Abstract
Apical extracellular matrix filling the lumen controls the morphology and geometry of epithelial tubes during development, yet the regulation of luminal protein composition and its role in tube morphogenesis are not well understood. Here we show that an endosomal-retrieval machinery consisting of Rab9, retromer and actin nucleator WASH (Wiskott–Aldrich Syndrome Protein and SCAR Homolog) regulates selective recycling of the luminal protein Serpentine in the Drosophila trachea. Secreted Serpentine is endocytosed and sorted into the late endosome. Vps35, WASH and actin filaments differentially localize at the Rab9-enriched subdomains of the endosomal membrane, where Serpentine containing vesicles bud off. In Rab9, Vps35 and WASH mutants, Serpentine was secreted normally into the tracheal lumen, but the luminal quantities were depleted at later stages, resulting in excessively elongated tubes. In contrast, secretion of many luminal proteins was unaffected, suggesting that retrograde trafficking of a specific class of luminal proteins is a pivotal rate-limiting mechanism for continuous tube length regulation.
The development of biological tubes is regulated by mutual interactions between cells and luminal extracellular matrix. Dong et al. show that retrograde recycling of luminal chitin deacetylase regulates Drosophila tracheal tubule geometry by restricting length independently of diameter.
Tubular organs support the uptake and exchange of nutrition, metabolites and gases that are essential for the normal physiology of animals. During development, geometry of such tubes must be precisely controlled, so that the circulation of luminal components matches the size of the growing organ and the rest of the organism. Loss of tube size regulation leads to pathological tubule dysfunctions such as polycystic kidney disease1.
The Drosophila tracheal system is a well-characterized model system for tubular organ morphogenesis2,3,4,5. After tube connection is complete, tracheal tubes undergo diametric and axial expansion to reach their final shape without cell proliferation, followed by clearance of luminal contents and gas filling before the larvae hatch into an air-filled environment6. Tracheal diametric expansion is initiated by a cell-intrinsic programme of apical membrane growth and secretion of luminal materials7, including zona pellucida domain-containing protein Piopio (Pio) and 2A12 antigen driven by the actin nucleator Dia and Myosin V motor6,8, and chitin, the major component of the apical extracellular matrix (aECM). Deposition of those luminal materials promotes the rapid diametric expansion9,10,11.
Longitudinal-axial growth follows diametric expansion. Src kinase has been recently identified as a positive factor for tube elongation12,13. aECM acts as a negative factor required to restrict tube length to a proper level14. When the remodelling of chitin polymer is compromised due to mutation of the secreted chitin deacetylases Serpentine (Serp) and Vermiform (Verm), the tracheal tubules exceed normal length15,16. Thus, maintaining the proper chitin deacetylase level is important for tube-length determination. The luminal localization of Serp and Verm is independent of Dia and Myosin V8. Thus, how chitin-modification enzymes are maintained in the tube and how cells dynamically regulate extracellular matrix protein composition in the lumen are not understood.
Retrograde protein trafficking involves the sorting of endocytosed proteins into a tubular endosomal membrane, which buds off and then fuses with the trans-Golgi network (TGN)17,18. This pathway requires the endosomal Rab family GTPase Rab9 (refs 19,20,21,22), the retromer, a multiple protein complex required for the outward budding of the endosomal membrane23,24,25,26 and actin nucleation-promoting factors WASH (Wiskott–Aldrich Syndrome Protein and SCAR Homolog)27,28. The protein cargoes recycled in this pathway include Mannose 6-phosphate receptors19,23, cell-surface protein Crumbs (Crb)29,30 and Wntless/Sprinter/Evenness31,32,33,34,35. The key remaining question is whether this pathway acts beyond the role in constitutive protein turnover and has an active regulatory role in morphogenesis.
