Regulation of Neurotransmitter Vesicles by the Homeodomain Protein UNC-4 and Its Transcriptional Corepressor UNC-37/Groucho inCaenorhabditis elegans Cholinergic  Motor Neurons

Kim M. Lickteig; Janet S. Duerr; Dennis L. Frisby; David H. Hall; James B. Rand; David M. Miller

doi:10.1523/JNEUROSCI.21-06-02001.2001

Abstract

Motor neuron function depends on neurotransmitter release from synaptic vesicles (SVs). Here we show that the UNC-4 homeoprotein and its transcriptional corepressor protein UNC-37 regulate SV protein levels in specific Caenorhabditis elegans motor neurons. UNC-4 is expressed in four classes (DA, VA, VC, and SAB) of cholinergic motor neurons. Antibody staining reveals that five different vesicular proteins (UNC-17, choline acetyltransferase, Synaptotagmin, Synaptobrevin, and RAB-3) are substantially reduced in unc-4 and unc-37mutants in these cells; nonvesicular neuronal proteins (Syntaxin, UNC-18, and UNC-11) are not affected, however. Ultrastructural analysis of VA motor neurons in the mutant unc-4(e120) confirms that SV number in the presynaptic zone is reduced (∼40%) whereas axonal diameter and synaptic morphology are not visibly altered. Because the UNC-4–UNC-37 complex has been shown to mediate transcriptional repression, we propose that these effects are performed via an intermediate gene. Our results are consistent with a model in which this unc-4 target gene (“gene-x”) functions at a post-transcriptional level as a negative regulator of SV biogenesis or stability. Experiments with a temperature-sensitive unc-4 mutant show that the adult level of SV proteins strictly depends on unc-4 function during a critical period of motor neuron differentiation.unc-4 activity during this sensitive larval stage is also required for the creation of proper synaptic inputs to VA motor neurons. The temporal correlation of these events may mean that a common unc-4-dependent mechanism controls both the specificity of synaptic inputs as well as the strength of synaptic outputs for these motor neurons.

The function of motor neuron circuits depends on synaptic transmission between specific cells. Studies of the nematode Caenorhabditis elegans have revealed that a homeodomain protein encoded by the unc-4 gene controls the pattern of synaptic inputs to one class of motor neurons in the ventral nerve cord (Miller et al., 1992; White et al., 1992). The strong backward movement defect that unc-4 mutants display is correlated with the miswiring of VA motor neurons with synapses from command interneurons normally reserved for their lineal sister cells, the VB motor neurons. Expression of the UNC-4 protein in the VA motor neurons rescues this phenotype and thereby establishes that unc-4 functions in the postsynaptic cell (i.e., VA motor neuron) to block input from inappropriate presynaptic partners (i.e., VB-type command interneurons) (Miller and Niemeyer, 1995). UNC-4 activity requires physical interaction with UNC-37, a ubiquitously expressed Groucho-like transcriptional corepressor protein (Miller et al., 1993; Pflugrad et al., 1997). Thus, we have proposed that the creation of appropriate synaptic inputs to VA motor neurons depends on UNC-4–UNC-37-mediated repression of “VB-specific genes” (Winnier et al., 1999).

LacZ and green fluorescent protein (GFP) reporter genes have also detected unc-4 expression in additional classes of motor neurons in the ventral nerve cord and in flanking ganglia (Miller and Niemeyer, 1995; Pflugrad et al., 1997). Because these motor neurons (e.g., DAs) are not miswired with improper inputs in unc-4mutants (White et al., 1992), the functional significance ofunc-4 expression in these cells has been unclear. Here we show that unc-4 and unc-37 mutations result in decreased levels of synaptic vesicle (SV) proteins in allunc-4-expressing motor neurons and that this deficit impairs the function of these cells.

SVs are clustered near the presynaptic density (PSD) where they are poised for rapid membrane fusion and release of neurotransmitter (for review, see Calakos and Scheller, 1996). Specialized vesicular proteins are incorporated into the SVs to modulate these events. Vesicle exocytosis and recycling also depend on interactions with cytoplasmic and axonal membrane proteins. Expression of these synaptic proteins is developmentally regulated and subject to both transcriptional and post-transcriptional mechanisms of control (Bergmann et al., 1991; Lou and Bixby, 1993; Melloni et al., 1994;Petersohn et al., 1995; Deans et al., 1997; Smith et al., 1997). Additional homeostatic mechanisms of regulation are suggested by the observation that neurons in many systems contain different types and numbers of synaptic vesicles (White et al., 1986; Jia et al., 1993;Merchan-Perez and Liberman, 1996; Jin et al., 1999). These differences may indicate that SV levels are actively regulated in each of these cell types to satisfy specific physiological requirements.

The evolutionary conservation of the secretory apparatus has facilitated the use of genetic approaches in simple model systems to discover new components of the mammalian exocytic pathway and to define their modes of action (Rothman, 1994; M. Nonet, 1999; Lloyd et al., 2000). Because UNC-4 and its cofactor UNC-37 (Pflugrad et al., 1997) have been shown to function as transcriptional repressors (Winnier et al., 1999), the decreased levels of vesicular proteins that we observe in unc-4 and unc-37 mutants must result from an indirect mechanism of action; UNC-4 and UNC-37 may repress a target gene (“gene-x”) that in turn exerts a negative effect on vesicular protein levels. Furthermore, our results indicate that this presumptive downstream gene acts via a post-transcriptional mechanism; derepression of gene-x in unc-4 orunc-37 mutants must either constrain SV biogenesis or enhance SV turnover. These outcomes are strictly dependent onunc-4 activity during embryonic and early larval stages of motor neuron differentiation; SV protein expression does not requireunc-4 function in the adult. This finding parallels a previous observation that the specificity of synaptic inputs to one class of cholinergic motor neurons (e.g., VAs) also depends onunc-4 function during a concurrent period of larval growth (Miller et al., 1992). The temporal coincidence of these events offers the intriguing possibility that both the specificity of synaptic inputs as well as the strength of synaptic outputs for these motor neurons may depend on a common unc-4-regulated mechanism.

MATERIALS AND METHODS

Nematode strains. C. elegans were grown as described (Brenner, 1974). The N2 (Bristol) strain was used as the wild-type strain. All genetic experiments were performed at 25°C with the exception that the unc-4(e2322ts) strain (Miller et al., 1992) was grown at the permissive temperature of 16°C when noted.

Chromosomal integration of the unc-4 promoter-gfpline (wdIs5) was achieved by γ irradiation (4000 rads). Animals with gfp reporter genes [wdIs5,unc-17-cha-1p:: gfp, andunc-4p:: synaptobrevin-1 (SNB-1):: gfp] were anesthetized with 1% tricaine and tetramisole and assessed as described previously (Miller et al., 1999). The following mutant strains were used: in linkage group I (LG I), unc-37(e262), unc-37(wd17),bli-4(e937), unc-11(n2954), andunc-13(e51); in LG II, bli-2(e768),unc-104(e1265), unc-4 alleles e120,wd1, e26, e2321, ande2322ts; and in LG IV, dpy-20(e1282),unc-17(e113), and cha-1(md39ts).

Genetics. unc-4 unc-104 double mutants were constructed by first marking unc-4 with bli-2. unc-104 was crossed into the bli-2 unc-4 strains, and nonblister Unc-4 animals were picked to select for a crossover event between bli-2 and unc-104. The presence of unc-4 in the unc-4 unc-104 double mutant was verified by a complementation test usingunc-4(e2322ts) males (Miller et al., 1993).

unc-37(wd17)-containing strains were constructed by crossingbli-4 unc-37(wd17) animals (Miller et al., 1993) withunc-4 unc-104 strains. The presence of the wd17mutation in this strain was confirmed by the appearance of non-Unc-4 progeny from matings with unc-4(e2322ts) males at the restrictive temperature (25°C).

UNC-18 antibody. The DNA sequence corresponding to amino acids 18–584 of UNC-18 was amplified from a cDNA library by PCR and cloned into pRSETB (Invitrogen, San Diego, CA). A fusion protein with a 6×-His terminal tag was expressed with the Xpress System (Invitrogen) and purified over a ProBond resin column. Purified fusion protein was used to immunize two goats and two rabbits. Anti-UNC-18 was affinity purified with the fusion protein coupled with methanol to nitrocellulose filters (Duerr et al., 1999). Antiserum from one goat (G247) gave the most specific signal on fixed C. elegans and was used for this study.

Synaptotagmin antibody. A bacterially expressed fusion protein containing amino acids 144–441 of the synaptotagmin (SNT-1) protein was produced and purified as described previously (Nonet et al., 1993) and used to immunize rabbits. The resulting sera were affinity purified using the bacterial fusion protein.

Immunofluorescence. To evaluate antibody staining of the DA and VA motor neurons, animals were synchronized using a Chlorox and NaOH solution, and the resultant embryos were grown to the late L2 stage (Sulston and Hodgkin, 1988). Antibody staining of the DAs and VAs was performed within 1 d of fixation to preserve the GFP fluorescence that tended to fade with time. Adult animals were antibody-stained for evaluation of vesicular and neuronal protein expression in the VC and SAB motor neurons. All antibodies were diluted in antibody buffer B, pH 7.2 (1× PBS, 0.5% Triton X-100, 1 mm EDTA, pH 8.0, and 0.1% BSA) (Duerr et al., 1999). Stained animals were placed in a mounting media containing 200 mg/mln-propyl gallate, 30 mm Tris, pH 9, 70% glycerol, and 20 μg/ml 4′,6-diamidino-2-phenylindole.

For UNC-17 and choline acetyltransferase (ChAT) antibody staining, animals were placed on a slide, immobilized by pressing down on a coverslip, and frozen on dry ice for 30 min. After removal of the coverslip (freeze–crack), the animals were fixed in methanol for 2 min and then acetone for 4 min at 4°C. Samples were blocked for 1 hr at room temperature (RT) with 10% goat serum. Incubation with a 1:200 dilution of monoclonal UNC-17 antibody or 100 μl of ChAT antibody sera (J. Duerr and J. Rand, unpublished observations) was performed for 4 hr to overnight at RT. Goat anti-mouse indocarbocyanine (Cy3) secondary antibody (1:400) (Jackson ImmunoResearch, West Grove, PA) was incubated for 4 hr at RT.

Double antibody staining with UNC-18 and UNC-17 antibodies was performed in a two-step process. Freeze-cracked animals were fixed for 2 min in methanol followed by 4 min in acetone. Animals were blocked in 1% BSA and then incubated with a 1:40 dilution of goat anti-UNC-18 at 4°C overnight. Secondary antibody of rabbit anti-goat Cy3 (1:200) was then incubated for 4 hr at RT. Next, 10% goat serum was added to block residual rabbit anti-goat Cy3-binding sites. Animals were then incubated with UNC-17 mouse monoclonal antibody (1:200) for 4 hr at RT followed by incubation with secondary antibody of goat anti-mouse Cy2 (1:600) for 4 hr at RT.

Antibody staining with UNC-11 (Nonet et al., 1999) was performed on freeze-cracked animals fixed for 10 min in methanol at −20°C. UNC-11 antibody was incubated at 1:200 dilution overnight at 4°C. Secondary antibody of goat anti-rabbit Cy3 (1:200) was incubated at RT for 4 hr.

Synaptotagmin antibody staining was performed on freeze-cracked animals prepared as described above except that animals were subsequently fixed in 2% paraformaldehyde on ice for 4 hr. Synaptotagmin antibody was incubated for 4 hr at RT at a 1:50 dilution. Incubation with goat anti-rabbit Cy3 secondary antibody (1:200) (Jackson ImmunoResearch) was performed for 4 hr at RT.

For the remainder of the antibodies used in these experiments (see below), animals were fixed with 0.4 ml of Bouin's solution (75 ml of saturated picric acid, 25 ml of formalin, and 5 ml of glacial acetic acid), 0.4 ml of methanol, and 0.01 ml of β-mercaptoethanol followed by incubations in primary antibodies for 2 hr at RT and secondary antibodies for 2 hr at RT. Primary antibody combinations included anti-Synaptobrevin (1:50) (Nonet et al., 1998) and monoclonal GFP antibody (1:2000) (Clontech, Cambridge, UK); anti-RAB-3 (1:100) (Nonet et al., 1997) and polyclonal GFP antibody (1:1000) (Molecular Probes, Eugene, OR); and anti-Syntaxin (1:1000) (Saifee et al., 1998) and anti-RAB-3 (1:50) (Nonet et al., 1997). Secondary antibodies used were goat anti-rabbit Cy3 (1:500), goat anti-mouse Cy2 (1:200), goat anti-mouse Cy3 (1:500), and goat anti-rabbit Cy2 (1:200) (Jackson ImmunoResearch).

Microscopy. Immunofluorescent micrographs were obtained in aZeiss Axioplan microscope and in a Zeiss LSM 410 confocal microscope.

