SLEEPLESS, a Ly-6/neurotoxin family member, regulates the levels, localization and activity of Shaker.

Sleep is a whole-organism phenomenon accompanied by global changes in neural activity. We previously identified SLEEPLESS (SSS) as a glycosylphosphatidyl inositol-anchored protein required for sleep in Drosophila. Here we found that SSS is critical for regulating the sleep-modulating potassium channel Shaker. SSS and Shaker shared similar expression patterns in the brain and specifically affected each other's expression levels. sleepless (sss) loss-of-function mutants exhibited altered Shaker localization, reduced Shaker current density and slower Shaker current kinetics. Transgenic expression of sss in sss mutants rescued defects in Shaker expression and activity cell-autonomously and suggested that SSS functions in wake-promoting, cholinergic neurons. In heterologous cells, SSS accelerated the kinetics of Shaker currents and was co-immunoprecipitated with Shaker, suggesting that SSS modulates Shaker activity via a direct interaction. SSS is predicted to belong to the Ly-6/neurotoxin superfamily, suggesting a mechanism for regulation of neuronal excitability by endogenous toxin-like molecules.

In mammals, sleep is associated with broad changes in patterns of neuronal activity in the brain. Sleep in fruit flies shares several features of mammalian sleep, such as circadian and homeostatic regulation and increased arousal threshold1,2, and is similarly accompanied by broad changes in brain activity3. Modulation of neuronal excitability may be an essential component of sleep regulation. This view is supported by several studies demonstrating that mice and flies bearing mutations in genes encoding ion channels and their associated proteins exhibit altered sleep4–8. For instance, a forward genetic screen led to the identification of a mutation in the gene encoding the canonical voltage–gated potassium channel Shaker as the defect underlying a short–sleeping phenotype in Drosophila, and targeted disruption of the mammalian Shaker ortholog, Kv1.2, also leads to reduced sleep in mice9,10.

We recently identified a novel gene required for sleep in Drosophila, which we named sleepless (sss). sss mutants exhibit a severe reduction in sleep and a decreased level of Shaker expression, providing an additional link between sleep and neuronal excitability11. However, the mechanism by which SSS regulates Shaker, and thereby neuronal excitability, is not known. The mature SSS protein, ~15 kD in size, is cysteine–rich and covalently linked to the plasma membrane by a glycosylphosphatidyl–inositol (GPI) anchor11. We now show that SSS belongs to the Ly–6/neurotoxin superfamily of proteins12. This superfamily includes diverse proteins such as secreted signaling molecules and receptors13–15, as well as snake neurotoxins, which bind to and modulate the activity of various ion channels12,16.

The predicted Ly–6/neurotoxin domain in SSS suggests at least two distinct potential molecular mechanisms of action. One possibility is that SSS acts as a “proto–toxin,” forming a complex with Shaker to control its expression and activity within the same cell. An endogenous toxin–like molecule that regulates Shaker–type channels has been postulated, based on the finding that expression of a Shaker–specific neurotoxin in the endoplasmic reticulum (ER) of mammalian cells increases the surface localization of these channels17. Alternatively, since SSS is tethered to the cell surface by a GPI anchor and cleavage of the anchor by phospholipase C results in release of SSS into the media in cultured cells11, SSS may be a secreted molecule that acts on Shaker indirectly through a receptor–mediated signaling pathway.

Here we present evidence demonstrating a role for SSS as an endogenous toxin–like regulator of Shaker expression, localization, and activity. SSS and Shaker share a similar expression pattern in the Drosophila brain, and loss of either SSS or Shaker results in a reduction of the other protein, suggesting that these proteins are required for each other’s stability. We show that the ability of SSS to promote sleep localizes to wake–promoting, cholinergic neurons that are distinct from circuitry involved in sss–dependent, ether–induced leg–shaking. In sss mutants, Shaker appears to be mislocalized, and Shaker currents are smaller and slower. Shaker protein levels as well as current amplitude and kinetics are all rescued in sss mutants in a cell–autonomous manner by targeted expression of a sss transgene. Finally, in heterologous systems, SSS accelerates kinetics of Shaker currents and can be co–immunoprecipitated with Shaker, suggesting that SSS forms a complex with Shaker and regulates its activity. Together, these results establish SSS as a critical regulator of Shaker channels, defining a novel molecular mechanism for the modulation of neuronal excitability.

RESULTS

Differential rescue of sss mutant phenotypes

We previously demonstrated that SSS is markedly enriched in adult brains and that the sss mutant sleep phenotype can be rescued using a transgene containing the sss genomic region11. To examine the neuronal circuitry required for the sleep phenotype observed in sss mutants, we used the Gal4–UAS system to perform targeted rescue of the sss mutation18. We generated transgenic flies bearing Gal4 under control of the sss promoter (sss–Gal4, see Methods) and found that daily sleep amount is restored to wild–type levels in sss mutant flies carrying both the sss–Gal4 driver and the UAS–sss transgene (Fig. 1a). By crossing flies bearing the sss–Gal4 driver to those carrying a UAS–GFP transgene, we found that the sss–Gal4 driver expresses broadly, with prominent enrichment in areas such as the mushroom bodies, a region previously shown to be important for sleep regulation,19,20 and antennal nerves, in a pattern that overlaps substantially with the SSS immunostaining pattern (compare Supplementary Fig. 1 and Fig. 2, below). Pan–neuronal expression of UAS–sss under the control of the elav–Gal4 driver also fully rescued the sss mutant sleep phenotype (Fig. 1a).

