Sec22 Regulates Endoplasmic Reticulum Morphology but Not Autophagy and Is Required for Eye Development in Drosophila

Background: ER morphological changes are often observed in disease conditions, but the molecular mechanisms remain unclear. Results: Malfunction of Sec22 and its binding partners resulted in ER expansion and defects in fly eye development. Conclusion: Sec22 regulates ER morphology through regulating ER-Golgi trafficking but not autophagy. Significance: ER morphology changes under the disease conditions might be due to the defects of ER-Golgi trafficking. The endoplasmic reticulum (ER) is a highly dynamic organelle that plays a critical role in many cellular processes. Abnormal ER morphology is associated with some human diseases, although little is known regarding how ER morphology is regulated. Using a forward genetic screen to identify genes that regulated ER morphology in Drosophila, we identified a mutant of Sec22, the orthologs of which in yeast, plants, and humans are required for ER to Golgi trafficking. However, the physiological function of Sec22 has not been previously investigated in animal development. A loss of Sec22 resulted in ER proliferation and expansion, enlargement of late endosomes, and abnormal Golgi morphology in mutant larvae fat body cells. However, starvation-induced autophagy was not affected by a loss of Sec22. Mosaic analysis of the eye revealed that Sec22 was required for photoreceptor morphogenesis. In Sec22 mutant photoreceptor cells, the ER was highly expanded and gradually lost normal morphology with aging. The rhabdomeres in mutants were small and sometimes fused with each other. The morphology of Sec22 mutant eyes resembled the eye morphology of flies with overexpressed eyc (eyes closed). eyc encodes for a Drosophila p47 protein that is required for membrane fusion. A loss of Syntaxin5 (Syx5), encoding for a t-SNARE on Golgi, also phenocopied the Sec22 mutant. Sec22 formed complexes with Syx5 and Eyc. Thus, we propose that appropriate trafficking between the ER and Golgi is required for maintaining ER morphology and for Drosophila eye morphogenesis.

The endoplasmic reticulum (ER) 4 plays pivotal roles in many cellular processes. In addition to its important function in pro-tein synthesis, modifications, and quality control, the ER is also critical for lipid synthesis, autophagy, and calcium homeostasis (1)(2)(3). The ER makes close contacts with other organelles, including mitochondria, the Golgi apparatus, endosomes, peroxisomes, and lysosomes. It exchanges lipids and proteins with these organelles to regulate their biogenesis and function (4,5). Thus, the ER has diverse functions, and ER malfunctions can cause numerous human diseases, including diabetes and neurodegeneration (6).
The ER is a membrane network that consists of tubules and sheets that extend throughout a cell (7,8). The ER is highly dynamic and constitutively undergoes rearrangements, which are critical for ER functions (9 -11). ER morphological changes, including fragmentation and expansion, are often observed in cells that are subjected to pathological insults (6). However, the molecular mechanisms underlying these ER morphological changes remain unclear.
Using a forward genetic screen to identify genes that regulated ER morphology, we obtained a complementation group with remarkable ER proliferation and expansion. Molecular mapping located a lesion on Sec22, a gene encoding for a SNARE protein enriched on the ER (12,13). SNARE proteins are a family of conserved proteins that mediate membrane fusion between vesicles derived from one subcellular compartment and their targeted membranes (14,15). In the secretory pathway, proteins are transported by vesicle budding, docking, and fusion. Different SNAREs mediate the fusion step between various vesicles and their ultimate destinies. Vesicle membrane-localized v-SNAREs and targeting membrane-localized t-SNAREs form helix bundles to drive membrane fusion. Subsequently, these bundled SNAREs are dissociated and recycled by N-ethylmaleimide-sensitive factor (16).