The fluorescent intensity of individual DA and VA motor neurons was defined by comparison with flanking neurons in the ventral nerve cord (VNC) (i.e., VB, DB, and AS neurons). Staining intensity was scored in three categories: “wild type,” in which DA and VA staining was comparable with that of adjacent cholinergic neurons; “reduced,” in which DA and VA fluorescent intensity was visibly less bright than that of the reference neurons; “none,” in which staining was not detectable or very faint.

Electron micrograph analysis. Existing sets of serial electron micrographs (EMs) of N2 (White et al., 1986) and of twounc-4(e120) animals (White et al., 1992) were examined to determine the numbers of presynaptic neurotransmitter vesicles in VA and VB motor neurons. Randomly selected prints were digitized on a flat bed scanner and recorded on compact disks. The number of vesicles in the VA and VB motor neurons was counted in each image (Adobe Photoshop). Sections that contained a thickening that resembled a PSD were then used to calculate the number of vesicles per PSD. For N2, four VA neurons (40 PSDs) and three VB neurons (43 PSDs) were analyzed. Two unc-4 animals were analyzed with a total of four VA neurons (54 PSDs) and four VB neurons (41 PSDs). The Mann–Whitney test was performed to determine whether the average number of vesicles per PSD was statistically different in the VAs versus the VBs in wild-type and unc-4-mutant backgrounds.

Thrashing assay. Adult animals were subjected to Chlorox and NaOH solution to isolate embryos (Sulston and Hodgkin, 1988). Embryos were placed on clean plates and incubated for 2 hr at 25°C. Hatched L1 animals were placed in M9 buffer in a 96-well microtiter plate. The number of times an active animal thrashed in a given direction was counted in a 2 min interval (Miller et al., 1996).

unc-4:: SNB-1:: gfp transgenic strains. Transgenic lines were obtained by injectingpSB126.65 (unc-4:: SNB-1:: gfp) (M. L. Nonet, 1999) and pMH86 [the dpy-20(+) cotransformation marker] (Clark et al., 1995) at 25 ng/μl (Mello and Fire, 1995). Standard genetic crosses were used to place the reporter gene into unc-4(wd1) and unc-37(e262)backgrounds.

Temperature-shift experiments. UNC-17 antibody staining was evaluated as a function of unc-4 activity in DA and VA motor neurons. The double mutant unc-4(e2322ts) unc-104(e1265) was used for all temperature-shift experiments. For the analysis ofunc-4(e2322ts) animals (Miller et al., 1992) at the permissive temperature, animals were raised at 16°C and then synchronized by Chlorox treatment (Sulston and Hodgkin, 1988). These animals were grown at the permissive temperature until the early adult stage. For analysis of unc-4ts at the restrictive temperature, animals were raised at 25°C, synchronized, and grown to the early adult stage. For the temperature-shift experiments, animals were raised at the first temperature (“embryo”), synchronized, shifted to the second temperature, and grown until the end of the L2 stage (determined by the appearance of the postderid cells; “L1–L2”) (Sulston and Horvitz, 1977); these animals were then grown at the third temperature until the early adult stage (“adult”). UNC-17 antibody staining for these animals was performed as described above.

RESULTS

UNC-4 is expressed in cholinergic motor neurons

The homeodomain protein UNC-4 is expressed in specific classes of motor neurons. In the ventral nerve cord, UNC-4 is expressed in A-type motor neurons (the VAs and DAs) (Miller and Niemeyer, 1995) and in the VC motor neurons (Fig. 1). The VAs extend anteriorly directed axons within the ventral nerve fascicle, whereas the DAs send out commissural processes that also project anteriorly after entering the dorsal nerve cord (White et al., 1986). There are six VC motor neurons that innervate the vulval muscles in the midventral region (White et al., 1976, 1986). unc-4 is initially expressed in the VCs at the onset of vulval morphogenesis in the mid-L3 larval stage (data not shown). UNC-4 is also expressed in three SAB motor neurons (SABVL, SABVR, and SABD) (Miller and Niemeyer, 1995) that send out four anteriorly directed processes in the dorsal and ventral sublateral nerve cords adjacent to muscles in the head (White et al., 1986).

Fig. 1.

UNC-4:: GFP is expressed in four classes of ventral cord motor neurons (DA, VA, VC, and SAB). Theunc-4 promoter was fused to GFP for expression in transgenic animals (Pflugrad et al., 1997). A, Left lateral view showing a representative VA motor neuron with anteriorly directed axon in the VNC and a DA motor neuron with circumferential commissure and anteriorly directed axon in the dorsal nerve cord.B, Ventral view of L1 larva showing GFP accumulation in cell bodies of all nine DA motor neurons and in two SAB motor neurons (arrowheads). Axons are out of the plane of focus.C, Left lateral view of L2 larva showing GFP expression in all 12 VA motor neuron cell bodies. D, E, Ventral view of adult hermaphrodite showing GFP-positive VC4 and VC5 somata and VC1–VC6 axonal projections to vulval muscles (arrowhead). F, Left lateral view of GFP expression in anteriorly directed axonal projections (arrows) of SAB motor neurons. (Only two of four SAB processes are shown.) AVF processes in the nerve ring (arrowhead) and the I5 motor neuron (asterisk) in the posterior bulb of the pharynx also show UNC-4:: GFP expression. G, Three SAB motor neurons innervating ventral (SABVL, SABVR) and dorsal (SABD) muscles in the head. Images shown in D andF are flattened stacks of optical sections collected in the confocal microscope. Scale bars, 10 μm. Anterior is to theleft.

These four classes of “unc-4-motor neurons” (DA, VA, VC, and SAB) are known to express ChAT and the vesicular acetylcholine transporter (VAChT or UNC-17) (J. Duerr, D. L. Frisby, and J. Rand, unpublished observations) and are therefore likely to use acetylcholine as an excitatory neurotransmitter. UNC-17 is an integral membrane component of neurotransmitter vesicles; a substantial fraction of the ChAT protein is also associated with vesicles in C. elegans (J. Duerr, unpublished observations). Here we show that the levels of UNC-17 and ChAT as well as that of other vesicle-associated proteins are regulated by unc-4 in these cholinergic motor neurons. [unc-4 is also expressed in the pharyngeal I5 motor neuron and in AVF neurons in the retrovesicular ganglion (Miller and Niemeyer, 1995), but the effects ofunc-4 mutations on SV proteins were not evaluated in these cells.]

UNC-4 is required for expression of UNC-17 and ChAT inunc-4-motor neurons

Antibody staining of wild-type animals for UNC-17 and ChAT produces a punctate pattern that is characteristic of presynaptic varicosities at en passant synapses. These UNC-17- and ChAT-containing structures are especially well resolved in the ventral and dorsal sublateral nerve cords in the head (Fig.2) that contain tightly apposed axonal projections from two classes of cholinergic motor neurons, the SABs and SAAs (White et al., 1986) (J. Duerr, D. H. Hall, and J. Rand, unpublished observations). We observed a significant decrease in UNC-17 and ChAT staining in these processes in the null mutantunc-4(wd1) (Table 1); ∼55% of the dorsal and ventral head sublateral nerve cords show wild-type levels of UNC-17 and ChAT staining in unc-4(wd1) animals. UNC-17 and ChAT staining is either reduced or absent in the remaining fasicles. [The complete elimination of UNC-17 and ChAT staining in some cases may mean that both the SAB and SAA axons are affected. However, we believe that the SAA defect must be indirect because UNC-4 is normally expressed in the SAB motor neurons but not in the SAAs.] Comparable decreases in UNC-17 and ChAT staining were also observed in three additional unc-4 alleles including the canonical null allele unc-4(e120) as well as the missense mutantse26 and e2321 (Fig. 2, Table 1) (Winnier et al., 1999). In addition to the decrease in UNC-17 and ChAT antibody staining, we observed defects in axonal morphology; 10–15% of the dorsal and ventral head sublateral cords show misplaced, elongated, or branched processes in unc-4 and unc-37 mutants (data not shown). These morphologically abnormal SABs (and/or SAAs) also show reduced levels of UNC-17 and ChAT staining.

Fig. 2.

UNC-17 expression in motor neurons is decreased inunc-4 mutants. A, Left lateral view shows punctate pattern of UNC-17 antibody staining in the SAB-containing nerve cords in the head region of a wild-type animal.Arrows point to dorsal and ventral left sublateral processes. B, Punctate UNC-17 staining is reduced or eliminated in many of the head sublateral processes inunc-4(e120)-mutant animals. Note the absence of UNC-17 staining in the left ventral process containing SABVL.C, Ventral view of UNC-17 expression in wild-type VC axons that innervate the vulval muscles (arrowhead) is shown. D, UNC-17 staining of VC vulval projections is eliminated or reduced in unc-4(e120) mutants, but UNC-17 staining of other cholinergic processes in the VNC and ventral sublateral (SL) nerve cords is not noticeably affected. E–I, Left lateral views are shown. The unc-104 kinesin mutation was used to localize UNC-17 to the soma of ventral cord motor neurons (Hall and Hedgecock, 1991; Nonet et al., 1993). The nuclei of DA and VA motor neurons also express UNC-4:: GFP (see G) (Pflugrad et al., 1997). E, G, H, In animals that are wild-type for unc-4, strong UNC-17 antibody staining is visible in the cytoplasm of cholinergic motor neurons. F, I, In unc-4(e120) mutants, cytoplasmic UNC-17 staining is substantially reduced in theunc-4::gfp-expressing DA and VA motor neurons.H and I are enlargements of single VA neurons from E and F(arrows), respectively. Scale bars, 10 μm. Anterior is to the left.

View this table:

Table 1.

UNC-17 and ChAT antibody staining

UNC-17 and ChAT levels were also evaluated in the VC axons that exit the ventral nerve cord to innervate vulval muscles (White et al., 1986). As shown in Figure 2, UNC-17 and ChAT staining of VC neuromuscular synapses is readily detected in the wild-type animal. However, in unc-4 mutants, UNC-17 and ChAT staining is substantially reduced in the VC motor neuron presynaptic zones (Fig.2D, Table 1).

DA and VA motor neurons extend axons into the dorsal and ventral nerve cords, respectively (Fig. 1) (White et al., 1986). The active zones of these A-type motor neuronal processes are enmeshed in tightly packed fascicles and are thus not readily distinguished from the presynaptic regions of other overlapping motor neurons. To circumvent this problem, we evaluated UNC-17 and ChAT staining in the presence of a mutation in the unc-104 kinesin gene (Hall and Hedgecock, 1991). Theunc-104(e1265) mutation blocks anterograde axonal transport such that SVs accumulate in neuronal cell bodies where they can be detected by UNC-17 and ChAT antibody staining (Nonet et al., 1993). To aid in the identification of these unc-4 motor neurons in the ventral nerve cord, we used an integrated unc-4promoter-gfp line (wdIs5) to mark the DA and VA cell nuclei (Pflugrad et al., 1997). In animals containing wild-type UNC-4 activity, ∼80% of the VA and DAs (marked with GFP) show bright UNC-17 staining (Fig. 2, Table 1). However, in unc-4mutants, we observed that only ∼10% of the VA and DA neurons show wild-type levels of UNC-17 staining. ChAT staining in the A-type motor neurons is also reduced in unc-4 mutants (Table 1).

UNC-37 functions with UNC-4 to maintain cholinergic proteins

Other work from this laboratory has shown that the pattern of synaptic inputs to VA motor neurons (D. Hall, E. German, and D. Miller, unpublished observations) depends on unc-37 function (Pflugrad et al., 1997; Winnier et al., 1999). Here we show thatunc-37 is also required for regulation of cholinergic protein expression in the VAs and in other unc-4 motor neurons. UNC-17 and ChAT antibody staining is substantially reduced in all four types of unc-4 motor neurons in mutants bearing the hypomorphic allele unc-37(e262) (Table 1) (Miller et al., 1993). UNC-17 and ChAT staining was not detectably altered in other classes of cholinergic motor neurons (DB, VB, and AS) in the ventral nerve cord (data not shown), indicating that this UNC-37 missense mutation specifically perturbs the regulation of these neurotransmitter vesicle-associated proteins in unc-4 motor neurons.

UNC-4 and UNC-37 regulate the levels of other vesicular proteins

UNC-17 is an integral vesicular membrane protein (Alfonso et al., 1993). Although ChAT is a cytosolic enzyme, a significant fraction of ChAT protein is associated with the vesicles (Duerr, unpublished observations). Because these two vesicular proteins are downregulated in unc-4 and unc-37 animals, we wondered whether other vesicular proteins are also affected in these mutants. We used specific antibodies to assess the effects of unc-4 andunc-37 activity on the levels of three additional proteins that are associated with synaptic vesicles: (1) Synaptotagmin, an integral vesicular protein proposed to be involved in calcium-mediated SV release and vesicle endocytosis (Nonet et al., 1993), (2) Synaptobrevin, an integral vesicular protein that is a component of the SNARE complex (Nonet et al., 1998), and (3) RAB-3, a GTPase that associates with vesicles before fusion (Nonet et al., 1997). In all three cases, the levels of antibody staining were substantially reduced in DA and VA motor neurons in unc-4 and unc-37mutants (Fig. 3). Thus, our results show that five different vesicular or vesicle-associated proteins (UNC-17, ChAT, Synaptotagmin, Synaptobrevin, and RAB-3) are downregulated in animals with loss-of-function mutations in either the unc-4or unc-37 genes.