Figure 1

Rescue of the sleep phenotype of sss mutants with a UAS–sss transgene (a) Daily sleep amounts for female sss mutant flies with a UAS–sss transgene and either an elav–Gal4 or sss–Gal4 driver (white bar) were markedly increased relative to sss mutants with either the transgene or the driver alone (black bar). Heterozygous (het) sss flies served as a wild–type control (gray bar). Successful rescue of ether–induced leg shaking is indicated by “+” at the bottom. In this and subsequent figures, error bars indicate SEM. n ≥ 30 for each genotype. **P < 0.0001.

(b) Rescue of the sleep phenotype by expression of sss in cholinergic neurons. For each Gal4 driver, daily sleep amounts are presented for female sss mutant flies carrying either the driver alone (black bar) or for those carrying both the driver and a UAS–sss transgene (white bar). Rescue of ether–induced leg shaking is shown for each driver as successful (“+”) or unsuccessful (“−”). n ≥ 30 for each genotype, except for TH–Gal4 driver control, for which n = 12. *P < 0.01; **P < 0.0001.

Figure 2

Distribution of SSS and Shaker immunoreactivity in the adult fly brain Whole–mount brain samples of iso31 (wild–type– a–d) flies were stained with an antibody to SSS (a, c) or to Shaker (b, d). Appropriate mutant lines (sss for anti–SSS, e, and Shaker for anti–Shaker, f) are also shown. Maximal intensity projections of 1–μm confocal sections of the anterior third (ant–a, b) or posterior third (post–c, d) of the brain are shown for wild–type brains. For mutant brains, maximal projections of the entire brain are shown. The bracket and arrows point to the mushroom bodies (MB), anterior optic tubercle (AOT), superior protocerebrum (SP), and the antennal nerve (AN). SSS and Shaker expression in the posterior third of the brain included fibers from a group of visual projection neurons (VPN fiber) sending processes to the lobula plate (Lo P) of the optic lobe. Representative brains are shown, taken from at least three independent experiments. For iso31 brains, n=21 for anti–SSS and n=12 for anti–Shaker. For sss brains, n=16 and for Shaker brains, n=10. Scale bar, 50 μm.

Because both sss–Gal4 and elav–Gal4 drivers exhibited broad expression patterns, we also examined whether more restricted sss expression could rescue the mutant sleep phenotype. We screened a number of Gal4 driver lines with varying expression patterns for their ability to rescue reduced sleep in sss mutants. While several drivers promoted strong rescue, they all have broad expression patterns (Supplementary Figs. 2 and 3), making it difficult to pinpoint a specific region required for SSS function. Drivers that promoted more restricted expression patterns were associated with little or no rescue; these included drivers that direct expression in the mushroom bodies, clock cells, and the pars intercerebralis neurons, areas that have been implicated in sleep regulation19–25. We also examined the effects of overexpressing SSS on sleep amount in wild–type animals. As shown in Supplementary Fig. 4, SSS overexpression using a variety of Gal4 drivers had no significant effect on daily sleep amount.

To examine whether a specific neurotransmitter system underlies the short–sleeping phenotype of sss mutants, we employed Gal4 drivers that express in different neurotransmitter systems (Fig. 1b). Expression of sss preferentially in cholinergic neurons using Cha–Gal4 resulted in strong rescue of the short–sleeping phenotype of sss mutants. In contrast, preferential expression of sss in glutamatergic or dopaminergic neurons driven by vGlut– or TH–Gal4 respectively resulted in weak or no rescue of the mutant sleep phenotype. Together, these data suggest that SSS expression in cholinergic, but not glutamatergic or dopaminergic neurons, is important for sleep regulation. However, we cannot exclude the possibility that some non–cholinergic neurons also contribute to the strong rescue by Cha–Gal4. Like other drivers that rescue well, the Cha–Gal4 expression pattern is also anatomically broad, and thus the regulation of sleep by SSS may involve widely distributed neurons of the Drosophila brain.

Like Shaker mutants, sss mutants display rhythmic leg–shaking under ether anesthesia11,26. This leg–shaking phenotype was rescued by SSS expression using the elav–Gal4 and sss–Gal4 drivers (Fig. 1a). Interestingly, we found that while the cholinergic driver, Cha–Gal4, efficiently rescued the sleep phenotype of sss mutants, it had little effect on leg shaking. In contrast, expression of SSS in glutamatergic neurons with vGlut–Gal4 rescued the leg–shaking phenotype of sss mutants, but displayed only weak rescue of the sleep phenotype (Fig. 1b). These data demonstrate that the circuits mediating ether–induced leg shaking and sleep regulation are distinct, suggesting that the sleep dysfunction in sss mutants is not caused by a defect in motor neurons.

SSS and Shaker are enriched in the same brain regions

To investigate a possible cell–autonomous role for SSS in regulating Shaker, we sought to determine whether the two proteins could be colocalized in the adult Drosophila brain. To visualize SSS–expressing cells, we generated a new anti–SSS antibody and performed whole–mount immunostaining of adult brains. There was appreciable overlap between the SSS immunostaining and the expression of GFP driven by sss–Gal4 (compare Fig. 2 and Supplementary Fig. 1). SSS–specific immunoreactivity was observed in the mushroom bodies and other structures such as the antennal nerves, superior protocerebrum, and the lobula plate of the optic lobes (Figs. 2a,c). Loss of SSS immunoreactivity in sss null mutants demonstrates specificity of our antibody (Fig. 2e).