Sec22 family proteins are highly conserved from yeast to human. In yeast, there is only one Sec22 gene, and its functions partially overlap with those of another gene, ykt6 (13). Sec22p is involved in transport between the ER and Golgi compartments in both anterograde and retrograde directions in yeast (12). In addition, Sec22p is required for autophagosome biogenesis by regulating the transport of Atg9, an essential protein for autophagosome formation, to the phagophore assembly site (17). In both yeast and plants, Sec22p/SEC22 regulates cesium accumulation, which indicates that Sec22 proteins play a role in vacuole function (18). A loss of SEC22 in plants also results in Golgi fragmentation and defects in gametophyte development (19). Studies of the rice fungi show that Sec22 is required for conidiogenesis, cell wall integrity, and host plant infection (20). Several Sec22 genes, SEC22A, SEC22B, and SEC22C, were also found in humans. In cultured mammalian cells, SEC22 proteins are also required for ER to Golgi trafficking (21,22). However, knocking down SEC22B expression in cultured mammalian cells does not cause autophagy defects, presumably because of redundancy (23). It was recently shown that SEC22B also has a conserved nonfusogenic function in plasma membrane expansion (24).
All of these studies demonstrated that Sec22 was a key regulator of the secretory pathway. However, surprisingly, there have been no studies of the physiological functions of Sec22 in animal development and morphogenesis. In this study, we found that Sec22 was an essential gene in flies. A loss of Sec22 resulted in morphogenesis defects in fly eyes. The ER was highly proliferated, and its morphology underwent very dramatic changes in Sec22 mutant flies. In contrast to yeast orthologs, Sec22 was not required for starvation-induced autophagy in Drosophila. Interestingly, a loss of Syntaxin 5 (Syx5), which encodes for a t-SNARE in Golgi, also phenocopied Sec22 mutants, which indicated that appropriate trafficking between the ER and Golgi was critical for ER morphology.

EXPERIMENTAL PROCEDURES
Molecular Biology-To generate a Sec22 genomic rescue construct, a 3.3-kb genomic fragment that contained the Sec22 gene was amplified using the primers, 5Ј-TGAGATCTGTC-CATGCAGAGGATGGTCTTCG-3Ј and 5Ј-TACTCGAGCC-AGAGCTTCAGCAGAACCACAGC-3Ј, using genomic DNA that was purified from FRT19A isogenized flies. To generate a Sec22 expression vector, we inserted the Sec22 cDNA into a pattB UAS-3HA vector. A 3XHA tag was fused to Sec22 at the N terminus. To generate a Flag-tagged Syntaxin 5 expression vector, we inserted the Flag sequence and Syntaxin 5 cDNA into the pattB UAS expression vector. The Flag tag was fused to the N terminus of the Syx5 protein. A Myc-Eyc expression vector was generated by inserting full-length eyc cDNA into the pattB UAS-Myc expression vector. Myc was fused to the N terminus of the Eyc protein.
Immunostaining for Fly Fat Bodies-Dissected fly fat bodies were 3.7% formaldehyde in PBS for 20 min and then washed three times with PBST (PBS ϩ 0.1% Triton X-100). Tissues were incubated with a primary antibody (rabbit anti-HA used at 1:1000; CST) overnight, extensively washed, and then incubated with a secondary antibody (Alexa 488-conjugated used at 1:500; Invitrogen) at room temperature for 1 h. After extensive washing, samples were mounted in vector shield and observed by a confocal microscope.
Phalloidin and Immunostaining of the Photoreceptor Cells-For the late pupae stage flies, the dissected brain-eye complexes ware fixed in PBS with 4% formaldehyde for 20 min. For the adult flies, heads were fixed in PBS with 4% formaldehyde for 1 h upon removal of the proboscis. Then the photoreceptor cells were dissected and fixed for 15 min. After the fixation, the tissues were washed three times with PBST (PBS ϩ 0.4% Triton X-100) and stained with primary antibody mouse anti-Rh1 (1:50; Developmental Studies Hybridoma Bank) overnight at 4°C. After extensive washing with PBST, secondary antibody (1:500, Invitrogen) and Alexa 488-labeled phalloidin (1:1000, Invitrogen) were incubated with the tissues for 2 h at room temperature. Samples were washed with PBST four times and mounted in vector shield and observed by a confocal microscope.
Cell Culture and Immunoprecipitation-S2 cells were cultured at room temperature and transfected using Opti-PEI. For co-immunoprecipitation, cells were harvested at 48 h after transfection and lysed with lysis buffer. Cell lysates were incubated with beads (anti-HA, anti-Myc, or anti-Flag) at 4°C for 4 h in lysis buffer. After extensive washing, the immunoprecipitation products were analyzed by Western blot using anti-HA (1:1,000), anti-Myc (1:1,000), or anti-FLAG (1:1,000), followed by an HRP-conjugated secondary antibody (1:5,000).
