/Free Full Text] .- Griffith LC, Wang J, Zhong Y, Wu CF, Greenspan R (1994) Calcium/calmodulin-dependent protein kinase II and potassium channel subunit EAG similarly affect plasticity in Drosophila. Proc Natl Acad Sci USA 91:10044-10048
[Abstract/Free Full Text] .- Hodgkin J (1983) Male phenotypes and mating efficiency in Caenorhabditis elegans. Genetics 103:43-64
[Abstract/Free Full Text] .- Hodgkin JA, Doniach T (1997) Natural variation and copulatory plug formation in Caenorhabditis elegans. Genetics 146:149-164[Abstract].
- Hodgkin JA, Horvitz HR, Brenner S (1979) Nondisjunction mutants of the nematode Caenorhabditis elegans. Genetics 91:67-94
[Abstract/Free Full Text] .- Jackson FR, Wilson SD, Strichartz GR, Hall LM (1984) Two types of mutants affecting voltage-sensitive sodium channels in Drosophila melanogaster. Nature 308:189-191[Medline].
- Jackson FR, Gitschier J, Strichartz GR, Hall LM (1985) Genetic modifications of voltage-sensitive sodium channels in Drosophila: gene dosage studies of the seizure locus. J Neurosci 5:1144-1151[Abstract].
- Johnstone DB, Wei A, Butler A, Salkoff L, Thomas JH (1997) Behavioral defects in C. elegans egl-36 mutants result from potassium channels shifted in voltage dependence of activation. Neuron 19:151-164[Web of Science][Medline].
- Kamb A, Iverson LE, Tanouye MA (1987) Molecular characterization of Shaker, a Drosophila gene that encodes a potassium channel. Cell 50:405-413[Web of Science][Medline].
- Kaplan WD, Trout WE (1969) The behavior of four neurological mutants of Drosophila. Genetics 61:399-409
[Free Full Text] .- Kasbekar DP, Nelson JC, Hall LM (1987) Enhancer of seizure: a new genetic locus in Drosophila melanogaster defined by interactions with temperature-sensitive paralytic mutations. Genetics 116:423-431
[Abstract/Free Full Text] .- Kunkel MT, Johnstone DB, Thomas JH, Salkoff L (2000) Mutants of a temperature-sensitive two-P domain potassium channel. J Neurosci 20:7517-7524
[Abstract/Free Full Text] .- Lee RYN, Lobel L, Hengartner M, Horvitz HR, Avery L (1997) Mutations in the
- Liu KS, Sternberg PW (1995) Sensory regulation of male mating behavior in Caenorhabditis elegans. Neuron 14:79-89[Web of Science][Medline].
- Loer CM, Kenyon CJ (1993) Serotonin-deficient mutants and male mating behavior in the nematode Caenorhabditis elegans. J Neurosci 13:5407-5417[Abstract].
- Maryon EB, Coronado R, Anderson P (1996) unc-68 encodes a ryanodine receptor involved in regulating C. elegans body-wall muscle contraction. J Cell Biol 134:885-893
[Abstract/Free Full Text] .- McIntire SL, Jorgensen E, Kaplan J, Horvitz HR (1993) The GABAergic nervous system of Caenorhabditis elegans. Nature 364:337-341[Medline].
- Mello CC, Kramer JM, Stinchcomb D, Ambros V (1991) Efficient gene transfer in C. elegans: extrachromosomal maintenance and integration of transforming sequences. EMBO J 10:3959-3970[Web of Science][Medline].
- O'Dowd DK, Aldrich RW (1988) Voltage-clamp analysis of sodium channels in wild-type and mutant Drosophila neurons. J Neurosci 8:3633-3643[Abstract].
- Ogawa H, Harada S, Sassa T, Yamamoto H, Hosono R (1998) Functional properties of the unc-64 gene encoding a Caenorhabditis elegans syntaxin. J Biol Chem 273:2192-2198
[Abstract/Free Full Text] .- Papazian DM, Schwarz TL, Tempel BL, Timpe LC, Jan LY (1988) Ion channels in Drosophila. Annu Rev Physiol 50:379-394[Web of Science][Medline].
- Park EC, Horvitz HR (1986) Mutations with dominant effects on the behavior and morphology of the nematode Caenorhabditis elegans. Genetics 113:821-852
[Abstract/Free Full Text] .- Pongs O, Kecskemethy N, Muller R, Krah-Jentgens I, Baumann A, Kiltz HH, Canal I, Llamazares S, Ferrus A (1988) Shaker encodes a family of putative potassium channel proteins in the nervous system of Drosophila. EMBO J 7:1087-1096[Web of Science][Medline].