Fig. 3.

Vesicular protein levels depend onunc-4 and unc-37 activity. Antibodies to RAB-3 (A), Synaptobrevin (B), and Synaptotagmin (C) were used to detect these vesicular proteins in the DA and VA motor neurons in wild-type and in unc-4- andunc-37-mutant animals. (Methods were as described for Fig. 2.) Vertical bars in the histograms indicate the percentage of DA and VA motor neurons showing intense antibody staining (white) plus the percentage of animals showing reduced or intermediate levels of staining (gray) (see Materials and Methods). At least 125 VA and DA neurons were scored for each strain and for each vesicular protein antibody. Allunc-4 and unc-37 mutants in these experiments are loss-of-function alleles.

Nonvesicular proteins are not affected in unc-4 andunc-37 mutants

To determine whether unc-4 and unc-37 affect all proteins involved in exocytosis or whether this effect is restricted to vesicular proteins, we examined levels of Syntaxin (Ogawa et al., 1998; Saifee et al., 1998), a neuronal membrane component of the SNARE complex, as well as that of UNC-18 (Hosono et al., 1992;Geppert et al., 1994), a cytoplasmic protein implicated in regulating the docking of vesicles via its association with Syntaxin. Expression levels of these proteins were scored in the VC axonal projections and in the SAB-containing dorsal and ventral sublateral nerve cords in the head. UNC-18 is readily detected in axonal projections of the VC motor neurons in wild-type as well as in unc-4 andunc-37 animals. This finding stands in contrast to our observation that UNC-17 expression in the VCs is only seen in wild-type animals (Fig. 4, Table2).

Fig. 4.

UNC-18 expression is not altered inunc-4 and unc-37 mutants. A ventral view of the vulval area is shown. Anterior is to the left. Double antibody staining was performed with UNC-17 and UNC-18 antibodies. A, D, UNC-18 antibody (red) stains the axonal processes of the VCs in a diffuse pattern (arrow). B, E, UNC-17 (green) is detected in VC varicosities associated with vulval muscles (arrow). C, F,Merged images show overlapping UNC-17 and UNC-18 antibody staining (yellow). A–C, In wild type, the UNC-17 and UNC-18 antibodies colocalize to VC axonal projections. D–F, In unc-4 mutants, UNC-18 (D, F) but not UNC-17 (E, F) (arrow) is detectable in VC axonal processes. All images are stacked confocal sections and were merged in Photoshop (C, F). Scale bar,A–C,D–F, 10 μm.

View this table:

Table 2.

Comparison of vesicular proteins RAB-3 and UNC-17 with nonvesicular proteins Syntaxin and UNC-18

Although Syntaxin expression is not detectable in the VCs, we did observe high levels of Syntaxin as well as UNC-18 staining in the head sublaterals in both unc-4 and unc-37 mutants (Table 2). In this case, it is possible that at least some of the Syntaxin and UNC-18 staining in the head sublaterals may be caused by the SAA axons that normally fasiculate with SAB processes. The differential effects of unc-4 and unc-37mutations on vesicular proteins are clearly seen in SAB (or SAA) axons with branching or guidance defects that stain for Syntaxin and UNC-18 but that do not show expression of either RAB-3 or UNC-17 (data not shown). These results indicate that specific synaptic membrane and docking regulatory proteins are expressed at wild-type levels inunc-4 and unc-37 mutants whereas vesicular proteins are downregulated.

We also assessed the potential effects of the unc-4mutations on UNC-11, a component of the endocytic machinery. TheC. elegans unc-11 gene encodes a homolog of the clathrin adaptor protein AP180 (Nonet et al., 1999). In the missense alleleunc-11(n2954), the UNC-11 protein is restricted to motor neuron cell bodies and does not accumulate at presynaptic termini. This property of the mutant protein was used to score UNC-11 expression in DA and VA motor neurons in the ventral nerve cord. Approximately 90% of ventral cord motor neurons including the DAs and VAs stain positive for UNC-11 in the unc-11 single mutant as well as in theunc-4;unc-11 double mutant (data not shown). Thus, theunc-4 mutation does not lower the levels of UNC-11 protein. This conclusion is also consistent with electron micrographs of VA motor neuron presynaptic zones that do not show the characteristically enlarged vesicular structures that are seen in unc-11mutants (data not shown) (Nonet et al., 1999).

Neurotransmitter vesicles are decreased inunc-4 mutants

EM reconstruction of unc-4(e120) has revealed that the VA motor neurons receive incorrect inputs but are otherwise morphologically wild-type with anteriorly directed axons that make normal-looking neuromuscular synapses (White et al., 1992). The axonal diameters of VA motor neurons are similar to those of adjacent VB motor neurons (data not shown). We have now reexamined these EM data to quantitate the number of vesicles in the VA motor neurons. In wild-type animals, the average number of vesicles in a section that contains a VA motor neuron PSD is comparable with the average number of PSD-adjacent vesicles in VB motor neurons (∼40) (Fig.5) (White et al., 1986). In contrast, vesicle number in the active zones of VAs is 40% lower than that of the VBs in unc-4(e120) animals (White et al., 1992). This difference is statistically significant (see Materials and Methods). Vesicle numbers within the intersynaptic regions of VAs and VBs are not significantly different between wild-type and unc-4 animals (data not shown). This finding is important because it excludes the possibility that the reduced number of vesicles that we observe at the presynaptic zones of VA motor neurons in unc-4 mutants is caused by the redistribution of vesicles within the intersynaptic regions as is the case in rab-3 mutants (Nonet et al., 1997). Therefore, we conclude that there are fewer vesicles in the VA motor neurons in unc-4 mutants and that this reduction is correlated with the reduced levels of vesicular protein antibody staining that we have observed in the light microscope.

Fig. 5.

Reduction of presynaptic vesicles in VA motor neurons in unc-4(e120). Vesicles were counted in EM photos of VA and VB cross sections showing PSDs (arrows). A, B, Presynaptic regions of VA (A) and VB (B) motor neurons in wild type are shown. C, D, Fewer vesicles are seen in the presynaptic region of VAs (C) versus VBs (D) in unc-4(e120). The circumference of individual VA and VB motor neuron processes is outlined with a heavy black border. Handwritten numbers on these prints were used to trace individual neurons through these serial sections for reconstruction of the wild-type andunc-4(e120) ventral nerve cords (White et al., 1986,1992). E, Plot of vesicles per PSD in VA and VB motor neurons in wild-type versus two unc-4-mutant animals [unc-4(1), unc-4(2)] is shown. Application of the Mann–Whitney statistical test indicates that the decreased number of vesicles in VA motor neurons inunc-4(e120) is significantly different from that of the VBs (*p < 0.005; **p ≪ 0.001). Error bars indicate SD.

Reduced vesicular protein staining is correlated with functional defects in unc-4 neurons

The ventral nerve cord of the newborn L1 larva contains a simple motor neuron circuit comprised of two classes of excitatory, cholinergic motor neurons (DA and DB) and one class of inhibitory, GABAergic motor neuron (DD) (White et al., 1986; McIntire et al., 1993). [VA motor neurons are not added to the backward movement circuit until the L1–L2 molt (Sulston and Horvitz, 1977)]. Our results showing that SV levels are drastically reduced in the DA motor neurons in unc-4 and unc-37 mutants predict that newly hatched L1 larvae should show impaired movement because of the lowered neurotransmitter signaling capacity of ∼50% of the excitatory ventral cord motor neurons in these animals. We used a liquid “thrashing” assay (Miller et al., 1996) to confirm thatunc-4 and unc-37 L1 larvae are substantially less active than are wild type (Fig. 6). The simplest interpretation of this effect is that the excitatory function of the DA motor neurons is compromised by unc-4 andunc-37 mutations. EM reconstruction of DA motor neurons in the adult indicates that these cells are not miswired inunc-4 mutants and appear otherwise morphologically normal (White et al., 1992). Therefore, we attribute the movement defect ofunc-4 L1 larvae to the observed reduction in neurotransmitter vesicles in these cells.

Fig. 6.

Thrashing rates of L1 animals. The total number of body thrashes was counted during a 2 min period. A thrash was scored as a movement of the animal's body in either the dorsal or ventral direction. Error bars are ±SD. Values that are statistically different from wild type using the Student's t test (p ≪ 0.001) are marked with anasterisk. Results of experiments performed withunc-37(wd17) strains are denoted withgray shading.

Although the SAB motor neurons make clearly visible synapses adjacent to muscles in the head, their role in locomotion has not been defined (J. Duerr, D. H. Hall, and J. Rand, unpublished observations). Recently, Zhao and Nonet (2000) reported that mutants with reduced levels of synaptic transmission show SAB axonal sprouting or branching defects. We have also observed this phenomenon in a significant number (10–15%) of SAB axons of unc-4 and unc-37mutants. Furthermore, of the SAB axons that do exhibit sprouting defects, most also show reduced levels of vesicular protein expression (data not shown). Therefore, our results are consistent with the model in which the lowered levels of neurotransmitter vesicles inunc-4 and unc-37 mutants result in a significant reduction in SAB synaptic activity.

The VC motor neurons innervate the vulval muscles to modulate egg-laying behavior (White et al., 1986; Waggoner et al., 1998). We have observed that unc-4 and unc-37 mutants are mildly resistant to serotonin-induced egg laying (Trent et al., 1983) and also show significantly smaller brood sizes than are seen in wild type (data not shown). These mutant phenotypes could be indicative of VC dysfunction in unc-4 and unc-37 mutants.

The VA motor neurons arise after hatching in the first larval stage and function in the backward movement circuit in larvae and adults (Sulston and Horvitz, 1977; Chalfie et al., 1985). That VA motor neuron activity is affected in unc-4 and unc-37 mutants is evident in the striking backward movement defects that these animals display (White et al., 1992). The inability of unc-4 mutants to crawl backward has been attributed to a miswiring defect in which VA motor neurons receive synaptic inputs from inappropriate command interneurons (White et al., 1992). It is also possible that the depletion of neurotransmitter vesicles in the VAs by unc-4and unc-37 mutations could contribute to this locomotory defect (see Discussion).

UNC-4- and UNC-37-dependent transcriptional repressor function is required to maintain normal levels of vesicular proteins

Having established that neurotransmitter proteins and the vesicles into which they assemble are substantially reduced in specific motor neurons in unc-4 and unc-37 mutants, we next performed experiments to address the molecular mechanism of this effect.

Missense mutations in the UNC-4 engrailed-like repressor domain (eh1) have been shown to inactivate UNC-4 repressor activity and to perturb interactions with UNC-37 (Winnier et al., 1999). We tested two of these eh1 mutations, e2321 and e26, and discovered that both result in reduced levels of UNC-17 and ChAT staining in unc-4 motor neurons (Table 1). Furthermore,unc-37(wd17), an allele-specific Unc-4 suppressor mutation in the UNC-37 WD repeat domain (Miller et al., 1993), restores physical interaction with the e2321-mutant UNC-4 protein and elevates levels of UNC-17 and ChAT staining in e2321-mutant animals (Table 1) (Winnier et al., 1999). However, UNC-17 and ChAT staining is not restored in the null allele unc-4(e120), which is also not suppressible by the unc-37(wd17) mutation (Winnier et al., 1999). Thus, we conclude that UNC-4 regulation of UNC-17 and ChAT protein levels depends on physical interactions with an intact UNC-37/Groucho protein.

The e2321-mutant animals also show reduced thrashing rates as L1 larvae (Fig. 6). The unc-37(wd17) mutation suppresses this effect for the e2321 mutation but not for the nonsuppressible unc-4(e120) null allele. The concomitant effects of the unc-37 suppressor mutation on vesicular protein expression and on L1 motility substantiate a model in which DA motor neuron function depends on UNC-4 interactions with UNC-37.

These results are consistent with a model in which the UNC-4–UNC-37 complex represses transcription of a downstream gene that in turn exerts a negative effect on synaptic vesicle levels. Experiments described in the next section indicate that this UNC-4–UNC-37 target gene (gene x) downregulates SV protein levels via a post-transcriptional mechanism (see Fig. 9).