Transmission Electron Microscopy-For electron microscopic observations of photoreceptors, fly heads were dissected and fixed in 4% paraformaldehyde and 1% glutaraldehyde at 4°C overnight. Then the samples were post-fixed in 2% OsO4 for 2 h, followed by dehydration in ethanol and propylene oxide. Samples were embedded in Embed-812 resin (Electron Microscopy Sciences). TEM images were acquired using a transmission electron microscope equipped with a digital camera.
Confocal Microscopy-All mounted samples were examined and imaged with a confocal microscope LSM710 (Carl Zeiss) outfitted with a Plan-Apochromat 63ϫ 1.4NA oil immersion objective lens (Carl Zeiss). The data were acquired using Zen 2010 Software and processed with Photoshop CS (Adobe).

RESULTS
Identifying a Complementation Group, ERM1, with ER Morphology Defects-To identify mutants that had ER morphology defects, we screened about 700 chemically induced lethal mutations on X chromosome (25). We labeled ER structures using Cg-Gal4-driven UAS-KDEL-GFP expression in the Drosophila fat body cells and made mutant clone negatively marked with RFP ( Fig. 1A). By comparing the patterns of the KDEL-GFP in the RFP negative mutant cells with those in the neighboring RFP positive wild type cells, we identified one complementation group, ERM1. KDEL-GFP punctate structures became larger and accumulated inside the ERM1 mutant clones (Fig.  1B, panels AЈ, aЈ, BЈ, and bЈ), which indicated that the ER was overproliferated and had expanded. To determine whether other organelles were also affected in these mutant clones, we also examined the patterns for Rab7-GFP, ManII-GFP (26), and Mito-GFP, which label late endosomes, the Golgi apparatus, and mitochondria, respectively. There was a dramatic enlargement and accumulation of Rab7-GFP punctate structures inside ERM1 mutant clones (Fig. 1B, panels CЈ, cЈ, DЈ, and dЈ). The Golgi marker ManII-GFP became diffusely distributed as compared with its distribution in a control (Fig. 1B, panels EЈ, eЈ, FЈ, and fЈ). The mitochondria pattern appeared to be intact inside these mutant clones (Fig. 1B, panels GЈ, gЈ, HЈ, and hЈ). These data suggested that the ER, late endosomes, and Golgi were all affected in ERM1 mutant cells.
ERM1 Mutants Correspond to Sec22 Mutants-Because the ERM1 phenotypes were interesting, we performed duplication and deficiency mapping. ERM1 was rescued by an X chromosome duplication that covered a region from 1A1 to 2C1. Several overlapping deficiencies that covered this region were used to further narrow down the mutant lesion. Df(1)BSC534 did but the overlapping Df(1)ED6433 did not rescue the lethality of ERM1, which indicated that the mutation was localized in the region deleted in Df(1)ED6433 but not in Df(1)BSC534. To further pinpoint the mutant region, small duplications that covered the deleted region in the deficiencies were used for a complementation test. ERM1 was rescued by two overlapping small duplications: Dp(1;3) DC012 and Dp(1;3) DC013, which narrowed the putative gene down to nine genes ( Fig. 2A). Sequencing revealed point mutations in Sec22 (Fig. 2B). A splicing acceptor G to A mutation at the end of the third intron was detected in ERM1. To analyze the transcripts in this mutant, we isolated mRNA from the mutant larvae, made cDNAs, and sequenced the cDNAs with two pair of primers. Two different cDNAs were identified: Sec22 mu1 and Sec22 mu2 (Fig. 2C). An alternative splicing acceptor site was adopted by Sec22 mu1, which resulted in a deletion of part of the fourth exon. Wild type Sec22 encodes for a SNARE protein that contains a longin domain and a synaptobrevin domain (Fig. 2D). The frameshift caused by the deletion in Sec22 mu1 resulted in the mistranslation of the most part of the synaptobrevin domain. Sec22 mu2 had an unspliced intron and that led to a premature stop codon in the synaptobrevin domain.
To confirm that ERM1 mutants indeed corresponded to Sec22 mutants, a genomic fragment that contained only the Sec22 gene was introduced into these mutants ( Fig. 2A). The genomic rescue construct not only fully rescued the lethality of ERM1 to adulthood but also rescued the ER morphology defects in the mutant clones (Fig. 2E). It indicated that Sec22 was the gene affected in this mutant.