To examine the Shaker expression pattern, we also raised a new Shaker antibody. We found that Shaker and SSS show similar expression patterns, with broad expression throughout the brain, but with clear enrichment in specific structures, including the mushroom bodies, the superior protocerebrum, antennal nerves, and neuronal processes in the lobula plate (Figs. 2b,d). This staining pattern was specific, as it was absent in Shaker deficiency (Shaker; B55/W32)27 brains (Fig. 2f), and is similar to that found in a previous Shaker immunohistochemical study28. The requirement of different fixatives for the anti–SSS and anti–Shaker antibodies prevented a direct assessment of colocalization. However, the finding that SSS and Shaker are enriched in similar regions of the brain suggests that SSS regulates Shaker in a cell–autonomous manner.

Shaker and SSS specifically affect each other’s expression

We next used our Shaker antibody to examine the relationship between Shaker and SSS in greater detail. The antibody recognized two bands of apparent molecular weight of ~65–75 kD on Western blots of wild–type fly head extracts, but not in Shaker extracts, demonstrating that the antibody selectively reacts with Shaker protein (Fig. 3a). Since alternative splicing produces multiple isoforms of Shaker, the two bands may represent different isoforms. Both Shaker bands were reduced in sss mutants, confirming our previous finding that sss affects Sh protein expression11. In contrast, Shaker mRNA levels were not reduced in sss mutants (Supplementary Fig. 5), indicating that the reduction of Shaker protein in sss mutants is caused by post–transcriptional regulation of Shaker.

Figure 3

Shaker and SSS specifically affect each other’s expression (a) Shaker was reduced in sss mutants, and SSS was reduced in Shaker (Sh) mutants. Shaker and SSS levels were not reduced in other short–sleeping mutants, DAT and Cl. Head extracts of background control and mutant flies of indicated genotypes were analyzed by Western blotting using antibodies to Shaker and SSS. Shaker and sss mutant flies were used as negative controls, and antibody to Actin was used to control for loading. Representative blots from 4 independent experiments are shown in a and b.

(b) Eag expression was not affected in sss mutants. Head extracts of eag and sss mutants, as well as background control, were analyzed by Western blotting using antibodies to Eag and Actin (for loading control).

Other short–sleeping mutants, such as DAT and Clk 29–31, did not exhibit noticeable reductions in Shaker protein levels (Fig. 3a), demonstrating that reduced sleep is not necessarily linked to a reduction in Shaker expression. In addition, sss does not affect expression of all potassium channels, as expression of Eag protein was comparable in sss mutants and wild–type flies (Fig. 3b).

To determine whether there is a reciprocal effect of Shaker on SSS expression, we examined SSS levels in Shaker mutants and found that SSS expression is reduced compared to controls, indicating that Shaker and SSS mutually affect each other’s expression. SSS levels were not reduced in DAT and Clk mutants (Fig. 3a and Supplementary Fig. 6), providing further evidence for a specific interaction between SSS and Shaker. The mutual effects of SSS and Shaker on each other’s expression are consistent with the hypothesis that SSS and Shaker exist in a complex.

Shaker localization is altered in sss mutants

Because neuronal output can be regulated not only by the number of ion channels, but also by their regional and subcellular localization, we examined Shaker staining in whole–mount brains. Consistent with the Western blot results in Figure 3, we found that overall Shaker expression was lower in sss mutants compared to control flies (Fig. 4b vs. 4a). However, the degree to which Shaker was reduced in sss mutants was not uniform across brain regions. For instance, Shaker immunoreactivity in sss mutants was greatly reduced in antennal nerves, lobula plate, and certain subregions (e.g., α and α’ lobes) of the mushroom bodies, but it was not as severely affected in other subregions (e.g., γ lobes) of the mushroom bodies (Fig. 4b vs. 4a).

Figure 4

Altered Shaker expression and localization in sss mutants Shaker immunostaining of control iso31 (a, c) and sss (b, d) whole–mount adult brains is shown. Maximal intensity projections from 1–μm sections from the entire brain are shown for (a) and (b), while a single 1–μm section from the posterior aspect of the brain including the protocerebral bridge is shown for (c) and (d). A 2x magnified inset is shown for (d). Shaker immunostaining in whole–mount adult thoracic ganglia of iso31 (e,g) and sss (f, h). (g) and (h) are 2x magnified images from the boxed areas in (e) and (f), respectively. Structures are labeled as follows: alpha and alpha’ (α/α’) and gamma (γ) lobes of the mushroom bodies, antennal nerve (an), processes of a group of visual projection neurons (vpn), and the central connective (cc). Representative images are shown, from at least three independent experiments. n=10 and n=11 for iso31 and sss brains, respectively. n=9 for iso31 and sss thoracic ganglia. Scale bar in (a) for (a–d), (e) for (e,f), and (g) for (g,h), 50 μm

Furthermore, the subcellular localization of Shaker appeared to be altered in sss mutants. In wild–type animals, Shaker was expressed widely in neuronal fiber tracts. For example, we observed strong Shaker expression in the antennal nerves (Fig. 4a), processes originating from visual projection neurons (Fig. 4c), and the cervical connective (Figs. 4e and 4g). In contrast, in sss mutants, we found Shaker predominantly in cell bodies in both brains (Fig. 4d) and thoracic ganglia (Figs. 4f and 4h). Although we cannot rule out the possibility that SSS is more important for Shaker expression in cells where Shaker is predominantly in neuronal processes than in cells where the channel is enriched in cell bodies, our data suggest that SSS is required for proper subcellular localization of Shaker, i.e. targeting to or retention at neuronal processes.