Vesicular proteins are regulated at a post-transcriptional level

unc-17 and cha-1 are arranged in an operon where they share a common promoter and first untranslated exon (Alfonso et al., 1994) A 3.2 kb promoter element from this upstream region is sufficient to drive expression of GFP in virtually all cholinergic neurons including excitatory motor neurons in the ventral cord (D. Frisby and J. Rand, unpublished observations). Expression of theunc-17-cha-1 promoter:: gfp reporter gene in unc-4 motor neurons is not altered by loss-of-function mutations in either unc-4 orunc-37 (Fig. 7). Thus, theunc-17-cha-1 promoter region does not respond to changes inunc-4 and unc-37 activity. In contrast, expression of unc-17-cha-1promoter:: gfp in these neurons does depend on the cell autonomous activity of the UNC-3 protein that has been shown to function as a regulator of unc-17-cha-1transcription (K. L. Lickteig, D. L. Frisby, J. Duerr, D. M. Miller, and J. Rand, unpublished observations). These findings argue against a mechanism in which unc-4 and unc-37mutations affect unc-17 and cha-1transcription.

Fig. 7.

unc-4 mutations do not affectunc-17-cha-1 promoter:: gfpexpression. The 3.2 kb unc-17-cha-1promoter:: gfp reporter gene is expressed in virtually all cholinergic neurons. A, B, Lateral view of GFP-positive DA and DB motor neurons in both wild-type andunc-4(e120) L1 larvae. C, D, Lateral view of L2 stage larva showing equivalent levels of GFP expression in postembryonically derived VA and VB motor neurons in wild-type and unc-4(e120) animals. Thearrowhead denotes AS motor neurons that are seen in both wild-type and unc-4 animals. Asterisksmark gut autofluorescence. Scale bars, 10 μm.

To determine whether other vesicular proteins are also regulated at a post-transcriptional level by unc-4 and unc-37, we evaluated expression of a GFP-tagged Synaptobrevin driven by the unc-4 promoter (M. L. Nonet, 1999). This construct (unc-4p:: SNB-1:: gfp) contains the full-length Synaptobrevin protein with a C-terminal GFP tag. Expression of this transgene produces a punctate pattern of GFP staining that is correlated with the localization of SNB-1:: GFP at the PSDs ofunc-4 motor neurons. This pattern is especially well resolved in the SAB processes in the head and in VC axons that exit the nerve cord to innervate vulval muscles (Fig.8). To determine whether the regulation of Synaptobrevin by unc-4 and unc-37 is independent of the Synaptobrevin promoter, we placed theunc-4p:: SNB-1:: gfp construct inunc-4- and unc-37-mutant backgrounds. In these animals, expression of GFP-tagged Synaptobrevin is clearly reduced in the axonal projections of the VC and SAB motor neurons (Fig. 8). A similar reduction is seen for UNC-17 and ChAT antibody levels in these cells in unc-4 and unc-37 mutants (compare Table1, Fig. 8E). Because unc-4 expression is not regulated by unc-4 or unc-37 (Miller et al., 1993; Miller and Niemeyer, 1995), it follows that the decreased levels of SNB-1:: GFP in these mutants is not a result ofunc-4 or unc-37 regulation of theunc-4 promoter. Therefore, unc-4 andunc-37 regulation of Synaptobrevin expression does not occur via a transcriptional mechanism but must depend on some feature of the Synaptobrevin-transcribed sequence. This finding parallels the observation above that UNC-17 and ChAT are also likely to be regulated by unc-4 and unc-37 at a post-transcriptional level and therefore favors a model in which all of the affected vesicular proteins are similarly regulated.

Fig. 8.

GFP-tagged Synaptobrevin is downregulated inunc-4-mutant motor neurons. The unc-4promoter was used to drive expression of SNB-1:: GFP (M. L. Nonet, 1999). A–D, Punctate SNB-1:: GFP staining is seen in SAB (A) and VC processes (C) in wild-type animals but is either reduced (B) or eliminated (D) in these neurons in unc-37(e262) mutants (arrows). Images are compressed stacks of optical sections obtained in the confocal microscope. E, Histogram of SNB-1:: GFP expression in VC and SAB motor neurons shows decreased GFP expression in unc-4(wd1) andunc-37(e262) mutants. Two sets of VC vulval synapses (anterior vs posterior) were scored per animal. Staining of these VC varicosities was usually correlated with staining in the adjacent VC4 and VC5 somata (n = 60 animals). Four SAB processes were scored per animal (n = 80 animals). Scale bars, 10 μm.

Vesicular protein levels are developmentally regulated by unc-4

We performed temperature-shift experiments with the temperature-sensitive mutant unc-4(e2322ts) (Miller et al., 1992) to define the developmental periods in which unc-4 is required to maintain wild-type levels of the vesicular protein UNC-17 in DA and VA motor neurons. DA motor neurons are generated in the embryo; VA motor neurons arise after hatching in the late L1 larva (Sulston and Horvitz, 1977; Sulston et al., 1983). Whene2322ts animals are maintained at the permissive temperature (16°C) throughout development, both the DA and VA motor neurons express high levels of UNC-17 protein (Table3). Growth at the restrictive temperature (25°C) results in substantially lower levels of UNC-17 expression (18% of DAs and 6% of VAs). Temperature-shift experiments have revealed, however, that unc-4 function is specifically required during the early developmental periods in which DA and VA motor neurons differentiate but is not necessary in older larvae or adults for maintaining normal levels of UNC-17 protein. For example, exposure of L1 and L2 larvae to 25°C results in UNC-17 staining in only 30% of the VAs, whereas exposure of older animals (L3 to adult) does not reduce UNC-17 expression in these cells. DA motor neurons are similarly sensitive to restrictive temperature. In this case, however, DAs in both embryos and L1–L2 larvae are affected with only ∼20% of the DAs showing UNC-17 expression; exposure of older animals to the restrictive temperature has no effect (Table 3).

View this table:

Table 3.

UNC-17 expression in A-class motor neurons is temperature sensitive in unc-4(e2322ts) animals

DISCUSSION

unc-4 and unc-37 regulate vesicle biogenesis or stability

By what mechanism does the unc-4–unc-37pathway regulate vesicle number in the affected cholinergic motor neurons?

Our results exclude a model in which the decreased number of synaptic vesicles at the PSD is caused by defective anterograde transport or localization in unc-4 and unc-37 mutants. First, we showed that SV protein levels, as assayed in the cell soma of DA and VA motor neurons, are still diminished by unc-4 andunc-37 mutations even when vesicle translocation to the synapse is blocked by a mutation in the unc-104 kinesin gene (Hall and Hedgecock, 1991). Second, our analysis of EM serial sections did not detect any evidence to support a model in which decreased accumulation of SVs at the PSD is caused by their redistribution to intersynaptic regions as occurs in rab-3 null mutants (data not shown) (Nonet et al., 1997). Although RAB-3 protein levels are reduced in unc-4 and unc-37 mutants, we assume that the residual level of RAB-3 expression in the affected motor neurons of these animals is sufficient for normal SV localization.

In an alternative model, vesicle number could be effectively diminished by a dramatic increase in exocytosis. If that were the case, mutations in the unc-13 gene, which is required for vesicle fusion (Richmond et al., 1999), should prevent SV depletion by this mechanism in unc-4 and unc-37 mutants. We observed the opposite result, however; the elimination of unc-13 activity did not restore the SV protein UNC-17 to normal levels in eitherunc-4- or unc-37-mutant backgrounds (data not shown). Thus, our results exclude the possibility that enhanced rates of vesicle exocytosis account for the reduced levels of SV proteins inunc-4- and unc-37-mutant motor neurons.

Lastly, our results argue against the possibility that defective vesicle endocytosis effectively diminishes the steady-state level of PSD-localized vesicles in unc-4 and unc-37mutants. unc-4 mutants are not affected in their expression of UNC-11, a homolog of the endocytic protein AP180 (data not shown). Although AP180 is not essential for endocytosis, it does play a role in regulating clathrin coat size; unc-11-mutant motor neurons show vesicles that are normal in number but with an enlarged diameter (Nonet et al., 1999). EM analysis of unc-4mutants does not reveal these large recycling intermediates or other defects commonly associated with mutations in the endocytic machinery (i.e., increased axonal diameter, membrane infoldings, collared vesicles) (Cremona and De Camilli, 1997). In addition, our results showing that SV levels are decreased even when anterograde transport is blocked by the unc-104 mutation indicate that nascent SVs are affected and therefore argue against the possibility that this reduction is caused by defective endocytosis in unc-4 andunc-37 mutants.

We favor a model in which unc-4 and unc-37regulate some aspect of vesicle biogenesis or stability. Genetic ablation of Synapsin in cultured neurons and in knock-out mice results in a significant reduction of vesicles and SV proteins but not other synaptic membrane or cytosolic proteins (Li et al., 1995; Rosahl et al., 1995; Takei et al., 1995). This effect has been attributed to an increased rate of vesicle turnover. The striking similarity of this phenotype to that of unc-4 and unc-37 mutants is consistent with the formal hypothesis that unc-4 andunc-37 are indirectly responsible for maintaining Synapsin protein levels in specific neurons. The recent identification of aC. elegans Synapsin homolog (Kao et al., 1999) offers the possibility of experimentally testing this model.

Neuronal function depends on post-transcriptional regulation of SV protein expression

Because the unc-4 and unc-37 mutations that reduce SV protein levels are also known to disable the transcriptional repressor activity of the UNC-4 and UNC-37 proteins, it seems unlikely that the UNC-4–UNC-37 complex acts as a direct regulator of SV gene transcription. If that were the case, then SV protein levels should increase in unc-4 andunc-37 mutants as opposed to the substantial reduction of vesicular proteins that we observe in these animals. Thus, we propose that the UNC-4 and UNC-37 normally function to repress transcription of an intermediate gene (gene-x) that in turn exerts a negative effect on SV levels (Fig. 9). In this model, mutations that disable either unc-4 orunc-37 result in inappropriate expression ofgene-x that then downregulates SV proteins. Although the molecular identity of the putative gene-x is unknown, our results indicate that it is likely to act via a post-transcriptional mechanism.

Fig. 9.

Model. A, UNC-4 and UNC-37 function together to repress an intermediate gene (gene-x) that negatively regulates vesicle number. In unc-4 orunc-37 loss-of-function mutants, gene-xis derepressed, thereby leading to decreased levels of synaptic vesicles and SV proteins. B, In wild-type animals, VA motor neurons receive input from specific command interneurons (interneuron A). In unc-4 andunc-37 mutants, VA motor neurons exhibit a reduced number of SVs and receive input from a different set of presynaptic partners (interneuron B) (White et al., 1992) (Hall, German, and Miller, unpublished observations).

Studies of SV biogenesis in vertebrate neurons have revealed multiple post-transcriptional levels of control. For example, in cultured hippocampal neurons, Synaptophysin expression appears to depend on the rate of mRNA translation, whereas the accumulation of Synaptotagmin, Synaptobrevin, and Synapsin is linked to increased protein half-life as these neurons develop. The rates of SV assembly and SV protein degradation may be interdependent; SV creation relies on the available pool of SV proteins, and conversely, precursor proteins that are not rapidly incorporated into an SV may be degraded (Daly and Ziff, 1997). Wide variations in SV number and quantal content among different classes of neurons argue that developmental and homeostatic control of vesicle-dependent signaling capacity is inherently important to neuronal physiology (White et al., 1986; Jia et al., 1993;Merchan-Perez and Liberman, 1996). Tight regulation of SV levels could be provided by the opposing effects of both positively and negatively acting pathways. In this instance, the normal function ofunc-4 and unc-37 is to inhibit the activity of a negatively acting pathway that acts, via a post-transcriptional mechanism, to decrease the levels of SV proteins and the vesicles that they comprise in specific cholinergic motor neurons.

The negative effect of the unc-4 mutation on cholinergic SVs also applies to other classes of neurotransmitter vesicles. Antibody-staining experiments have detected reduced expression of the neuropeptide FMRFamide (Li and Chalfie, 1990; Schinkmann and Li, 1992) (C. Li, personal communication) and the vesicular monoamine transporter in the VC motor neurons (Duerr et al., 1999) (Duerr, unpublished observations). These observations indicate thatunc-4 and unc-37 may mediate a general event in the creation or maintenance of all types of neurotransmitter vesicles.

Experiments with a temperature-sensitive unc-4 mutant indicate that SV levels depend on unc-4 function during a brief period of early development but do not require unc-4activity in the adult. This finding may mean that unc-4 andunc-37 mediate a key event during the differentiation of an affected motor neuron that then sets the steady-state level of SV proteins in the mature cell (see below).