Sec22 Is Not Required for Autophagy in Drosophila-A recent study with yeast showed that Sec22 is required for autophagosome formation. Because the ER is degraded in the autophagosome through "ER-phagy" (27), the accumulated morphologically abnormal ER in Sec22 mutants could be due to an autophagy malfunction.
To test whether Sec22 was required for autophagy in flies, we examined different autophagy markers in Sec22 mutant cells after their starvation. We labeled autophagy vacuoles in fat bodies by expressing different markers driven by a fat body Gal4 driver, Cg-Gal4 (28). We negatively labeled the Sec22 mutant clones with RFP in third instar larvae fat bodies and then examined the different autophagy markers after starvation for 4 h.
Autophagy initiation requires type III PI3K activity, which can be monitored based on the intracellular distribution of FYVE-GFP. Without PI3K activity, FYVE-GFP signals are dif-FIGURE 1. Identifying a complementation group with ER morphology defects. A, screening strategy used to identify mutants with ER morphology defects. B, complementation group ERM1 had an expanded ER, enlargements of late endosomes, and abnormal Golgi morphology. However, mitochondria were intact. Control and mutant clones are marked by a loss of RFP (red) and outlined by the dashed lines. aЈ-hЈ, green channels of AЈ-HЈ, KDEL-GFP was used to label the ER, Rab7-GFP was used to label late endosomes, ManII-GFP was used to label the Golgi apparatus, and Mito-GFP was used to label mitochondria.
fusely distributed inside cells. If PI3K is activated, then FYVE-GFP exhibits punctate staining (29). In Sec22 mutant cells, FYVE-GFP exhibited a punctate distribution that was similar to that in control cells (Fig. 3, A and AЈ), which indicated that PI3K activity was intact.
Atg8 is an ubiquitin-like protein that is required for autophagosome formation and autophagy progression (30). Without starvation, Atg8 signals are diffusely distributed inside cells. Upon starvation, Atg8 forms punctate structures and labels autophagosomes. Once autophagosomes fuse with lysosomes, Atg8 is degraded inside autolysosomes. In Sec22 mutant clones, Atg8-GFP punctate structures were formed, and these patterns were comparable with those in controls (Fig. 3, B and BЈ), which indicated that Sec22 was not required for autophagosome formation.
To monitor autophagosome and lysosome fusion, Atg8-GFPRFP was used as a marker. GFP signals but not RFP signals are quenched inside acidic autolysosomes; thus, autophagosomes will appear yellow, and autolysosomes will appear red (31). If there are fusion defects between autophagosomes and FIGURE 2. ERM1 mutants correspond to Sec22 mutants. A, deficiency and duplication mapping located the ERM1 lesion to a small genomic fragment that contains nine genes, including Sec22. B, Sanger sequencing reviewed a G to A mutation at the splicing acceptor site on Sec22. C, diagram indicating the genomic organization and the resulting mRNA of the Sec22 locus. The exons were shown as bars with different colors, and the introns were shown as dotted lines. The positions of the primers used for RT-PCR were indicated. The point mutation on ERM1 resulted in two transcripts (Sec22 mu1 and Sec22 mu2) different from the wild type (Sec22 WT). The alignment of the Sec22 mu1 with Sec22 WT showed that a deletion in Sec22 mu1 resulted from an alternative splicing site used by Sec22 mu1. The alignment of Sec22 mu2 with Sec22 WT showed that an intron was failed to be spliced, and an insertion was produced in Sec22 mu2. D, diagram indicating the domain organization of Sec22 protein. The proteins encoded by Sec22 WT, mu1, and mu2 were shown. E, Sec22 genomic rescue construct rescued the ER morphology defects of Sec22 mutant clones. The ER was labeled with KDEL-GFP. The clones were negatively labeled with RFP.

Sec22 Regulates ER Morphology but Not Autophagy
lysosomes, then most Atg8 punctate structures will appear as yellow; otherwise, the majority of Atg8 punctate structures will appear as red. The yellow and red signals of Atg8-GFPRFP punctate structures in Sec22 mutant clones were same as those in control cells (Fig. 3, C and CЈ), which indicated that Sec22 was not required for autophagosome maturation.