Targeted expression of sss restores Shaker expression

To address whether SSS regulates Shaker in a cell–autonomous manner, we first examined whether restoration of SSS in specific brain regions of sss mutants selectively rescues Shaker expression in the same regions. We coupled the expression of a sss transgene to the OK107– and vGlut–Gal4 drivers, which have complementary expression patterns in two brain regions where Shaker is normally enriched. Whereas OK107–Gal4 directed GFP expression to the mushroom bodies but not to a group of visual projection neurons sending processes to the optic lobe, the opposite was true for the vGlut–Gal4 driver (Figs. 5a,c,e,g).

Figure 5

Rescue of Shaker expression in sss mutants by transgenic expression of sss (a–d) OK107–Gal4 was used to direct expression of GFP (a, c) or sss (b, d), and GFP or Shaker expression was examined, respectively. Since Shaker was enriched in synapse–rich neuropil, GFP fused to synaptogamin (syt–GFP), which is targeted to the synapse, was used. GFP expression was seen in the mushroom bodies (a), but not in the group of visual projection neurons (VPNs) sending processes to the optic lobe (c). Transgenic expression of sss using OK107–Gal4 increased Shaker expression in the mushroom bodies (b), but not in the optic lobe (d).

(e–h) vGlut–Gal4 directed GFP expression in the visual projection neurons and the optic lobe (g), but not the mushroom bodies (e). Transgenic expression of sss using vGlut–Gal4 increased Shaker expression in the optic lobe (h), but not in the mushroom bodies (f). Arrows point to the fiber bundles formed by the VPNs. Maximal intensity projections of seven 1–μm sections from the anterior of the brain are shown for (a), (b), (e), and (f), and a single 1–μm section from the posterior of the brain at the level of the protocerebral bridge is shown for (c), (d), (g), and (h). Representative brains are shown, taken from two independent experiments. n=5 or 6 for all genotypes. Scale bar in (a) for (a,b,e,f) and (c) for (c,d,g,h), 50 μm

Using these drivers to express UAS–sss, we found that Shaker expression in sss mutants was restored in the regions where GFP, and presumably transgenic SSS, was expressed. Thus, restoration of SSS in sss mutants by OK107–Gal4 increased Shaker expression in the mushroom bodies, especially the α and α’ lobes (Fig. 5b), but not in the visual projection neurons (Fig. 5d). In contrast, vGlut–Gal4 rescue of sss enhanced Shaker expression in the visual projection neurons (Fig. 5h) but not in the mushroom bodies (Fig. 5f). While it is possible that SSS exerts local non–cell–autonomous effects on Shaker levels, these data are consistent with a cell–autonomous role for SSS regulation of Shaker expression.

Rescue of SSS function at the neuromuscular junction

We next addressed whether SSS cell–autonomously regulates Shaker function in vivo by examining the synaptic signaling properties at the larval neuromuscular junction (NMJ), as a prior study of the hypomorphic sss allele reported that functional properties at the NMJ are altered32. Pre– and post–synaptic phenotypes at the NMJ were assayed by measuring spontaneous miniature excitatory junctional potential (mEJP) frequency and the amplitude and kinetics of specific ionic currents, respectively.

The mEJP frequency was significantly increased in sss mutant larvae compared to their wild–type control line (Fig. 6a). A similar increase in the mEJP frequency was observed in Shaker mutant larvae (Fig. 6a), showing that disruption of either sss or Shaker leads to similar NMJ phenotypes. The increased mEJP frequency observed in sss larvae was abolished by expression of SSS presynaptically using the pan–neuronal elav–Gal4 driver. In contrast, consistent with presynaptic release frequency being regulated by glutamatergic motor neurons, expression of SSS in muscle with the 24B– Gal4 driver or in cholinergic neurons with the Cha–Gal4 driver failed to reduce the high mEJP frequency in sss mutants (Fig. 6a).

Figure 6

Cell–autonomous rescue of the sss phenotypes at the Drosophila larval NMJ (a) mEJP frequencies for sss (black bars) and Shaker (gray bar) larvae were significantly increased relative to background controls (white bar). The UAS–sss transgene (gray bars) significantly decreased mEJP frequencies in the sss mutant background only when combined with the elav–GAL4 driver.

(b) Time–to–peak IA current (t) was significantly greater in sss (black bars) than in background controls (white bar). The UAS–sss transgene (gray bars) significantly decreased IA t in the sss mutant background only when paired with the 24B–Gal4 driver.

(c) Representative traces of IA current illustrating the decrease in current magnitude and delayed time–to–peak in sss mutant larvae. Dashed line is from wild–type; solid line is from mutant muscle.

(d) IA density in larval muscle could be partially rescued over a range of voltages in sss mutants bearing a UAS–sss transgene under control of the muscle–specific driver 24B–Gal4, compared to background and driver controls. Rescue was not observed using the pan–neuronal driver elav–Gal4 coupled to UAS–sss. Values for n are the same as in (b). *P < 0.05; **P < 0.01.

The magnitude and kinetics of the Shaker–dependent IA current in larval muscles was also altered in sss mutants (Figs. 6b–d). The sss mutation significantly delayed the time–to–peak (t) of IA at 10 mV (Fig. 6b) and also decreased the IA current magnitude at every voltage ≥ −20 mV (Figs. 6c,d). In contrast, magnitude and kinetics of non–inactivating, Shaker–independent IK current were not altered in sss mutants (Supplementary Fig. 7). The increase in t and the reduction in IA amplitude in sss mutants can be rescued by transgenic expression of SSS in muscle with 24B–Gal4, but not in neurons with elav–Gal4 (Figs. 6b,d). It should be noted that only a partial rescue of IA amplitude is obtained with 24B–Gal4. Interestingly, a reduction in IA current was observed when SSS is overexpressed in muscles of wild–type animals using 24B–Gal4 (Supplementary Fig. 8), suggesting that the presence of excess SSS can impair Shaker function in muscle. Together, the electrophysiological results demonstrate that SSS regulates Shaker function in a cell–autonomous manner in both neurons and muscles.