Motor neuron dysfunction contributes to the Unc-4 movement defect

Body wall muscle excitation during backward locomotion has been attributed to the coordinated activities of cholinergic DA and VA motor neurons and the command interneurons (AVA, AVD, and AVE) that drive them (Chalfie et al., 1985). The striking backward movement defect shown by unc-4 and unc-37 loss-of-function mutants is correlated with the loss of normal inputs to VA motor neurons. These synapses are replaced with gap junctions from a command interneuron (AVB) that usually mediates forward locomotion (White et al., 1992) (Hall, German, and Miller, unpublished observations). Recent results suggest that the simple elimination of synaptic inputs to the VAs may be insufficient to account for the total abrogation of backward movement in unc-4 mutants; genetic ablation of the “backward command interneurons” (AVA, AVD, and AVE) retards but does not block reverse locomotion (Zheng et al., 1999). Our finding that the neurotransmitter signaling capacity of VA motor neurons is also reduced in unc-4 mutants may provide an explanation for the enhanced severity of the Unc-4 backward movement defect.

Does the vesicular signaling capacity of VA motor neurons specify presynaptic inputs or vice versa?

Experiments with a temperature-sensitive unc-4 mutant indicate that both the input and output defects of VA motor neurons are caused by the loss of unc-4 activity during early larval development. VA motor neurons are generated during the first larval stage (L1) (Sulston and Horvitz, 1977). Although the adult pattern of presynaptic connections is established before the L1–L2 molt (J. White, personal communication), additional motor neuron inputs are probably added during subsequent larval development to accompany dramatic increases in neuronal size (Rongo and Kaplan, 1999). Ifunc-4 activity is effectively turned off during this critical period (L2 to mid-L3) by exposing the unc-4tsallele to a restrictive temperature, then adult animals show a strong backward movement defect (Miller et al., 1992) as well as a reduction in synaptic vesicles in the VAs. The temporal correlation of the miswiring event and the reduction in VA signaling capacity is suggestive of a causal relationship between these defects.

In one model, the change in synaptic inputs triggers the depletion of synaptic vesicles in the VAs. However, an identical mechanism could not account for the loss of synaptic vesicles in the DAs because these motor neurons are not miswired in unc-4 mutants. Perhaps theunc-4 mutation induces transient miswiring of the DAs (and SAB and VC motor neurons), and this brief loss of normal inputs is sufficient to induce the synaptic vesicle defect.

It is also possible that the opposite mechanism applies. The loss of vesicular proteins in the VA motor neurons results in an altered pattern of presynaptic inputs. This model supposes that either the vesicular proteins or the signaling activity that they provide may define presynaptic specificity. Ample evidence exists for models in which both the strength and selectivity of presynaptic connections can be influenced by retrograde signals from the postsynaptic partner. The mechanisms of these effects, however, are primarily unknown (Fitzsimonds and Poo, 1998). Recent experiments have shown thatN-ethylmaleimide-sensitive factor (NSF), a cytosolic protein involved in vesicular fusion, may be involved in targeting glutamate receptors to the postsynaptic membrane (Nishimune et al., 1998; Osten et al., 1998; Song et al., 1998). In addition, the application of inhibitors of NSF activity or cleavage of the SNARE protein Synaptobrevin by microinjection or cell autonomous expression of tetanus toxin can reduce the strength of synaptic inputs to the affected neurons (Lledo et al., 1998; Baines et al., 1999). These studies indicate that SV fusion may be important for the correct localization of receptors at the postsynaptic membrane in addition to providing neurotransmitter signaling capacity at the presynaptic density. It is conceivable that a similar effect on the localization of key receptor or marker proteins in the VA postsynaptic membrane could effectively specify presynaptic inputs. This model predicts that VA motor neurons should adopt the VB pattern of synaptic inputs in mutants in which SV accumulation or activity is reduced (Jorgensen et al., 1995). This model also assumes, of course, that the loss of SV activity in other classes of motor neurons (e.g., the DAs) is not sufficient to alter presynaptic inputs.

Lastly, it is conceivable that the loss of synaptic vesicles and the rewiring of VA motor neurons are independently induced by theunc-4 mutation and have no mechanistic relationship other than the common link to unc-4 activity. Perhaps the most effective way to resolve this question is to identify theunc-4 target genes that mediate these events.

Footnotes

This work was supported by National Institutes of Health Grants MH12260 (K.M.L.), NS26115 (D.M.M.), GM38679 (J.B.R.), and NCRR12596 (D.H.H.) and OCAST Grant HN3-023 (J.S.D.). We thank R. Blakely and members of the D. M. Miller and D. Greenstein laboratories for helpful discussions; M. Nonet for antibodies against RAB-3, Synaptobrevin, and Syntaxin and for the unc-4promoter-SNB-1::GFP plasmid; A. Alfonso for theunc-11(n2954) strain and UNC-11 antibody; John White for wild-type and unc-4(e120) electron micrographs; Tylon Stephney for scanning EM prints; and Chris Li for communicating unpublished data.
Correspondence should be addressed to Dr. David M. Miller, III, C2310 Medical Center North, 1161 21st Avenue South, Vanderbilt University, Nashville, TN 37232. E-mail: david.miller{at}mcmail.vanderbilt.edu.