To examine autophagy flux in Sec22 mutant cells, we checked the patterns of p62 (32), an adapter protein that is digested via autophagy. There was no difference in the p62 protein distribution between Sec22 mutants and wild type controls (Fig. 3, D and DЈ). In summary, Sec22 was not required for autophagy in fly fat body cells. Thus, the accumulated ER and morphological changes were not due to autophagy failure.
Syx5 Interacts with Sec22 to Regulate ER Morphology-Because autophagy was not affected by a loss of Sec22, the accumulation of morphologically abnormal ER could have resulted from other conserved functions of Sec22. In yeast, Sec22 forms a complex with the Golgi SNARE protein Sed5p to mediate the fusion of ER-derived vesicles with the Golgi compartment (33). In Sec22 mutant fat body cells, the ER was expanded, and Golgi morphology had changed, which indicated that Sec22 indeed was required for membrane trafficking between the ER and Golgi in flies. Thus, we hypothesized that trafficking defects between the ER and Golgi had resulted in the ER morphological changes.
To test this, we first examined whether Syx5 (Syntaxin 5), encoded by the fly ortholog of sed5, could bind to Sec22. We performed immunoprecipitation using cultured S2 cells and found that Sec22 indeed formed a complex with Syx5 (Fig. 4A). When we knocked down Syx5 in fly fat bodies using RNAi, we found that KDEL-RFP punctate structures became larger and had accumulated inside cells (Fig. 4, B and C). This indicated that the ER had expanded in Syx5 RNAi tissues, a phenotype that was very similar to the Sec22 mutants. Sec22 is a v-SNARE on the ER membrane, and Syx5 is a t-SNARE on the Golgi compartment. The ER morphology change in those cells that had lost either SNARE protein suggested that the trafficking failure between the ER and Golgi had triggered ER expansion.
Interestingly, Syx5 overexpression in fat body cells also led to ER expansion similar to the ER morphology in the Syx5 RNAi tissues, suggesting Syx5 overexpression has dominant negative effects (Fig. 4E). In yeast, ER-Golgi transport requires four SNARE proteins, Sec22p, Bos1p, Bet1p, and Sed5p (encoded by a yeast ortholog of Syx5), to form complexes. The dominant negative effects of Syx5 overexpression probably is due to the extra Syx5 competing with the endogenous Syx5 to form ineffective complexes with other endogenous SNARE proteins, such as Sec22 or the proteins encoded by the orthologs of Bos1p or Bet1p. Strikingly, when we co-expressed Sec22 and Syx5, the ER punctuate structures in the fat body cells were much larger than those in the cells with Syx5 overexpression alone (Fig. 4,  D-F). Because Sec22 overexpression did not have ER morphology defects, the enhancement of the Syx5 overexpression phenotypes suggested that Sec22 might form a complex with Syx5, and together they were a better competitor than Syx5 alone to titrate out of other SNARE proteins. These data implied that Sec22 and Syx5 might function in a same pathway to regulate ER morphology.   panels). B-F, Syx5 RNAi (C) and overexpression (E) resulted in KDEL-RFP labeled ER proliferation and expansion. Sec22 overexpression alone had no effect on the ER morphology (D) but enhanced the ER morphology defects when co-expressed with Syx5 (F). Cg-Gal4 was used to drive the expression of KDEL-RFP, Syx5shRNA, UAS-Flag-Syx5, and UAS-3XHA Sec22. CTL, control; IP, immunoprecipitation.
Sec22 Is Required for Eye Morphogenesis-The dramatic ER morphological changes in the Sec22 mutant cells suggested that Sec22 played a critical role in regulating ER function. However, the physiological function of Sec22 has not been previously investigated in animals. We found that a Sec22 hemizygous mutant cannot survive to the adulthood. To investigate whether Sec22 was required for nerve system development and neuron homeostasis, we generated Sec22 mutant clones in the eye using the eyFLP system. In wild type control eyes, round, tightly packed, and oval-shaped rhabdomeres were in a trapezoid arrangement. In Sec22 mutant eyes, irregularly shaped rhabdomeres were small and sometimes fused with each other (Fig. 5, A, a, C, and c). Inside photoreceptor cells, the ER was highly expanded with numerous stacks and gradually lost its normal morphology with aging (Fig. 5, A-D and a-d). Occasionally, lipid droplets could be detected in the cytoplasm, another hallmark of ER malfunction (Fig. 5, A-D and a-d).