Here we addressed the role of retrograde trafficking in tracheal tube morphogenesis, and found that Rab9, Vps35 (the core component of the retromer’s cargo recognition complex) and WASH together control the tracheal tube length by positively regulating the luminal deposition of Serp. We further show that Serp is a specific cargo for retromer-dependent endocytic trafficking. Combining genetic, biochemical and cell biological approaches, we established the relationship between Rab5, Rab9 and Rab7 in the retromer recruitment, and propose that Rab9 and the retromer function cooperatively in endocytotic Serp sorting from late endosomes (LEs) to the TGN via a WASH-associated vesicle-budding machinery. Our study further elucidates the connection between luminal protein trafficking and epithelial tube size control.
Results
Requirement for Rab9 in tracheal tube length restriction
Rab9 was identified from a screen of Rab family proteins showing localization similar to Arf-like3 GTPase in the tracheal system36. Rab9 mRNA was detected broadly in embryonic tissues, including the tracheal system (white arrowhead in Supplementary Fig. S1a). Three lethal deletions of rab9 were identified by mobilization of Minos transposon37 inserted into the rab9 locus (Supplementary Fig. S1c). In situ hybridization demonstrated that the mRNA expression level was significantly decreased in rab9-mutant homozygous embryos compared with wild-type embryos (Supplementary Fig. S1a,b). Trans-heterozygosity of rab956 and rab9199 created a deletion of rab9 only, and was used to identify rab9-mutant phenotypes. The most apparent defect among rab9 mutants (rab956/rab9199 and homozygotes of each mutant) was a convoluted dorsal trunk (DT) that was increased in length by approximately 15%, compared with wild-type embryos (Fig. 1a, Supplementary Fig. S1d–f). In contrast, the tube diameter was unaffected by the mutations (Supplementary Fig. S1g). Expression of UAS-GFP-Rab9 in the trachea (with btl-Gal4 driver) in rab9 mutants rescued the tracheal tube phenotype (Fig. 1c), indicating that Rab9 is essential for restricting the tracheal tube length.
Rab9 is required for the luminal retention of Serp
The long tracheal tube phenotype of the rab9 mutants resembled that of chitin deacetylase mutants15,16. The secreted chitin deacetylase Serp was first detected as cytoplasmic puncta in tracheal cells; it was then released into the lumen at the onset of the massive secretion that initiates tube diameter expansion (Supplementary Fig. S2a)6. At this stage, the GFP-Rab9 puncta overlapped only minimally with Serp (Fig. 2c and Supplementary Fig. S2a,b). After stage 15, the Serp-positive fraction among the GFP-Rab9 endosomes increased while the tracheal lumen expansion proceeded (Fig. 2a–c). A similar colocalization of RFP-Rab9 and Serp-chitin-binding domain (CBD)-GFP15 was observed in the tracheal system, in which Serp puncta were contained within RFP-Rab9 endosomes (Fig. 2d).
In rab9-mutant embryos, Serp secretion at early stage (stage 14) was normal (Fig. 2f). At late stage (stage 16), Serp expression was reduced in the tracheal lumen (blue arrowheads in Fig. 2k), and the Serp associated with the apical membrane was increased (Fig. 2p, white arrowheads). Strikingly, chitin deposition was not altered in rab9 mutants (compare Fig. 2m with Fig. 2k, , yellow arrowheads). To determine whether other luminal or membrane proteins were affected, we examined the expression and localization of the luminally accumulated 2A12 antigen (Fig. 2o), Pio and Verm (Supplementary Fig. S2c,d) and the membrane proteins Crb and Uninflatible (Uif) (Supplementary Fig. S2e,f), and found that their expression and localization were unaltered in the rab9 mutants. These data indicated that among the luminal and membrane proteins examined, Serp specifically requires Rab9 for its luminal localization.
To learn whether Rab9 is involved in the protein stability of Serp, we examined the expression level of Serp by western blotting, and found that the total amount of Serp was not altered by the rab9 mutation (Fig. 2e), suggesting that Rab9 regulates the localization rather than the stability of Serp.