REFERENCES

↵
1. Alfonso A,
2. Grundahl K,
3. Duerr JS,
4. Han HP,
5. Rand JB
(1993) The Caenorhabditis elegans unc-17 gene: a putative vesicular acetylcholine transporter. Science 261:617–619.
OpenUrl Abstract/FREE Full Text
↵
1. Alfonso A,
2. Grundahl K,
3. McManus JR,
4. Asbury JM,
5. Rand JB
(1994) Alternative splicing leads to two cholinergic proteins in Caenorhabditis elegans. J Mol Biol 241:627–630.
OpenUrl CrossRef PubMed
↵
1. Baines RA,
2. Robinson SG,
3. Fujioka M,
4. Jaynes JB,
5. Bate M
(1999) Postsynaptic expression of tetanus toxin light chain blocks synaptogenesis in Drosophila. Curr Biol 9:1267–1270.
OpenUrl CrossRef PubMed
↵
1. Bergmann M,
2. Lahr G,
3. Mayerhofer A,
4. Gratzl M
(1991) Expression of synaptophysin during the prenatal development of the rat spinal cord: correlation with basic differentiation processes of neurons. Neuroscience 42:569–582.
OpenUrl CrossRef PubMed
↵
1. Brenner S
(1974) The genetics of Caenorhabditis elegans. Genetics 77:71–94.
OpenUrl Abstract/FREE Full Text
↵
1. Calakos N,
2. Scheller RH
(1996) Synaptic vesicle biogenesis, docking, and fusion: a molecular description. Physiol Rev 76:1–29.
OpenUrl PubMed
↵
1. Chalfie M,
2. Sulston JE,
3. White JG,
4. Southgate E,
5. Thompson JN,
6. Brenner S
(1985) The neural circuit for touch sensitivity in Caenorhabditis elegans. J Neurosci 5:956–964.
OpenUrl Abstract/FREE Full Text
↵
1. Clark DV,
2. Suleman DS,
3. Beckenbach KA,
4. Gilchrist EJ,
5. Baillie DL
(1995) Molecular cloning and characterization of the dpy-20 gene of Caenorhabditis elegans. Mol Gen Genet 247:367–378.
OpenUrl CrossRef PubMed
↵
1. Cremona O,
2. De Camilli P
(1997) Synaptic vesicle endocytosis. Curr Opin Neurobiol 7:323–330.
OpenUrl CrossRef PubMed
↵
1. Daly C,
2. Ziff EB
(1997) Post-transcriptional regulation of synaptic vesicle protein expression and the developmental control of synaptic vesicle formation. J Neurosci 17:2365–2375.
OpenUrl Abstract/FREE Full Text
↵
1. Deans ZC,
2. Dawson SJ,
3. Kilimann MW,
4. Wallace D,
5. Wilson MC,
6. Latchman DS
(1997) Differential regulation of genes encoding synaptic proteins by the Oct-2 transcription factor. Brain Res Mol Brain Res 51:1–7.
OpenUrl PubMed
↵
1. Duerr JS,
2. Frisby DL,
3. Gaskin J,
4. Duke A,
5. Asermely K,
6. Huddleston D,
7. Eiden LE,
8. 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.
OpenUrl Abstract/FREE Full Text
↵
1. Fitzsimonds RM,
2. Poo MM
(1998) Retrograde signaling in the development and modification of synapses. Physiol Rev 78:143–170.
OpenUrl PubMed
↵
1. Geppert M,
2. Bolshakov VY,
3. Siegelbaum SA,
4. Takei K,
5. De Camilli P,
6. Hammer RE,
7. Sudhof TC
(1994) The role of Rab3A in neurotransmitter release. Nature 369:493–497.
OpenUrl CrossRef PubMed
↵
1. Hall DH,
2. Hedgecock ED
(1991) Kinesin-related gene unc-104 is required for axonal transport of synaptic vesicles in C. elegans. Cell 65:837–847.
OpenUrl CrossRef PubMed
↵
1. Hosono R,
2. Hekimi S,
3. Kamiya Y,
4. Sassa T,
5. Murakami S,
6. Nishiwaki K,
7. Miwa J,
8. Taketo A,
9. Kodaira KI
(1992) The unc-18 gene encodes a novel protein affecting the kinetics of acetylcholine metabolism in the nematode Caenorhabditis elegans. J Neurochem 58:1517–1525.
OpenUrl CrossRef PubMed
↵
1. Jia XX,
2. Gorczyca M,
3. Budnik V
Ultrastructure of neuromuscular junctions in Drosophila: comparison of wild type and mutants with increased excitability. J Neurobiol 24 1993 1025 1044 [Erratum(1994)25:893–895]
OpenUrl CrossRef PubMed
↵
1. Jin Y,
2. Jorgensen E,
3. Hartwieg E,
4. Horvitz HR
(1999) The Caenorhabditis elegans gene unc-25 encodes glutamic acid decarboxylase and is required for synaptic transmission but not synaptic development. J Neurosci 19:539–548.
OpenUrl Abstract/FREE Full Text
↵
1. Jorgensen EM,
2. Hartwieg E,
3. Schuske K,
4. Nonet ML,
5. Jin Y,
6. Horvitz HR
(1995) Defective recycling of synaptic vesicles in synaptotagmin mutants of Caenorhabditis elegans. Nature 378:196–199.
OpenUrl CrossRef PubMed
↵
1. Kao HT,
2. Porton B,
3. Hilfiker S,
4. Stefani G,
5. Pieribone VA,
6. DeSalle R,
7. Greengard P
(1999) Molecular evolution of the synapsin gene family. J Exp Zool 285:360–377.
OpenUrl CrossRef PubMed
↵
1. Li C,
2. Chalfie M
(1990) Organogenesis in C. elegans: positioning of neurons and muscles in the egg-laying system. Neuron 4:681–695.
OpenUrl CrossRef PubMed
↵
1. Li L,
2. Chin LS,
3. Shupliakov O,
4. Brodin L,
5. Sihra TS,
6. Hvalby O,
7. Jensen V,
8. Zheng D,
9. McNamara JO,
10. Greengard P,
11. Andersen P
(1995) Impairment of synaptic vesicle clustering and of synaptic transmission, and increased seizure propensity, in synapsin I-deficient mice. Proc Natl Acad Sci USA 92:9235–9239.
OpenUrl Abstract/FREE Full Text
↵
1. Lledo PM,
2. Zhang X,
3. Sudhof TC,
4. Malenka RC,
5. Nicoll RA
(1998) Postsynaptic membrane fusion and long-term potentiation. Science 279:399–403.
OpenUrl Abstract/FREE Full Text
↵
1. Lloyd TE,
2. Verstreken P,
3. Ostrin EJ,
4. Phillippi A,
5. Lichtarge O,
6. Bellen HJ
(2000) A genome-wide search for synaptic vesicle cycle proteins in Drosophila. Neuron 26:45–50.
OpenUrl CrossRef PubMed
↵
1. Lou X,
2. Bixby JL
(1993) Coordinate and noncoordinate regulation of synaptic vesicle protein genes during embryonic development. Dev Biol 159:327–337.
OpenUrl CrossRef PubMed
↵
1. McIntire SL,
2. Jorgensen E,
3. Kaplan J,
4. Horvitz HR
(1993) The GABAergic nervous system of Caenorhabditis elegans. Nature 364:337–341.
OpenUrl CrossRef PubMed
↵
1. Mello C,
2. Fire A
(1995) DNA transformation. Methods Cell Biol 48:451–482.
OpenUrl CrossRef PubMed
↵
1. Melloni RH Jr.,
2. Apostolides PJ,
3. Hamos JE,
4. DeGennaro LJ
(1994) Dynamics of synapsin I gene expression during the establishment and restoration of functional synapses in the rat hippocampus. Neuroscience 58:683–703.
OpenUrl CrossRef PubMed
↵
1. Merchan-Perez A,
2. Liberman MC
(1996) Ultrastructural differences among afferent synapses on cochlear hair cells: correlations with spontaneous discharge rate. J Comp Neurol 371:208–221.
OpenUrl CrossRef PubMed
↵
1. Miller DM,
2. Shen MM,
3. Shamu CE,
4. Burglin TR,
5. Ruvkun G,
6. Dubois ML,
7. Ghee M,
8. Wilson L
(1992) C. elegans unc-4 gene encodes a homeodomain protein that determines the pattern of synaptic input to specific motor neurons. Nature 355:841–845.
OpenUrl CrossRef PubMed
↵
1. Miller DM,
2. Desai N,
3. Hardin D,
4. Piston DW,
5. Patterson GH,
6. Fleenor J,
7. Xu SQ,
8. Fire A
(1999) A two-color GFP expression system for C. elegans. Biotechniques 26:914–921.
OpenUrl PubMed
↵
1. Miller DM III.,
2. Niemeyer CJ
(1995) Expression of the unc-4 homeoprotein in Caenorhabditis elegans motor neurons specifies presynaptic input. Development 121:2877–2866.
OpenUrl Abstract
↵
1. Miller DM III.,
2. Niemeyer CJ,
3. Chitkara P
(1993) Dominant unc-37 mutations suppress the movement defect of a homeodomain mutation in unc-4, a neural specificity gene in Caenorhabditis elegans. Genetics 135:741–753.
OpenUrl Abstract/FREE Full Text
↵
1. Miller KG,
2. Alfonso A,
3. Nguyen M,
4. Crowell JA,
5. Johnson CD,
6. Rand JB
(1996) A genetic selection for Caenorhabditis elegans synaptic transmission mutants. Proc Natl Acad Sci USA 93:12593–12598.
OpenUrl Abstract/FREE Full Text
↵
1. Nishimune A,
2. Isaac JT,
3. Molnar E,
4. Noel J,
5. Nash SR,
6. Tagaya M,
7. Collingridge GL,
8. Nakanishi S,
9. Henley JM
(1998) NSF binding to GluR2 regulates synaptic transmission. Neuron 21:87–97.
OpenUrl CrossRef PubMed
1. Nonet M
(1999) Studying mutants that affect neurotransmitter release in C. elegans. in Neurotransmitter release, ed Bellen HJ (Oxford UP, New York), pp 265–303.
↵
1. Nonet ML
(1999) Visualization of synaptic specializations in live C. elegans with synaptic vesicle protein-GFP fusions. J Neurosci Methods 89:33–40.
OpenUrl CrossRef PubMed
↵
1. Nonet ML,
2. Grundahl K,
3. Meyer BJ,
4. Rand JB
(1993) Synaptic function is impaired but not eliminated in C. elegans mutants lacking synaptotagmin. Cell 73:1291–1305.
OpenUrl CrossRef PubMed
↵
1. Nonet ML,
2. Staunton JE,
3. Kilgard MP,
4. Fergestad T,
5. Hartwieg E,
6. Horvitz HR,
7. Jorgensen EM,
8. Meyer BJ
(1997) Caenorhabditis elegans rab-3 mutant synapses exhibit impaired function and are partially depleted of vesicles. J Neurosci 17:8061–8073.
OpenUrl Abstract/FREE Full Text
↵
1. Nonet ML,
2. Saifee O,
3. Zhao H,
4. Rand JB,
5. Wei L
(1998) Synaptic transmission deficits in Caenorhabditis elegans synaptobrevin mutants. J Neurosci 18:70–80.
OpenUrl Abstract/FREE Full Text
↵
1. Nonet ML,
2. Holgado AM,
3. Brewer F,
4. Serpe CJ,
5. Norbeck BA,
6. Holleran J,
7. Wei L,
8. Hartwieg E,
9. Jorgensen EM,
10. Alfonso A
(1999) UNC-11, a Caenorhabditis elegans AP180 homologue, regulates the size and protein composition of synaptic vesicles. Mol Biol Cell 10:2343–2360.
OpenUrl Abstract/FREE Full Text
↵
1. Ogawa H,
2. Harada S,
3. Sassa T,
4. Yamamoto H,
5. Hosono R
(1998) Functional properties of the unc-64 gene encoding a Caenorhabditis elegans syntaxin. J Biol Chem 273:2192–2198.
OpenUrl Abstract/FREE Full Text
↵
1. Osten P,
2. Srivastava S,
3. Inman GJ,
4. Vilim FS,
5. Khatri L,
6. Lee LM,
7. States BA,
8. Einheber S,
9. Milner TA,
10. Hanson PI,
11. Ziff EB
(1998) The AMPA receptor GluR2 C terminus can mediate a reversible, ATP-dependent interaction with NSF and alpha- and beta-SNAPs. Neuron 21:99–110.
OpenUrl CrossRef PubMed
↵
1. Petersohn D,
2. Schoch S,
3. Brinkmann DR,
4. Thiel G
(1995) The human synapsin II gene promoter. Possible role for the transcription factor zif268/egr-1, polyoma enhancer activator 3, and AP2. J Biol Chem 270:24361–24369.
OpenUrl Abstract/FREE Full Text
↵
1. Pflugrad A,
2. Meir JY-J,
3. Barnes TM,
4. Miller DM III.
(1997) The Groucho-like transcription factor UNC-37 functions with the neural specificity gene unc-4 to govern motor neuron identity in C. elegans. Development 124:1699–1709.
OpenUrl Abstract
↵
1. Richmond JE,
2. Davis WS,
3. Jorgensen EM
(1999) UNC-13 is required for synaptic vesicle fusion in C. elegans. Nat Neurosci 2:959–964.
OpenUrl CrossRef PubMed
↵
1. Rongo C,
2. Kaplan JM
(1999) CaMKII regulates the density of central glutamatergic synapses in vivo. Nature 402:195–199.
OpenUrl CrossRef PubMed
↵
1. Rosahl TW,
2. Spillane D,
3. Missler M,
4. Herz J,
5. Selig DK,
6. Wolff JR,
7. Hammer RE,
8. Malenka RC,
9. Sudhof TC
(1995) Essential functions of synapsins I and II in synaptic vesicle regulation. Nature 375:488–493.
OpenUrl CrossRef PubMed
↵
1. Rothman JE
(1994) Mechanisms of intracellular protein transport. Nature 372:55–63.
OpenUrl CrossRef PubMed
↵
1. Saifee O,
2. Wei L,
3. Nonet ML
(1998) The Caenorhabditis elegans unc-64 locus encodes a syntaxin that interacts genetically with synaptobrevin. Mol Biol Cell 9:1235–1252.
OpenUrl Abstract/FREE Full Text
↵
1. Schinkmann K,
2. Li C
(1992) Localization of FMRFamide-like peptides in Caenorhabditis elegans. J Comp Neurol 316:251–260.
OpenUrl CrossRef PubMed
↵
1. Smith MD,
2. Dawson SJ,
3. Latchman DS
(1997) The Brn-3a transcription factor induces neuronal process outgrowth and the coordinate expression of genes encoding synaptic proteins. Mol Cell Biol 17:345–354.
OpenUrl Abstract/FREE Full Text
↵
1. Song I,
2. Kamboj S,
3. Xia J,
4. Dong H,
5. Liao D,
6. Huganir RL
(1998) Interaction of the N-ethylmaleimide-sensitive factor with AMPA receptors. Neuron 21:393–400.
OpenUrl CrossRef PubMed
↵
1. Sulston J,
2. Hodgkin J
(1988) Methods. in The nematode Caenorhabditis elegans, ed Wood WB (Cold Spring Harbor Laboratory, Cold Spring Harbor, NY), pp 587–606.
↵
1. Sulston JE,
2. Horvitz HR
(1977) Post-embryonic cell lineages of the nematode, Caenorhabditis elegans. Dev Biol 56:110–156.
OpenUrl CrossRef PubMed
↵
1. Sulston JE,
2. Schierenberg E,
3. White JG,
4. Thomson JN
(1983) The embryonic cell lineage of the nematode Caenorhabditis elegans. Dev Biol 100:64–119.
OpenUrl CrossRef PubMed
↵
1. Takei Y,
2. Harada A,
3. Takeda S,
4. Kobayashi K,
5. Terada S,
6. Noda T,
7. Takahashi T,
8. Hirokawa N
(1995) Synapsin I deficiency results in the structural change in the presynaptic terminals in the murine nervous system. J Cell Biol 131:1789–1800.
OpenUrl Abstract/FREE Full Text
↵
1. Trent C,
2. Tsung N,
3. Horvitz H
(1983) Egg-laying defective mutants of the nematode Caenorhabditis elegans. Genetics 104:619–647.
OpenUrl Abstract/FREE Full Text
↵
1. Waggoner LE,
2. Zhou GT,
3. Schafer RW,
4. Schafer WR
(1998) Control of alternative behavioral states by serotonin in Caenorhabditis elegans. Neuron 21:203–214.
OpenUrl CrossRef PubMed
↵
1. White JG,
2. Southgate E,
3. Thomson JN,
4. Brenner S
(1976) Structure of the ventral nerve cord of Caenorhabditis elegans. Philos Trans R Soc Lond [Biol] 275:327–348.
OpenUrl CrossRef PubMed
↵
1. White JG,
2. Southgate E,
3. Thomson JN,
4. Brenner S
(1986) The structure of the nervous system of the nematode Caenorhabditis elegans. Philos Trans R Soc Lond [Biol] 314:1–340.
OpenUrl CrossRef
↵
1. White JG,
2. Southgate E,
3. Thomson JN
(1992) Mutations in the Caenorhabditis elegans unc-4 gene alter the synaptic input to ventral cord motor neurons. Nature 355:838–841.
OpenUrl CrossRef PubMed
↵
1. Winnier AR,
2. Meir JY,
3. Ross JM,
4. Tavernarakis N,
5. Driscoll M,
6. Ishihara T,
7. Katsura I,
8. Miller DM III.
(1999) UNC-4/UNC-37-dependent repression of motor neuron-specific genes controls synaptic choice in Caenorhabditis elegans. Genes Dev 13:2774–2786.
OpenUrl Abstract/FREE Full Text
↵
1. Zhao H,
2. Nonet ML
(2000) A retrograde signal is involved in activity-dependent remodeling at a C. elegans neuromuscular junction. Development 127:1253–1266.
OpenUrl Abstract
↵
1. Zheng Y,
2. Brockie PJ,
3. Mellem JE,
4. Madsen DM,
5. Maricq AV
(1999) Neuronal control of locomotion in C. elegans is modified by a dominant mutation in the GLR-1 ionotropic glutamate receptor. Neuron 24:347–361.
OpenUrl CrossRef PubMed

In this issue

View Full Page PDF

Citation Tools

Respond to this article

Request Permissions

Keywords

Cited By...

ARTICLE

Show more ARTICLE

Development/Plasticity/Repair

Show more Development/Plasticity/Repair

[1] ↵
Alfonso A,
Grundahl K,
Duerr JS,
Han HP,
Rand JB
(1993) The Caenorhabditis elegans unc-17 gene: a putative vesicular acetylcholine transporter. Science 261:617–619.
OpenUrl Abstract/FREE Full Text

[2] Alfonso A,

[3] Grundahl K,

[4] Duerr JS,

[5] Han HP,

[6] Rand JB

[7] ↵
Alfonso A,
Grundahl K,
McManus JR,
Asbury JM,
Rand JB
(1994) Alternative splicing leads to two cholinergic proteins in Caenorhabditis elegans. J Mol Biol 241:627–630.
OpenUrl CrossRef PubMed

[8] Alfonso A,

[9] Grundahl K,

[10] McManus JR,

[11] Asbury JM,

[12] Rand JB

[13] ↵
Baines RA,
Robinson SG,
Fujioka M,
Jaynes JB,
Bate M
(1999) Postsynaptic expression of tetanus toxin light chain blocks synaptogenesis in Drosophila. Curr Biol 9:1267–1270.
OpenUrl CrossRef PubMed

[14] Baines RA,

[15] Robinson SG,

[16] Fujioka M,

[17] Jaynes JB,

[18] Bate M

[19] ↵
Bergmann M,
Lahr G,
Mayerhofer A,
Gratzl M
(1991) Expression of synaptophysin during the prenatal development of the rat spinal cord: correlation with basic differentiation processes of neurons. Neuroscience 42:569–582.
OpenUrl CrossRef PubMed

[20] Bergmann M,

[21] Lahr G,

[22] Mayerhofer A,

[23] Gratzl M

[24] ↵
Brenner S
(1974) The genetics of Caenorhabditis elegans. Genetics 77:71–94.
OpenUrl Abstract/FREE Full Text

[25] Brenner S

[26] ↵
Calakos N,
Scheller RH
(1996) Synaptic vesicle biogenesis, docking, and fusion: a molecular description. Physiol Rev 76:1–29.
OpenUrl PubMed

[27] Calakos N,

[28] Scheller RH

[29] ↵
Chalfie M,
Sulston JE,
White JG,
Southgate E,
Thompson JN,
Brenner S
(1985) The neural circuit for touch sensitivity in Caenorhabditis elegans. J Neurosci 5:956–964.
OpenUrl Abstract/FREE Full Text