SSS enhances Shaker channel function

We have shown that SSS is required for normal levels, localization, and activity of Shaker in vivo. Bioinformatic prediction of SSS tertiary structure using PHYRE (Protein Homology/analogY Recognition Engine)33 revealed a single disulfide–bonded domain containing three beta sheet–rich loops (or “fingers”) found in the Ly–6/neurotoxin superfamily of proteins (Supplementary Fig. 9a)12. Furthermore, the sss gene contains two conserved intron breaks in the coding region shared by Ly–6/neurotoxin gene family members34 (Supplementary Fig. 9b). The SSS protein also exhibits other features of the Ly–6 domain, such as an N–terminal leucine/isoleucine and a C–terminal asparagine, as well as pairs of cysteine residues with characteristic spacing. Together, these observations suggest SSS is a member of the Ly–6/neurotoxin superfamily. Since many neurotoxins are known to act on ion channels, including Shaker–type K+ channels16,35,36, the structural similarity of SSS to neurotoxins suggests that SSS might be an endogenous “proto–toxin” that binds to Shaker and regulates its activity.

To determine whether SSS affects Shaker channel activity, we co–expressed sss and Shaker in heterologous cells and examined the effects on Shaker current amplitude and kinetics. We first recorded Shaker currents in human embryonic kidney (HEK–tsA) cells expressing wild–type Shaker in the presence or absence of sss (Fig. 7). Co–expression with sss resulted in faster kinetics of Shaker current, significantly reducing t (Figs. 7a,c). A similar effect on the kinetics of Shaker current was observed with co–expression of SSS and wild–type Shaker channels in Xenopus oocytes (Figs. 7b,c), whereas amplitude of Shaker current was largely unaffected (Supplementary Fig. 10). Although the conditions used to coexpress Shaker and sss may not have been optimal to observe an effect on current amplitude, another potential explanation is that an additional component required for regulation of Shaker expression by SSS, which is present in brain and muscle, is missing in oocytes. Taken together with the slower kinetics of IA current in sss mutants (Figs. 6b,c), these findings suggest that SSS enhances Shaker activity in vivo.

Figure 7

SSS modulates Shaker function.

(a) Representative normalized currents measured at 15 mV from a holding potential of −100 mV in excised patches of HEK–tsA cells transfected with cDNA encoding the ShakerB (ShB) isoform in the absence or presence of sss.

(b) Representative normalized currents measured by two–electrode voltage clamp at 20 mV from a holding potential of −70 mV in oocytes expressing the ShakerD (ShD) isoform in the absence or presence of sss.

(c) Time to reach peak current (t) following a step change to 15 mV from a holding potential of −100 mV in HEK-tsA cells or following a step change to 20 mV from a holding potential of −70 mV in oocytes. n=5 for ShakerB alone, n=6 for ShakerB + sss, n=14 for ShakerD alone, n=14 for ShakerD + sss; **P < 0.01.

(d) Extracts from oocytes injected with cRNA derived from ShakerD, sss, or both were immunoprecipitated (IP) with an antibody to Shaker and analyzed by Western blotting (WB) using an antibody to SSS. Prior to immunoprecipitation, 5% of cell extracts (Input) were analyzed separately using antibodies to SSS and Shaker. A non–specific band (*) served as a loading control.

In order to assess whether SSS and Shaker can physically interact in a complex, we performed co–immunoprecipitation experiments in Xenopus oocytes. When both sss and Shaker were expressed in oocytes, SSS could be co–immunoprecipitated with Shaker (Fig. 7d). This interaction was specific, because SSS was not detected when immunoprecipitations were performed in the absence of Shaker. In summary, these data show that SSS can form a complex with and enhance the kinetic properties of Shaker.

DISCUSSION

We have presented in vivo and in vitro evidence that SSS is a novel modulator of Shaker expression, subcellular localization, and activity, and thus is an important regulator of nervous system function. While SSS probably modulates neuronal excitability at multiple anatomical loci, dissociation of the neural circuits responsible for sleep and ether–dependent leg–shaking suggests that the role of SSS in sleep regulation is distinct from its effect on motor control. Our data suggest that SSS acts on Shaker in a cell–autonomous manner and that expression of SSS in cholinergic neurons restores sleep in sss mutants, although unidentified non–cholinergic neurons included in the Cha–Gal4 expression pattern may also be required. Since upregulation of Shaker by SSS in cholinergic neurons presumably decreases excitability and results in increased sleep, excitation of these cholinergic neurons is likely to promote wakefulness in Drosophila. Recent studies have demonstrated involvement of monoaminergic signaling and GABA–responsive peptidergic cells in regulating wakefulness in Drosophila21,23–25,30,37–39. Thus, as in mammals40, sleep in Drosophila is controlled by arousal systems that include distinct populations of cholinergic, monoaminergic, and peptidergic neurons.

We found that SSS and Shaker were enriched in the same regions of the Drosophila brain and that SSS appeared to affect the subcellular distribution of Shaker. Thus, in sss mutants the distribution of Shaker channels shifts from an enrichment in processes to a predominance in cell bodies in brains and thoracic ganglia. In addition, loss of SSS or Shaker resulted in a reduction of the other protein, without a concomitant reduction in transcript, suggesting that these proteins stabilize each other in a complex. The reduction in brain Shaker expression in sss mutants could be rescued by transgenic expression of SSS. However, we only observed partial rescue of muscle IA amplitude in sss mutants with overexpression of SSS in muscles. Along these lines, we also found that overexpression of SSS in wild–type muscles reduced IA amplitude, suggesting that the presence of either too little or too much SSS can impair Shaker function, at least at the larval NMJ.