Rab9 is involved in trafficking from endosomes to the TGN
To determine if Rab9 is involved in endocytic trafficking, we conducted a dextran dye uptake assay using fly embryos (Fig. 3a). The labelled dextran was found associated with GFP-Rab9 endosomes (arrowheads in Fig. 3a) at 30 min after dye injection and co-trafficked in tracheal cells (Fig. 3b). In S2 cells, the labelled dextran was included in GFP-Rab9-labelled vacuoles (Fig. 3c), indicating that Rab9 is involved in endocytic trafficking. Because Rab9 is implicated in retrograde trafficking in vitro19,20, we predicted that Rab9 would be colocalized with the TGN or the early or late endosomal markers. To test this hypothesis, we expressed markers for the TGN (GalT-CFP), early endosomes (GFP-Rab5), LEs (YFP-Rab7), lysosomes (GFP-LAMP1) or endoplasmic reticulum (GFP-KDEL) in RFP-Rab9-expressing tracheal cells. We found that RFP-Rab9 colocalized with GalT-CFP, GFP-Rab5 and YFP-Rab7 (blue arrowheads in Fig. 3d–f). Partial colocalization was observed with GFP-LAMP1 (Fig. 3g), but not with GFP-KDEL (Fig. 3h). The recycling endosome marker Rab11 did not colocalize with GFP-Rab9 (Fig. 3i). Collectively, these results suggest that Rab9 is involved in the trafficking pathway from endosomes to the TGN.
Vps35 regulates Serp-dependent tracheal tube-length control
The results described above are consistent with a model in which Rab9 has a role in the recycling of Serp from endosomes to the TGN. To determine if the retromer complex is involved in this process, we first examined the tracheal tube phenotype in zygotic mutants of vps35 (core retromer component). vps3531 exhibited the long-tube phenotype (Fig. 4a) and reduced luminal Serp levels (Fig. 4f and Supplementary Fig. S3a,b). The luminal labelling of 2A12, chitin-binding probe (CBP) and Pio was unaffected (Supplementary Fig. S3a–d). This phenotype was identical to that observed in the rab9 mutants. In addition, a mild reduction in Crb expression was noted (Supplementary Fig. S3e,f), as previously described for maternal vps35 mutants30. A combination of the vps35 and rab9 mutants did not exacerbate the mutant phenotypes (Fig. 4c–e), suggesting that vps35 and rab9 act in the same genetic pathway.
Vps35 interacts with Rab9 in Drosophila S2 cells
As both Rab9 and Vps35 are required for Serp trafficking and may act in the same genetic pathway, we next examined whether Rab9 and Vps35 can physically interact each other. The purified GST-Rab9 were immobilized on glutathione-sepharose beads and conversed into guanosine diphosphate (GDP)- and guanosine triphosphate (GTP)-loaded forms. Then myc-Vps35 lysates from S2 cells was loaded onto the samples, and the detected results showed that both GTP- and GDP-loaded forms of GST-Rab9, but not GST pulled down myc-Vps35 (Fig. 4l), indicating that Rab9 physically interacts with Vps35. Similar interaction was observed with GST-Rab7.
Vps35 and Serp colocalize at late endosomal Rab9 domains
The binding of Rab9 with Vps35 prompted us to further examine their endosomal localization in S2 cell and the tracheal system. When Vps35-mRFP was coexpressed with GFP-Rab9 in S2 cells, the Vps35-mRFP signal was detected as small puncta localized to small endosomes and vacuolar endosomes labelled with GFP-Rab9 (Fig. 5a, yellow and white arrowhead). Moreover, the Vps35-mRFP signal coincided with the enrichment of GFP-Rab9 in the vacuolar endosomal membrane (Fig. 5c and white arrowheads in Fig. 5a), implying that the retrieval vesicles formed at these domains. In GFP-Rab9- and myc-DVps35-expressing tracheal cells, Vps35 also localized at the Rab9-labelling endosomal membrane (white arrowheads in the insets in Fig. 5e). Consistent with this finding, time-lapse observation of GFP-Rab9 revealed small vesicles budding off the Rab9 endosomes within 40–50 s (Fig. 5d and Supplementary Movie 1). Long tubular structures were often observed in GFP-Rab7 and RFP-Rab9 co-expressing endosomal membrane (yellow arrowheads in Fig. 5i). Knockdown of Vps35 compromised this phenotype (Fig. 5j), indicating that Vps35 is required for the tubular structure formation.