- Reiner DJ, Weinshenker D, Thomas JH (1995) Analysis of dominant mutations affecting muscle excitation in Caenorhabditis elegans. Genetics 141:961-976[Abstract].
- Reiner DJ, Newton EM, Tian H, Thomas JH (1999) Diverse behavioural defects caused by mutations in Caenorhabditis elegans unc-43 CaM kinase II. Nature 402:199-203[Medline].
- Riddle DL (1977) A genetic pathway for dauer larva formation in C. elegans. Stadler Genet Symp 9:101-120.
- Saifee O, Wei L, Nonet ML (1998) The Caenorhabditis elegans unc-64 locus encodes a syntaxin that interacts genetically with synaptobrevin. Mol Biol Cell 9:1235-1252
[Abstract/Free Full Text] .- Sanguinetti MC, Jiang C, Curran ME, Keating MT (1995) A mechanistic link between an inherited and an acquired cardiac arrhythmia: HERG encodes the IKr potassium channel. Cell 81:299-307[Web of Science][Medline].
- Sanguinetti MC, Curran ME, Spector PS, Keating MT (1996) Spectrum of HERG K+ channel dysfunction in an inherited cardiac arrhythmia. Proc Natl Acad Sci USA 93:2208-2212
[Abstract/Free Full Text] .- Schafer WR, Kenyon CJ (1995) A calcium-channel homologue required for adaptation to dopamine and serotonin in Caenorhabditis elegans. Nature 375:73-78[Medline].
- Schnabel H, Schnabel R (1990) An organ-specific differentiation gene, pha-1, from Caenorhabditis elegans. Science 250:686-688
[Abstract/Free Full Text] .- Simon JM, Sternberg PW (2002) Evidence of a mate-finding cue in the hermaphrodite nematode Caenorhabditis elegans. Proc Natl Acad Sci USA 99:1598-1603
[Abstract/Free Full Text] .- Sulston J, Dew M, Brenner S (1975) Dopaminergic neurons in the nematode Caenorhabditis elegans. J Comp Neurol 163:215-226[Web of Science][Medline].
- Sulston JE, Albertson DG, Thomson JN (1980) The Caenorhabditis elegans male: postembryonic development of nongonadal structures. Dev Biol 78:542-576[Web of Science][Medline].
- Temple BL, Papazian DM, Schwarz TL, Jan YN, Jan LY (1987) Sequence of a probable potassium channel component encoded at the Shaker locus of Drosophila. Science 237:770-775
[Abstract/Free Full Text] .- Thomas JH (1990) Genetic analysis of defecation in Caenorhabditis elegans. Genetics 124:855-872[Abstract].
- Titus SA, Warmke JW, Ganetzky B (1997) The Drosophila erg K+ channel polypeptide is encoded by the seizure locus. J Neurosci 17:875-881
[Abstract/Free Full Text] .- Trent C, Tsung N, Horvitz HR (1983) Egg-laying defective mutants of the nematode Caenorhabditis elegans. Genetics 104:619-647
[Abstract/Free Full Text] .- Trudeau MC, Warmke JW, Ganetzky B, Robertson GA (1995) HERG, a human inward rectifier in the voltage-gated potassium channel family. Science 269:92-95
[Abstract/Free Full Text] .- Wang XJ, Reynolds ER, Deak P, Hall LM (1997) The seizure locus encodes the Drosophila homolog of the HERG potassium channel. J Neurosci 17:882-890
[Abstract/Free Full Text] .- Wang ZW, Saifee O, Nonet ML, Salkoff L (2001) SLO-1 potassium channels control quantal content of neurotransmitter release at the C. elegans neuromuscular junction. Neuron 32:867-881[Web of Science][Medline].
- Ward S, Carrel JS (1979) Fertilization and sperm competition in the nematode Caenorhabditis elegans. Dev Biol 73:304-321[Web of Science][Medline].
- Waring DA, Kenyon CJ (1990) Selective silencing of cell communication influences anteroposterior pattern formation in C. elegans. Cell 60:123-131[Web of Science][Medline].
- Warmke JW, Drysdale R, Ganetzky B (1991) A distinct potassium channel polypeptide encoded by the Drosophila eag locus. Science 252:1560-1562
[Abstract/Free Full Text] .- Weinshenker D, Wei A, Salkoff L, Thomas JH (1999) Block of an ether-a-go-go-like K+ channel by imipramine rescues egl-2 excitation defects in Caenorhabditis elegans. J Neurosci 19:9831-9840
[Abstract/Free Full Text] .- Wicks SR, Yeh RT, Gish WR, Waterston RH, Plasterk RHA (2001) Rapid gene mapping in Caenorhabditis elegans using a high density polymorphism map. Nat Genet 28:160-164[Web of Science][Medline].
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