[30] Chalfie M,

[31] Sulston JE,

[32] White JG,

[33] Southgate E,

[34] Thompson JN,

[35] Brenner S

[36] ↵
Clark DV,
Suleman DS,
Beckenbach KA,
Gilchrist EJ,
Baillie DL
(1995) Molecular cloning and characterization of the dpy-20 gene of Caenorhabditis elegans. Mol Gen Genet 247:367–378.
OpenUrl CrossRef PubMed

[37] Clark DV,

[38] Suleman DS,

[39] Beckenbach KA,

[40] Gilchrist EJ,

[41] Baillie DL

[42] ↵
Cremona O,
De Camilli P
(1997) Synaptic vesicle endocytosis. Curr Opin Neurobiol 7:323–330.
OpenUrl CrossRef PubMed

[43] Cremona O,

[44] De Camilli P

[45] ↵
Daly C,
Ziff EB
(1997) Post-transcriptional regulation of synaptic vesicle protein expression and the developmental control of synaptic vesicle formation. J Neurosci 17:2365–2375.
OpenUrl Abstract/FREE Full Text

[46] Daly C,

[47] Ziff EB

[48] ↵
Deans ZC,
Dawson SJ,
Kilimann MW,
Wallace D,
Wilson MC,
Latchman DS
(1997) Differential regulation of genes encoding synaptic proteins by the Oct-2 transcription factor. Brain Res Mol Brain Res 51:1–7.
OpenUrl PubMed

[49] Deans ZC,

[50] Dawson SJ,

[51] Kilimann MW,

[52] Wallace D,

[53] Wilson MC,

[54] Latchman DS

[55] ↵
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.
OpenUrl Abstract/FREE Full Text

[56] Duerr JS,

[57] Frisby DL,

[58] Gaskin J,

[59] Duke A,

[60] Asermely K,

[61] Huddleston D,

[62] Eiden LE,

[63] Rand JB

[64] ↵
Fitzsimonds RM,
Poo MM
(1998) Retrograde signaling in the development and modification of synapses. Physiol Rev 78:143–170.
OpenUrl PubMed

[65] Fitzsimonds RM,

[66] Poo MM

[67] ↵
Geppert M,
Bolshakov VY,
Siegelbaum SA,
Takei K,
De Camilli P,
Hammer RE,
Sudhof TC
(1994) The role of Rab3A in neurotransmitter release. Nature 369:493–497.
OpenUrl CrossRef PubMed

[68] Geppert M,

[69] Bolshakov VY,

[70] Siegelbaum SA,

[71] Takei K,

[72] De Camilli P,

[73] Hammer RE,

[74] Sudhof TC

[75] ↵
Hall DH,
Hedgecock ED
(1991) Kinesin-related gene unc-104 is required for axonal transport of synaptic vesicles in C. elegans. Cell 65:837–847.
OpenUrl CrossRef PubMed

[76] Hall DH,

[77] Hedgecock ED

[78] ↵
Hosono R,
Hekimi S,
Kamiya Y,
Sassa T,
Murakami S,
Nishiwaki K,
Miwa J,
Taketo A,
Kodaira KI
(1992) The unc-18 gene encodes a novel protein affecting the kinetics of acetylcholine metabolism in the nematode Caenorhabditis elegans. J Neurochem 58:1517–1525.
OpenUrl CrossRef PubMed

[79] Hosono R,

[80] Hekimi S,

[81] Kamiya Y,

[82] Sassa T,

[83] Murakami S,

[84] Nishiwaki K,

[85] Miwa J,

[86] Taketo A,

[87] Kodaira KI

[88] ↵
Jia XX,
Gorczyca M,
Budnik V
Ultrastructure of neuromuscular junctions in Drosophila: comparison of wild type and mutants with increased excitability. J Neurobiol 24 1993 1025 1044 [Erratum(1994)25:893–895]
OpenUrl CrossRef PubMed

[89] Jia XX,

[90] Gorczyca M,

[91] Budnik V

[92] ↵
Jin Y,
Jorgensen E,
Hartwieg E,
Horvitz HR
(1999) The Caenorhabditis elegans gene unc-25 encodes glutamic acid decarboxylase and is required for synaptic transmission but not synaptic development. J Neurosci 19:539–548.
OpenUrl Abstract/FREE Full Text

[93] Jin Y,

[94] Jorgensen E,

[95] Hartwieg E,

[96] Horvitz HR

[97] ↵
Jorgensen EM,
Hartwieg E,
Schuske K,
Nonet ML,
Jin Y,
Horvitz HR
(1995) Defective recycling of synaptic vesicles in synaptotagmin mutants of Caenorhabditis elegans. Nature 378:196–199.
OpenUrl CrossRef PubMed

[98] Jorgensen EM,

[99] Hartwieg E,

[100] Schuske K,

[101] Nonet ML,

[102] Jin Y,

[103] Horvitz HR

[104] ↵
Kao HT,
Porton B,
Hilfiker S,
Stefani G,
Pieribone VA,
DeSalle R,
Greengard P
(1999) Molecular evolution of the synapsin gene family. J Exp Zool 285:360–377.
OpenUrl CrossRef PubMed

[105] Kao HT,

[106] Porton B,

[107] Hilfiker S,

[108] Stefani G,

[109] Pieribone VA,

[110] DeSalle R,

[111] Greengard P

[112] ↵
Li C,
Chalfie M
(1990) Organogenesis in C. elegans: positioning of neurons and muscles in the egg-laying system. Neuron 4:681–695.
OpenUrl CrossRef PubMed

[113] Li C,

[114] Chalfie M

[115] ↵
Li L,
Chin LS,
Shupliakov O,
Brodin L,
Sihra TS,
Hvalby O,
Jensen V,
Zheng D,
McNamara JO,
Greengard P,
Andersen P
(1995) Impairment of synaptic vesicle clustering and of synaptic transmission, and increased seizure propensity, in synapsin I-deficient mice. Proc Natl Acad Sci USA 92:9235–9239.
OpenUrl Abstract/FREE Full Text

[116] Li L,

[117] Chin LS,

[118] Shupliakov O,

[119] Brodin L,

[120] Sihra TS,

[121] Hvalby O,

[122] Jensen V,

[123] Zheng D,

[124] McNamara JO,

[125] Greengard P,

[126] Andersen P

[127] ↵
Lledo PM,
Zhang X,
Sudhof TC,
Malenka RC,
Nicoll RA
(1998) Postsynaptic membrane fusion and long-term potentiation. Science 279:399–403.
OpenUrl Abstract/FREE Full Text

[128] Lledo PM,

[129] Zhang X,

[130] Sudhof TC,

[131] Malenka RC,

[132] Nicoll RA

[133] ↵
Lloyd TE,
Verstreken P,
Ostrin EJ,
Phillippi A,
Lichtarge O,
Bellen HJ
(2000) A genome-wide search for synaptic vesicle cycle proteins in Drosophila. Neuron 26:45–50.
OpenUrl CrossRef PubMed

[134] Lloyd TE,

[135] Verstreken P,

[136] Ostrin EJ,

[137] Phillippi A,

[138] Lichtarge O,

[139] Bellen HJ

[140] ↵
Lou X,
Bixby JL
(1993) Coordinate and noncoordinate regulation of synaptic vesicle protein genes during embryonic development. Dev Biol 159:327–337.
OpenUrl CrossRef PubMed

[141] Lou X,

[142] Bixby JL

[143] ↵
McIntire SL,
Jorgensen E,
Kaplan J,
Horvitz HR
(1993) The GABAergic nervous system of Caenorhabditis elegans. Nature 364:337–341.
OpenUrl CrossRef PubMed

[144] McIntire SL,

[145] Jorgensen E,

[146] Kaplan J,

[147] Horvitz HR

[148] ↵
Mello C,
Fire A
(1995) DNA transformation. Methods Cell Biol 48:451–482.
OpenUrl CrossRef PubMed

[149] Mello C,

[150] Fire A

[151] ↵
Melloni RH Jr.,
Apostolides PJ,
Hamos JE,
DeGennaro LJ
(1994) Dynamics of synapsin I gene expression during the establishment and restoration of functional synapses in the rat hippocampus. Neuroscience 58:683–703.
OpenUrl CrossRef PubMed

[152] Melloni RH Jr.,

[153] Apostolides PJ,

[154] Hamos JE,

[155] DeGennaro LJ

[156] ↵
Merchan-Perez A,
Liberman MC
(1996) Ultrastructural differences among afferent synapses on cochlear hair cells: correlations with spontaneous discharge rate. J Comp Neurol 371:208–221.
OpenUrl CrossRef PubMed

[157] Merchan-Perez A,

[158] Liberman MC

[159] ↵
Miller DM,
Shen MM,
Shamu CE,
Burglin TR,
Ruvkun G,
Dubois ML,
Ghee M,
Wilson L
(1992) C. elegans unc-4 gene encodes a homeodomain protein that determines the pattern of synaptic input to specific motor neurons. Nature 355:841–845.
OpenUrl CrossRef PubMed

[160] Miller DM,

[161] Shen MM,

[162] Shamu CE,

[163] Burglin TR,

[164] Ruvkun G,

[165] Dubois ML,

[166] Ghee M,

[167] Wilson L

[168] ↵
Miller DM,
Desai N,
Hardin D,
Piston DW,
Patterson GH,
Fleenor J,
Xu SQ,
Fire A
(1999) A two-color GFP expression system for C. elegans. Biotechniques 26:914–921.
OpenUrl PubMed

[169] Miller DM,

[170] Desai N,

[171] Hardin D,

[172] Piston DW,

[173] Patterson GH,

[174] Fleenor J,

[175] Xu SQ,

[176] Fire A

[177] ↵
Miller DM III.,
Niemeyer CJ
(1995) Expression of the unc-4 homeoprotein in Caenorhabditis elegans motor neurons specifies presynaptic input. Development 121:2877–2866.
OpenUrl Abstract

[178] Miller DM III.,

[179] Niemeyer CJ

[180] ↵
Miller DM III.,
Niemeyer CJ,
Chitkara P
(1993) Dominant unc-37 mutations suppress the movement defect of a homeodomain mutation in unc-4, a neural specificity gene in Caenorhabditis elegans. Genetics 135:741–753.
OpenUrl Abstract/FREE Full Text

[181] Miller DM III.,

[182] Niemeyer CJ,

[183] Chitkara P

[184] ↵
Miller KG,
Alfonso A,
Nguyen M,
Crowell JA,
Johnson CD,
Rand JB
(1996) A genetic selection for Caenorhabditis elegans synaptic transmission mutants. Proc Natl Acad Sci USA 93:12593–12598.
OpenUrl Abstract/FREE Full Text

[185] Miller KG,

[186] Alfonso A,

[187] Nguyen M,

[188] Crowell JA,

[189] Johnson CD,

[190] Rand JB

[191] ↵
Nishimune A,
Isaac JT,
Molnar E,
Noel J,
Nash SR,
Tagaya M,
Collingridge GL,
Nakanishi S,
Henley JM
(1998) NSF binding to GluR2 regulates synaptic transmission. Neuron 21:87–97.
OpenUrl CrossRef PubMed

[192] Nishimune A,

[193] Isaac JT,

[194] Molnar E,

[195] Noel J,

[196] Nash SR,

[197] Tagaya M,

[198] Collingridge GL,

[199] Nakanishi S,

[200] Henley JM

[201] Nonet M
(1999) Studying mutants that affect neurotransmitter release in C. elegans. in Neurotransmitter release, ed Bellen HJ (Oxford UP, New York), pp 265–303.