We next followed the vesicular movement of full-length Serp-GFP, and found that it was associated with the Rab9-positive endosomal membrane, and some of the Serp-GFP was concentrated at the Rab9-enriched domains (white arrowheads in Fig. 5f). Importantly, the Serp puncta colocalized with small GFP-Rab9 vesicles that were budding from larger endosomes (blue arrowheads in Fig. 5f).
Endosomal recruitment and sorting of Vps35
We next asked the role of Rab proteins in endosomal recruitment of Vps35. We observed the colocalization of GFP-Rab5 and RFP-Rab9 in tracheal cells (Fig. 3d). In S2 cells (Supplementary Fig. S4a), they colocalized in two populations. One is large vacuoles where localization of GFP-Rab5 was weaker compared with RFP-Rab9, or transient (Supplementary Fig. S4a–c, Supplementary Movie 2). The other is small vesicles with high GFP-Rab5 concentration (diameter <0.4 μm, Supplementary Fig. S4a–c). Decrease of Rab5 expression by RNA interference (RNAi) treatments reduced vacuolar population of RFP-Rab9 and dissociation of Vps35-mRFP from endosomal membrane (Supplementary Fig. S4d,e, see also similar results by expression of the GDP-locked from GFP-Rab5-S43N, Supplementary Fig. S4h,i), suggesting that Rab5 is essential for recruitment of Vps35 and maturation of Rab9 LE.
Downregulation of Rab9 expression using RNAi treatment caused dissociation of Vps35-mRFP puncta from vacuolar LEs (yellow arrowheads in Fig. 5h, compared with Fig. 5g). On the other hand, overexpression of a GDP-locked form GFP-Rab9-S26N caused Vps35-mRFP to spread on the entire vacuolar membrane (white arrowheads in Supplementary Fig. S4j). Given the result of Vps35 association with both GDP- and GTP-bound forms of Rab9 (Fig. 4l), it appears that GFP-Rab9-S26N recruits Vps35 to the endosomal membrane but failed to concentrate it to the membrane budding site.
Rab7 is known to recruit the retromer complex to LEs38,39. Downregulation of Rab7 prevented the accumulation of Vps35-mRFP in the budding structures (Supplementary Fig. S4k). Notably, Vps35-mRFP was often found inside endosomes (yellow arrowheads in Supplementary Fig. S4f, see also Supplementary Fig. S4k, showing a similar phenotype induced by a GDP-locked form GFP-Rab7-T22N), suggesting that the blockade of Rab7 activity resulted in the missorting of Vps35-mRFP into the endosomal lumen. Taken together, the results indicate that Rab5, Rab9 and Rab7 act sequentially during early to late endosomal maturation to recruit Vps35 to the endosomal-budding site (see Discussion).
Sorting of Serp into actin-rich endosomal-budding sites
Actin is vital for vesicles to bud off the endosome. We therefore wondered if actin constitutes a component of the vesicle-budding machinery for Serp retrieval. Phalloidin staining of S2 cells revealed intracellular puncta (Fig. 6a) that colocalized with Vps35-mRFP (Fig. 6a) and the budding structures on LEs labelled with GFP-Rab9 (Fig. 6b). The colocalization of actin at the GFP-Rab9-labelled endosomal-budding sites was also observed in tracheal cells at stages 15 and 16 (blue arrowheads in Fig. 6c). Triple labelling with GFP-Rab9, Vps35-mRFP and phalloidin confirmed that they all colocalized at the endosomal-budding site (white arrowheads in Fig. 6e). Importantly, the cargo Serp was also colocalized with the actin-enriched endosomal-budding site (Fig. 6f). These results led us to investigate the actin dynamics in the endosome membrane. We co-transfected S2 cells with actin filament marker lifeact-mEGFP, and RFP-Rab9, and observed that endosomal budding occurred at actin patches on the RFP-Rab9 endosomes (Supplementary Movie 3, Fig. 6g magenta and green arrowheads). Strikingly, actin appeared before formation of the budding vesicles (compare the green arrowheads with magenta ones in Fig. 6g), suggesting that the recruitment of actin is a prerequisite for vesicle budding. GDP form of Rab7 (Fig. 6h) and Rab9 (Fig. 6i) did not impair the localization of actin puntca at the endosomal membrane, indicating that recruitment of actin patches is Rab7 and Rab9 independent. Taken together, these data indicate that Serp-containing vesicles leave the LEs using an actin-involved budding machinery.