In addition to modulating the level of Shaker, SSS regulates kinetics of Shaker–dependent potassium currents. Kinetics of Shaker–mediated IA potassium currents in muscle were selectively slower in sss mutants, a phenotype that could be rescued by targeted expression of sss in muscle. In heterologous cells, co–expression of Shaker and SSS accelerated Shaker currents and resulted in detectable complex formation between the two proteins. Taken together, these data suggest that SSS directly interacts with Shaker to regulate its levels, localization, and activity.

Properties of voltage–gated potassium channels, such as expression level, subcellular localization, and gating characteristics are influenced by a number of associated regulatory proteins including Kvß/Hyperkinetic, KCNEs, KChIPs, and KChAP41–43. The in vivo relevance of these regulatory proteins is underscored by the finding that mutations in some of the genes encoding them are associated with human diseases, including Long QT syndromes41,43. Unlike most other known regulators of voltage–gated potassium channels, which generally interact with cytoplasmic domains of channel proteins, SSS, as a GPI–anchored protein tethered to the plasma membrane, probably interacts with an extracellular domain of the Shaker channel. The predicted structure of SSS is also unlike those of other known endogenous regulators of voltage–gated potassium channels. Bioinformatic analysis predicts that SSS contains a compact disulfide–bonded beta–sheet structure (three–finger fold) found in the Ly–6/neurotoxin superfamily of proteins. This diverse family includes proteins involved in the modulation of receptor function and immune complex formation, as well as snake neurotoxins that bind the extracellular domains of various ion channels at the cell surface12,13,15,44.

Snake neurotoxins do not have GPI anchors like SSS. However, ER–targeted expression of soluble dendrotoxin, a specific blocker of Shaker–type potassium channels, results in increased surface expression of Kv1.117, a mammalian ortholog of Shaker. This finding led Vacher et al. (2007) to postulate the existence of an endogenous toxin–like ER protein that tethers Shaker channels to the ER membrane and with which dendrotoxin competes for binding. SSS may be such an endogenous neurotoxin–like molecule regulating Shaker function and localization. However, rather than retaining Shaker in the ER, SSS appears to increase surface localization of the channel, either through promotion of Shaker trafficking to or retention at the cell surface.

Lynx1, another GPI–anchored neurotoxin/Ly–6 family member found in mammals, binds to and modulates the activity of a ligand–gated ion channel (nicotinic acetylcholine receptor)34,45. Thus, regulation of various ion channels by toxin–like GPI–anchored proteins may be an evolutionarily conserved mechanism, and SSS and Lynx–1 may be founding members of a family of cell–surface proto–toxins that modulate ion channel properties to control neuronal excitability and signaling. Although BLAST analysis with the primary sequence of SSS does not reveal an obvious mammalian ortholog11, there are a number of mammalian proteins with a Ly–6 domain and a GPI anchor, one of which may represent a functional homolog of SSS.

In summary, we demonstrate that SSS is a novel regulator of Shaker expression, localization, and function in vivo. We propose that SSS acts as an endogenous “proto–toxin” that forms a complex with Shaker and promotes its stability and activity at the cell surface. Since dysregulation of channel function causes a number of inherited human diseases, including migraine, epilepsy, and cardiac arrhythmias46,47, identification and characterization of additional toxin–like regulators of ion channels may prove to be a fruitful approach for discovering novel treatment options for these diseases.

METHODS

Fly Stocks and Transgenic Fly Lines

All lines used in behavioral experiments, including Gal4 and UAS lines, were outcrossed at least 5 times into an isogenic white background (iso31) obtained from the Bloomington Stock Center. Shaker line was obtained from D. Bushey and B. Ganetzky, and DAT was obtained from K. Kume. eag (#1442), Cha-Gal4 (#6793), D42-Gal4 (#8816), OK107-Gal4 (#854), TH-Gal4 (#8848), repo-Gal4 (#7415), 24B-Gal4 (#1767) and elav-Gal4 (#458) were obtained from the Bloomington Stock Center. Sep54-Gal4 and Mai301-Gal4 were obtained from G. Korge, and vGlut-Gal4 and dilp2-Gal4 were obtained from J. Simpson and E. Rulifson, respectively. Other driver lines were obtained as previously described19. sss and sss were described previously11.

Transgenic fly lines carrying either the UAS-sss or sss-Gal4 construct were generated by standard techniques in the isogenic background iso31 (Rainbow Transgenics). For the UAS-sss construct, the entire coding region of sss was amplified by PCR using the following primers: 5′-GAA TTC ACC ATG TGG ACG CAG AGA AAT GCA GTT GG-3′ and 5′-GTC GAC GAG CCT AAC ACT TTC TAT CTG CTG AGC-3′. The PCR product was inserted into the EcoRI and XhoI restriction sites of pUAST, a P-element vector that contains the Gal4 binding sequence, UAS. The sss-Gal4 construct contained ~3.5 kb of the sss promoter, including the upstream intergenic region and the first and second introns of the sss gene. The following primers were used to amplify this region from wild-type genomic DNA: 5′-AAT CTA GAC TTG TAC TCT CAT GCG CTC-3′ and 5′-GCG GAT CCG CCT TGC CAC CCA CC-3′. The PCR product was inserted into the XbaI and BamHI restriction sites of the pPT-Gal transformation vector, upstream of the Gal4 coding sequence.