It has been reported that mistrafficking of Rh1 (Rhodopsin 1) leads to retinal developmental defects and degeneration (34,35). Rh1 is a light sensor that presents in the R1-R6 photoreceptor cells. During fly photoreceptor cell development, Rh1 is synthesized and matured in the ER and transports to the rhabdomeres through the Golgi. The ER defects are likely to cause mistrafficking of Rh1 (34,35). We therefore tested whether there is Rh1 trafficking defects in the Sec22 mutants. We made Sec22 mutant clones in the fly eyes and stained the tissue with anti-Rh1 antibody and phalloidin to examine the distribution Rh1 in the photoreceptor cells at the late pupae (84 h after puparium formation) and adult stages. There was a massive accumulation of Rh1 in the cytoplasm (Fig. 5E), which might explain the degeneration phenotypes we observed in Sec22 mutant eyes.
Syx5 Mutants, Sec22 Mutants, and Eyc Overexpression Animals All Have Similar ER Phenotypes-Studies of Syx5 functions in the fat body cells suggested that it might form a complex with Sec22 to regulate ER morphology. We then tested whether Syx5 mutants also had phenotypes similar to those of Sec22 mutants in the eyes. Indeed, the rhabdomeres were small and irregularly shaped in the Syx5 mutants. The photoreceptor cells were also packed with overproliferated ER and lipid droplets (Fig. 6, A and a).
The photoreceptor morphogenesis defects and ER accumulation in Sec22 mutants were reminiscent of a mutant called eyc (eyes closed) (36). eyc encodes for a fly p47 protein that forms a complex with p97 ATPase to regulate membrane fusion (37). Eyc overexpression during the early pupal stage resulted in fused rhabdomeres. Eyc misexpression at a later stage resulted in ER proliferation in the photoreceptor cells (Fig. 6, B and b) (36). The trafficking of Rh1 is defective in the fly eyes with Eyc overexpressed (36). All of these phenotypes were very similar to what we observed in Sec22 mutant eyes. To test whether Sec22 and Eyc interacts with each other, we performed IP experiments with cultured fly S2 cells. Indeed, Sec22 bound to Eyc (Fig. 6, C and D). We wondered whether Sec22, Syx5, and Eyc function in a same pathway to regulate ER morphology and photoreceptor cell morphogenesis. We knocked Syx5 known or overexpressed Eyc in the Sec22 mutant background using MARCM technology and analyzed the ER morphology in the fat body cells. Both Syx5 RNAi and Eyc overexpression in the Sec22 mutant cells led to cell growth defects. The cells became very small, which hindered the ER morphology analysis (Fig. 6, E-J). The synergistic effects of regulating cell size suggested that these proteins may have paralleled functions in cell growth. However, whether they work together in regulating ER morphology is still an open question.
Because both Eyc and Syx5 interact with Sec22, we hypothesized that Eyc might compete with Syx5 to bind Sec22. However, we did not observe any decrease of the interaction between Sec22 and Syx5 when Eyc was overexpressed (Fig. 6K). FIGURE 5. Sec22 is required for eye morphogenesis. A, a, C, and c, in 1-dayold wild type control (CTL) eyes, round, tightly packed, oval-shaped rhabdomeres were in a trapezoid arrangement (A and a). In age-matched Sec22 mutant eyes (C and c), the rhabdomeres were small and sometimes fused with each other (blue arrows). The ER was highly proliferated (red arrows), and lipid droplets (yellow arrows) were accumulated. B, b, D, and d, the ER gradually lost its shape and became highly accumulated inside photoreceptor cells with aging. E, the Rh1 trafficking was defective in Sec22 mutant photoreceptor cells. The Sec22 mutant clones were generated by eyFLP/FRT system. The mutant area was outlined, and the typical mutant photoreceptor cells were indicated with yellow arrows. Red, phalloidin (Pha); blue, Rh1.
We also did not observe any alleviation of ER morphology defects in Eyc overexpression cells when Sec22 was overexpressed. Therefore, Eyc overexpression phenotypes were not due to competing Sec22 with Syx5 (Fig. 6, L-O).