[202] Nonet M

[203] ↵
Nonet ML
(1999) Visualization of synaptic specializations in live C. elegans with synaptic vesicle protein-GFP fusions. J Neurosci Methods 89:33–40.
OpenUrl CrossRef PubMed

[204] Nonet ML

[205] ↵
Nonet ML,
Grundahl K,
Meyer BJ,
Rand JB
(1993) Synaptic function is impaired but not eliminated in C. elegans mutants lacking synaptotagmin. Cell 73:1291–1305.
OpenUrl CrossRef PubMed

[206] Nonet ML,

[207] Grundahl K,

[208] Meyer BJ,

[209] Rand JB

[210] ↵
Nonet ML,
Staunton JE,
Kilgard MP,
Fergestad T,
Hartwieg E,
Horvitz HR,
Jorgensen EM,
Meyer BJ
(1997) Caenorhabditis elegans rab-3 mutant synapses exhibit impaired function and are partially depleted of vesicles. J Neurosci 17:8061–8073.
OpenUrl Abstract/FREE Full Text

[211] Nonet ML,

[212] Staunton JE,

[213] Kilgard MP,

[214] Fergestad T,

[215] Hartwieg E,

[216] Horvitz HR,

[217] Jorgensen EM,

[218] Meyer BJ

[219] ↵
Nonet ML,
Saifee O,
Zhao H,
Rand JB,
Wei L
(1998) Synaptic transmission deficits in Caenorhabditis elegans synaptobrevin mutants. J Neurosci 18:70–80.
OpenUrl Abstract/FREE Full Text

[220] Nonet ML,

[221] Saifee O,

[222] Zhao H,

[223] Rand JB,

[224] Wei L

[225] ↵
Nonet ML,
Holgado AM,
Brewer F,
Serpe CJ,
Norbeck BA,
Holleran J,
Wei L,
Hartwieg E,
Jorgensen EM,
Alfonso A
(1999) UNC-11, a Caenorhabditis elegans AP180 homologue, regulates the size and protein composition of synaptic vesicles. Mol Biol Cell 10:2343–2360.
OpenUrl Abstract/FREE Full Text

[226] Nonet ML,

[227] Holgado AM,

[228] Brewer F,

[229] Serpe CJ,

[230] Norbeck BA,

[231] Holleran J,

[232] Wei L,

[233] Hartwieg E,

[234] Jorgensen EM,

[235] Alfonso A

[236] ↵
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.
OpenUrl Abstract/FREE Full Text

[237] Ogawa H,

[238] Harada S,

[239] Sassa T,

[240] Yamamoto H,

[241] Hosono R

[242] ↵
Osten P,
Srivastava S,
Inman GJ,
Vilim FS,
Khatri L,
Lee LM,
States BA,
Einheber S,
Milner TA,
Hanson PI,
Ziff EB
(1998) The AMPA receptor GluR2 C terminus can mediate a reversible, ATP-dependent interaction with NSF and alpha- and beta-SNAPs. Neuron 21:99–110.
OpenUrl CrossRef PubMed

[243] Osten P,

[244] Srivastava S,

[245] Inman GJ,

[246] Vilim FS,

[247] Khatri L,

[248] Lee LM,

[249] States BA,

[250] Einheber S,

[251] Milner TA,

[252] Hanson PI,

[253] Ziff EB

[254] ↵
Petersohn D,
Schoch S,
Brinkmann DR,
Thiel G
(1995) The human synapsin II gene promoter. Possible role for the transcription factor zif268/egr-1, polyoma enhancer activator 3, and AP2. J Biol Chem 270:24361–24369.
OpenUrl Abstract/FREE Full Text

[255] Petersohn D,

[256] Schoch S,

[257] Brinkmann DR,

[258] Thiel G

[259] ↵
Pflugrad A,
Meir JY-J,
Barnes TM,
Miller DM III.
(1997) The Groucho-like transcription factor UNC-37 functions with the neural specificity gene unc-4 to govern motor neuron identity in C. elegans. Development 124:1699–1709.
OpenUrl Abstract

[260] Pflugrad A,

[261] Meir JY-J,

[262] Barnes TM,

[263] Miller DM III.

[264] ↵
Richmond JE,
Davis WS,
Jorgensen EM
(1999) UNC-13 is required for synaptic vesicle fusion in C. elegans. Nat Neurosci 2:959–964.
OpenUrl CrossRef PubMed

[265] Richmond JE,

[266] Davis WS,

[267] Jorgensen EM

[268] ↵
Rongo C,
Kaplan JM
(1999) CaMKII regulates the density of central glutamatergic synapses in vivo. Nature 402:195–199.
OpenUrl CrossRef PubMed

[269] Rongo C,

[270] Kaplan JM

[271] ↵
Rosahl TW,
Spillane D,
Missler M,
Herz J,
Selig DK,
Wolff JR,
Hammer RE,
Malenka RC,
Sudhof TC
(1995) Essential functions of synapsins I and II in synaptic vesicle regulation. Nature 375:488–493.
OpenUrl CrossRef PubMed

[272] Rosahl TW,

[273] Spillane D,

[274] Missler M,

[275] Herz J,

[276] Selig DK,

[277] Wolff JR,

[278] Hammer RE,

[279] Malenka RC,

[280] Sudhof TC

[281] ↵
Rothman JE
(1994) Mechanisms of intracellular protein transport. Nature 372:55–63.
OpenUrl CrossRef PubMed

[282] Rothman JE

[283] ↵
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.
OpenUrl Abstract/FREE Full Text

[284] Saifee O,

[285] Wei L,

[286] Nonet ML

[287] ↵
Schinkmann K,
Li C
(1992) Localization of FMRFamide-like peptides in Caenorhabditis elegans. J Comp Neurol 316:251–260.
OpenUrl CrossRef PubMed

[288] Schinkmann K,

[289] Li C

[290] ↵
Smith MD,
Dawson SJ,
Latchman DS
(1997) The Brn-3a transcription factor induces neuronal process outgrowth and the coordinate expression of genes encoding synaptic proteins. Mol Cell Biol 17:345–354.
OpenUrl Abstract/FREE Full Text

[291] Smith MD,

[292] Dawson SJ,

[293] Latchman DS

[294] ↵
Song I,
Kamboj S,
Xia J,
Dong H,
Liao D,
Huganir RL
(1998) Interaction of the N-ethylmaleimide-sensitive factor with AMPA receptors. Neuron 21:393–400.
OpenUrl CrossRef PubMed

[295] Song I,

[296] Kamboj S,

[297] Xia J,

[298] Dong H,

[299] Liao D,

[300] Huganir RL

[301] ↵
Sulston J,
Hodgkin J
(1988) Methods. in The nematode Caenorhabditis elegans, ed Wood WB (Cold Spring Harbor Laboratory, Cold Spring Harbor, NY), pp 587–606.

[302] Sulston J,

[303] Hodgkin J

[304] ↵
Sulston JE,
Horvitz HR
(1977) Post-embryonic cell lineages of the nematode, Caenorhabditis elegans. Dev Biol 56:110–156.
OpenUrl CrossRef PubMed

[305] Sulston JE,

[306] Horvitz HR

[307] ↵
Sulston JE,
Schierenberg E,
White JG,
Thomson JN
(1983) The embryonic cell lineage of the nematode Caenorhabditis elegans. Dev Biol 100:64–119.
OpenUrl CrossRef PubMed

[308] Sulston JE,

[309] Schierenberg E,

[310] White JG,

[311] Thomson JN

[312] ↵
Takei Y,
Harada A,
Takeda S,
Kobayashi K,
Terada S,
Noda T,
Takahashi T,
Hirokawa N
(1995) Synapsin I deficiency results in the structural change in the presynaptic terminals in the murine nervous system. J Cell Biol 131:1789–1800.
OpenUrl Abstract/FREE Full Text

[313] Takei Y,

[314] Harada A,

[315] Takeda S,

[316] Kobayashi K,

[317] Terada S,

[318] Noda T,

[319] Takahashi T,

[320] Hirokawa N

[321] ↵
Trent C,
Tsung N,
Horvitz H
(1983) Egg-laying defective mutants of the nematode Caenorhabditis elegans. Genetics 104:619–647.
OpenUrl Abstract/FREE Full Text

[322] Trent C,

[323] Tsung N,

[324] Horvitz H

[325] ↵
Waggoner LE,
Zhou GT,
Schafer RW,
Schafer WR
(1998) Control of alternative behavioral states by serotonin in Caenorhabditis elegans. Neuron 21:203–214.
OpenUrl CrossRef PubMed

[326] Waggoner LE,

[327] Zhou GT,

[328] Schafer RW,

[329] Schafer WR

[330] ↵
White JG,
Southgate E,
Thomson JN,
Brenner S
(1976) Structure of the ventral nerve cord of Caenorhabditis elegans. Philos Trans R Soc Lond [Biol] 275:327–348.
OpenUrl CrossRef PubMed

[331] White JG,

[332] Southgate E,

[333] Thomson JN,

[334] Brenner S

[335] ↵
White JG,
Southgate E,
Thomson JN,
Brenner S
(1986) The structure of the nervous system of the nematode Caenorhabditis elegans. Philos Trans R Soc Lond [Biol] 314:1–340.
OpenUrl CrossRef

[336] White JG,

[337] Southgate E,

[338] Thomson JN,

[339] Brenner S

[340] ↵
White JG,
Southgate E,
Thomson JN
(1992) Mutations in the Caenorhabditis elegans unc-4 gene alter the synaptic input to ventral cord motor neurons. Nature 355:838–841.
OpenUrl CrossRef PubMed

[341] White JG,

[342] Southgate E,

[343] Thomson JN

[344] ↵
Winnier AR,
Meir JY,
Ross JM,
Tavernarakis N,
Driscoll M,
Ishihara T,
Katsura I,
Miller DM III.
(1999) UNC-4/UNC-37-dependent repression of motor neuron-specific genes controls synaptic choice in Caenorhabditis elegans. Genes Dev 13:2774–2786.
OpenUrl Abstract/FREE Full Text

[345] Winnier AR,

[346] Meir JY,

[347] Ross JM,

[348] Tavernarakis N,

[349] Driscoll M,

[350] Ishihara T,

[351] Katsura I,

[352] Miller DM III.

[353] ↵
Zhao H,
Nonet ML
(2000) A retrograde signal is involved in activity-dependent remodeling at a C. elegans neuromuscular junction. Development 127:1253–1266.
OpenUrl Abstract

[354] Zhao H,

[355] Nonet ML

[356] ↵
Zheng Y,
Brockie PJ,
Mellem JE,
Madsen DM,
Maricq AV
(1999) Neuronal control of locomotion in C. elegans is modified by a dominant mutation in the GLR-1 ionotropic glutamate receptor. Neuron 24:347–361.
OpenUrl CrossRef PubMed

[357] Zheng Y,

[358] Brockie PJ,

[359] Mellem JE,

[360] Madsen DM,

[361] Maricq AV

Main menu

User menu

Search

Regulation of Neurotransmitter Vesicles by the Homeodomain Protein UNC-4 and Its Transcriptional Corepressor UNC-37/Groucho inCaenorhabditis elegans Cholinergic Motor Neurons

Abstract

MATERIALS AND METHODS

RESULTS

UNC-4 is expressed in cholinergic motor neurons

UNC-4 is required for expression of UNC-17 and ChAT inunc-4-motor neurons

UNC-37 functions with UNC-4 to maintain cholinergic proteins

UNC-4 and UNC-37 regulate the levels of other vesicular proteins

Nonvesicular proteins are not affected in unc-4 andunc-37 mutants

Neurotransmitter vesicles are decreased inunc-4 mutants

Reduced vesicular protein staining is correlated with functional defects in unc-4 neurons

UNC-4- and UNC-37-dependent transcriptional repressor function is required to maintain normal levels of vesicular proteins

Vesicular proteins are regulated at a post-transcriptional level

Vesicular protein levels are developmentally regulated by unc-4

DISCUSSION

unc-4 and unc-37 regulate vesicle biogenesis or stability

Neuronal function depends on post-transcriptional regulation of SV protein expression

Motor neuron dysfunction contributes to the Unc-4 movement defect

Does the vesicular signaling capacity of VA motor neurons specify presynaptic inputs or vice versa?

Footnotes

REFERENCES

In this issue

Citation Manager Formats

Keywords

Responses to this article

Jump to comment:

Related Articles

Cited By...

More in this TOC Section

ARTICLE

Development/Plasticity/Repair

Main menu

User menu

Search

Regulation of Neurotransmitter Vesicles by the Homeodomain Protein UNC-4 and Its Transcriptional Corepressor UNC-37/Groucho inCaenorhabditis elegans Cholinergic Motor Neurons

Abstract

MATERIALS AND METHODS

RESULTS

UNC-4 is expressed in cholinergic motor neurons

UNC-4 is required for expression of UNC-17 and ChAT inunc-4-motor neurons

UNC-37 functions with UNC-4 to maintain cholinergic proteins

UNC-4 and UNC-37 regulate the levels of other vesicular proteins

Nonvesicular proteins are not affected in unc-4 andunc-37 mutants

Neurotransmitter vesicles are decreased inunc-4 mutants

Reduced vesicular protein staining is correlated with functional defects in unc-4 neurons

UNC-4- and UNC-37-dependent transcriptional repressor function is required to maintain normal levels of vesicular proteins

Vesicular proteins are regulated at a post-transcriptional level

Vesicular protein levels are developmentally regulated by unc-4

DISCUSSION

unc-4 and unc-37 regulate vesicle biogenesis or stability

Neuronal function depends on post-transcriptional regulation of SV protein expression

Motor neuron dysfunction contributes to the Unc-4 movement defect

Does the vesicular signaling capacity of VA motor neurons specify presynaptic inputs or vice versa?

Footnotes

REFERENCES

In this issue

Citation Manager Formats

Jump to section

Keywords

Responses to this article

Jump to comment:

Related Articles

Cited By...

More in this TOC Section

ARTICLE

Development/Plasticity/Repair