Antibody Generation

Because our previously-described antibody raised against a peptide antigen poorly recognizes glycosylated SSS11 and does not produce SSS-specific signal in whole-mount brain samples, we raised a new antibody against glycosylated SSS as the antigen. To produce soluble, glycosylated SSS protein, we inserted the coding region of sss minus the C-terminal GPI-anchor signal into the pAcGP67A baculovirus transfer vector (BD BioSciences) via the following primers: 5′-TAC CCG GGG AAT GTC AAA CGC GAT CG-3′ and 5′-ATC TAG ACT ACT TGT CAT CGT CGT CCT TGT AGT CAT TGC ACA TAT CTT CCT CAC-3′. Since the vector contains an N-terminal signal peptide, the native signal peptide was also removed from the sss coding region, and to facilitate purification, a C-terminal FLAG tag was added. Expression and purification of soluble SSS protein was performed at the Protein Expression Facility of Wistar Institute. To ensure proper glycosylation, SSS protein was expressed in High-Five insect cells (Invitrogen). Soluble SSS protein, purified using an anti-FLAG M2 agarose bead column (Sigma), was used to generate a new polyclonal antibody, UPGP69, in a guinea pig (Cocalico Biologicals).

To generate an antibody to Shaker, we used as the antigen a portion of the Shaker protein common to all isoforms fused to glutathione-S-transferase (GST). To generate this fusion construct, 215 amino acids were amplified by PCR using the following primers: 5′-AAG AAT TCA ATT TGC CCA AAT TGA GCA GTC AAG AC-3′ and 5′-AAT CTA GAG TCG ACA AGA TCT GTG ATG TCA GGC ACC TCG TCT TC-3′. The PCR product was subcloned into a modified pGEX vector (GE Lifesciences). GST-Shaker fusion protein was expressed in BL-21 cells (Novagen) and purified using glutathione sepharose beads (GE Life Sciences). After cleavage of GST using thrombin (GE Life Sciences), the Shaker antigen was used to generate a polyclonal antibody, UPR55, in a rat (Cocalico Biologicals).

Western Blot Analysis and Quantitative Real-Time PCR

Fly heads were homogenized and lysed in extraction buffer (20mM HEPES, pH 7.5, 100mM KCl, 20mM β-glycerophosphate, 100mM Na3VO4, 10mM EDTA, 0.3% Triton X-100, 1mM DTT, and a cocktail of protease inhibitors) for 15 min at 4°C. SDS sample buffer was added to head extracts and after 5 min of boiling, extracts were loaded onto 4-12% NuPAGE gels (Invitrogen) for SDS-PAGE. Head extracts from seven females were loaded per lane. Antibodies to SSS (UPGP69), Shaker (UPR55), and Eag48 were used at 1:1000, and antibody to β-Actin (Abcam) was used at 1:8000. Extracts from Shaker flies were included in the diluted Shaker antibody solution to reduce non-specific signal. Immunoreactive bands were visualized using enhanced chemiluminescence reagents (Pierce) and X-ray film. Films were scanned (Epson WorkForce 600) and imported into Photoshop 8.0 (Adobe), and the average intensity of each band was quantified using the histogram command. For background correction, the average intensity of the region immediately above or below the band of interest in the same lane was subtracted. To control for loading, the ratio between the signal intensities of the band of interest and the Actin band in the same lane was computed.

Quantitative real-time PCR was performed essentially as described49 except that the following Sh-specific primers were used: 5′-ATT ATC AGA GTG GTG GCC GAC T-3′ and 5′-CGT CTA AAG GGA CAT TGA CCG-3′.

Co-Immunoprecipitation

cDNA encoding the ShakerD isoform in a modified pGEM9zf- vector and cDNA encoding sss in a modified pBluescript vector were each linearized using NotI and used to generate cRNA with mMessage mMachine (Ambion). Xenopus laevis were handled according to approved protocols and anesthetized by immersion in 0.18% tricaine solution (Sigma). Oocytes were collected and dissociated in 25 mg/ml collagenase (Type I, Sigma) in 50% L-15 medium/50% 10 mM HEPES (pH 7.4) for 45 min at room temperature. Oocytes were then washed with L-15/HEPES, incubated at 18° C overnight and injected the following day with 1.4 ng ShakerD cRNA and either 1.4 ng sss cRNA or an equivalent concentration of transcription reaction mixture from which cDNA template was omitted. Following injection with cRNA, oocytes were maintained in L-15/HEPES at 18° C until experiments were performed, 3-4 days later. 20 cells were lysed in extraction buffer (10 mM Tris, pH 7.4, 100 mM NaCl, 5 mM EDTA, 1% Triton X-100, 0.05% SDS, and Complete protease inhibitors (Roche). Precipitates were removed by microcentrifugation at 10,600 RCF for 10 min at 4 C. 5% of supernatants were saved as a control for subsequent Western blotting. The remaining supernatants were mixed with 1 μl antibody to Shaker (UPR55) at 4° C for 2 hrs. 30 μl Dynal protein G-conjugated magnetic beads (Invitrogen) were used to precipitate Shaker-bound protein from solution overnight with shaking. Immunoprecipitates were washed 6 times with 1 ml cold extraction buffer except that Triton X-100 concentration was reduced to 0.5%. Western blotting was performed as above.