Losses of Sec22 and Syx5
Result in ER Expansion-The ER is highly dynamic, and its morphology is tightly regulated (10,11). Abnormal ER morphology is associated with hereditary spastic paraplegias and related disorders (38). In this study, we found that both Sec22 and Syx5 mutants had an overproliferated ER and expanded ER lumens. Sec22 is primarily localized on the ER, and Syx5 is found on the Golgi. The interaction between Sec22 and Syx5 mediates the fusion of ER-derived vesicles to Golgi cysts. The similar ER phenotypes between Sec22 and Syx5 mutants suggested that defective ER-Golgi trafficking resulted in ER proliferation and morphology defects.
ER proliferation has been found in cells that were exposed to multiple pathological insults; however, the molecular mechanisms involved are less well understood (6). It would be interesting to test whether the trafficking route between the ER and Golgi is blocked in these disease conditions. It is still not clear how these trafficking defects result in ER proliferation and morphology defects. ER stress could result in ER proliferation. Thus, it needs to be determined whether these Sec22 mutants have ER stress responses.
Eyc, p97, and ER Dynamics-SNARE proteins can assemble into unproductive cis-SNARE complexes that need to be disso-FIGURE 6. Syx5 mutants, Sec22 mutants, and Eyc overexpression animals have similar ER phenotypes. A and a, 1-day-old Syx5 mutants had phenotypes similar to those of Sec22 mutants. Rhabdomeres were small and fused (blue arrowhead), ER was proliferated (red arrowheads), and lipid droplets were accumulated (yellow arrows). B and b, GMR-Gal4-driven Eyc overexpression resulted in ER proliferation (red arrowheads) and lipid droplet accumulation (yellow arrows). C, HA-tagged Sec22 pulled down Myc-tagged Eyc. D, Myc-tagged Eyc also pulled down HA-tagged Sec22. E-J, Syx5 RNAi and Eyc overexpression in the Sec22 mutant cells led to cell growth defects. ER was labeled with KDEL-RFP (red). E, control clone. ciated by two ATPases: N-ethylmaleimide-sensitive factor (39) and p97 (40 -42). After their dissociation, SNAREs are available to form trans-complexes and promote another round of fusion. p47 is an adaptor protein that mediates the interaction between p97 and a SNARE complex (43,44). Interestingly, overexpression of Eyc (fly ortholog of p47) mimicked the loss of Sec22 and Syx5, which suggested that Eyc functioned within a paralleled or a same pathway as Sec22 and Syx5. We found that Sec22 could bind to Eyc. However, Eyc overexpression phenotypes are not due to Eyc competing Sec22 with Syx5. It is possible that the excess Eyc interferes the organization of the whole SNARE complex required for ER-Golgi trafficking. It is also possible that Eyc works in a paralleled pathway independent of Sec22 to regulate ER morphology.
Sec22 and Autophagy-Autophagy is a critical degradative pathway that is required for cellular homeostasis (45). SNAREs are important for membrane homophilic fusion during autophagosome formation (17,46). Sec22 facilitates Atg9 recruitment to the phagophore assembly site and therefore is required for autophagosome formation in yeast (17). However, in our study, Sec22 was dispensable for starvation-induced autophagy in flies. In yeast, autophagosomes are generated from the phagophore assembly site, which has not yet been identified in fly and mammalian cells (31). It is possible that different autophagic initiation structures determine whether Sec22 is required for autophagy. Interestingly, no autophagy defects are observed when SEC22B is knocked down in mammalian cells (46).
In yeast, ykt6 function overlaps with that of Sec22 (13). Ykt6p is required for autophagosome formation in yeast (17), and Ykt6p is highly conserved. It is possible that Ykt6 and Sec22 have redundant roles during autophagy.
The ER is one of the membrane sources of the autophagosome (47). In Sec22 mutants, the ER was highly proliferated. The lumens of the ER were expanded, and ER morphology changed dramatically. However, autophagosome formation was not affected in Sec22 mutants, which indicated that appropriate ER morphology was not absolutely required for autophagosome formation.
In summary, we found that trafficking between the ER and Golgi mediated by Sec22 and Syx5 was critical for maintaining ER morphology. Sec22 was also required for development and eye morphogenesis in flies.