Immunohistochemistry

Immunostaining of whole-mount brain samples was performed essentially as described19, except for the following modifications. For staining with antibody to Shaker, dissected brains were fixed in Bouin’s fixative (Fisher) for 20 min at 4°C. For staining with antibody to SSS, brains were fixed in 4% paraformaldehyde in phosphate buffered saline (1.86 mM NaH2PO4, 8.41 mM Na2HPO4, and 175 mM NaCl) for 30 min at room temperature. Antibodies to Shaker and SSS were used at 1:2000 and 1:3000, respectively. Fluorescent secondary antibodies were used at 1:2000 (Molecular Probes). To reduce non-specific signal, extracts of Shaker or sss mutant flies were included as additional blocking agents during incubation with antibodies to Shaker or SSS, respectively. Immunostained brain or thoracic ganglion samples for wild-type and mutant animals were processed at the same time and imaged with the same settings on a Leica TCS SP5 confocal microscope.

Behavioral Assays

Flies were maintained on standard molasses-yeast-cornmeal food at room temperature, and were entrained to a 12-hr:12-hr light:dark cycle for at least two days before being assayed for sleep. 3- to 7-day old female flies were monitored using the Drosophila Activity Monitoring System (Trikinetics) at 25°C, and data were analyzed using MATLAB-based (MathWorks) custom software as described11. Sleep was identified as periods of inactivity lasting at least 5 minutes2. Ether-induced leg shaking was assayed as described11.

In Vivo Electrophysiology

Wandering third-instar larvae were immersed in a Ca2+-free saline (HL3.1) and dissected to access the neuromuscular junction as described50. Recordings were collected from muscle 6 of hemisegments A3-A5 at room temperature (21-23°C)50 by Sylgard-coated (Dow Corning) electrodes. The voltage-sensing and current-injection electrodes had initial resistances of 8-20 and 4-10 MΩ, respectively, when filled with a 2 M KCl solution with 10 mM EGTA and a pH of 7.2 (with KOH). The output of the amplifier (OC-725C, Warner) was low-pass filtered at 1-kHz (8-pole Bessel, model 902, Frequency Devices) and digitized using an AD/DA converter (ITC16, HEKA). Data were recorded/stored by PatchMachine and exported to Igor Pro 6.0 (Wavemetrics) for later analysis.

mEJPs were recorded over 2.5 minutes in an HL3.1 saline containing 1.5 mM Ca2+ via a single intracellular electrode placed near the mid-point of the muscle. A custom Igor Pro (Wavemetrics) routine based on the NeuroMatic analysis software (www.neuromatic.thinkrandom.com) identified the mEJPs in the record and calculated the average mEJP frequency.

Ionic currents were elicited/recorded in a Ca2+-free HL3.1 solution (with 5 mM EGTA) via two intracellular electrodes placed at opposite ends of the muscle. Muscles were depolarized either from a resting potential of −80 mV to elicit IA and IK or after a 200 ms pre-pulse to −20 mV to elicit IK alone. I/V curves were generated by plotting peak (for IA) or steady state (for IK) current densities (nA/nC) against test pulse voltage. Cellular capacitance was calculated by the equation: Iramp–C(dV/dt)=Istep, where Iramp is recorded at a particular voltage during a ramp of dV/dt and Istep is recorded at steady state at that voltage. Time to peak was measured at 10 mV.

In Vitro Electrophysiology

Plasmid DNAs in pGWI or pcDNA3 expression vectors coding for Drosophila wild-type ShakerB, sss and GFP (for identification of successfully transfected cells) were transfected in HEK-tsA cells by FuGENE6 (Roche); inside-out and whole-cell patch-clamp recordings were conducted 2 days following transfection. For both, the extracellular solution contained (in mM): 130 NaCl, 10 KCl, 2 CaCl2, 2 MgCl2, 10 HEPES, 15 glucose, and pH 7.4 (with N-methyl-D-glucamine (NMG)). The intracellular solution contained (in mM): 140 KCl, 2 MgCl2, 11 EGTA, 10 HEPES, and pH 7.2 (with NMG). Ionic currents were elicited by depolarizing pulses from a holding voltage of - 100 mV. Time-to-peak (t) or time-to-half-max (t) were measured at 15 mV. There was no correlation between the Shaker current kinetic effects and current magnitude, indicating a specific effect of SSS on Shaker current kinetics. Inside-out and whole-cell patch-clamp experiments were performed using an Axopatch 200A amplifier (Molecular Devices). The amplifier output was filtered at 10 kHz and digitized at 100 kHz through an ITC-16 AD/DA interface (HEKA). Data were collected and analyzed by using Igor Pro.

For Xenopus oocyte recordings, cells were prepared and injected with cRNA encoded by ShakerD or sss as described above, except that 7 pg ShakerD cRNA and 14 ng sss cRNA were used per cell. Membrane currents were studied by two-microelectrode voltage clamp (Axoclamp-2A, Molecular Devices). The two intracellular microelectrodes (~1 MΩ) were filled with 3 M KCl. Currents were sampled at 10 kHz and filtered at 2 kHz. Shaker currents were recorded in standard saline containing (in mM): 2 KCl, 96 NaCl, 2 CaCl2, 10 HEPES (pH 7.4). Depolarizing pulses were elicited from a holding potential of −70 mV to voltages between −80 and 60 mV in 20 mV increments. P/4 leak subtraction was employed in hyperpolarizing pulses from the same holding potential. Only oocytes with leak currents less than 50 nA were used. Data collection and kinetic analyses were performed using PClamp9 (Molecular Devices).

Statistical Analyses

The differences in sleep amount or mEJP frequency among multiple genotypes were analyzed with one-way ANOVAs followed by Tukey’s HSD tests for post hoc comparisons. For comparison of behavioral and electrophysiological data between pairs of conditions, Student’s t-tests (unpaired, two-tailed) were performed with Bonferroni correction for multiple comparisons where applicable. The genetic rescue experiments of the NMJ phenotypes were analyzed with two-way ANOVAs followed by Student’s two-tailed t-tests with Bonferroni correction.