WASH is essential for endosome abscission and Serp recycling
WASH is a newly identified actin nucleation-promoting factor acting through its Arp2/3-interacting VCA domain (Verprolin homology, cofilin homology and acidic domain)40, having a critical role for endosomal vesicle budding in vitro27,28. To determine whether WASH is involved in Rab9 vesicle-budding process, we first showed that WASH expressed in the tracheal cells and colocalized with intracellular actin puncta labelled by lifeact-mEGFP (Fig. 7a). Then, we stained GFP-Rab9-expressing tracheal cells with WASH, and found that most of WASH puncta was localized at the Rab9 endosomal membrane (90%, n=8 cells Fig. 7b). Double staining of WASH and Serp showed that WASH partly colocalized with intracellular Serp granules, which was contained inside Rab9 endosomes (Fig. 7c). WASH localized more proximal (Fig. 7d) than Vps35-mRFP (Fig. 5b) at the Rab9-enriched endosomal membrane. Actin patch was adjacent to WASH (Fig. 7e) and localized to the proximal part of Vps35-mRFP (Fig. 6e). To probe the function of WASH, we generated full-length and VCA domain-deleted dominant-negative27 forms of GFP-WASH constructs, and transfected them into S2 cells with RFP-Rab9. The results showed that GFP-WASH formed puncta structures and localized at Rab9 endosomal membrane (white arrowheads in Fig. 7f). GFP-WASH-ΔVCA can also localize on the endosomal membrane. However, long tubular structures were ectopically formed on endosomal membranes (white arrowheads in Fig. 7g). In rab9 and vps35 mutant embryos, Association of WASH with Serp granules remained (white arrowheads in Fig. 7h), indicating that the association of WASH and actin with cargo is independent of Rab9 and Vps35. In washΔ185-mutant40 embryos, DT length was significantly longer than the control (Fig. 7j–l), and the luminal Serp level was reduced at stage 15 and later, phenocopying the Rab9- and Vps35-mutant phenotypes (white arrowheads in Fig. 7m). The data collectively indicate that WASH, actin and Vps35 orderly localize to the budding site of Rab9 endosomal membrane, and constitute the major components of endosomal retrieval of Serp for recycling (Fig. 7o).
Discussion
Maturation of the tracheal tube involves diameter expansion triggered by a cell-intrinsic programme of luminal material secretion and apical membrane growth6,7, and the tube’s longitudinal growth is negatively regulated by the presumed conversion of chitin to chitosan through deacetylation by chitin deacetylase15. Each step involves temporally regulated apical secretion, but the regulatory mechanism underlying this selective cargo secretion has not been understood. In this study, we identified Serp as a novel cargo for the Rab9-mediated retrograde recycling pathway. Using time-lapse imaging, we demonstrated that Serp in the endocytic compartment is sorted out by the budding of actin- and WASH-enriched portions of the LEs. The similarity of the Rab9, Vps35, WASH and Serp tracheal tube-length phenotypes, and the colocalization of those in the Serp-containing endosomal-budding sites in S2 cells, suggest that Serp is one of the major cargoes of the retrograde trafficking mediated by Rab9, Vps35 and WASH (Fig. 7p). We also found that association of WASH and actin filaments with retrograde cargo is Rab9 and Vps35 independent. Modular organization of machineries for cargo retrieval (retromer) and membrane remodelling (WASH) may allow flexibility in endosomal sorting systems. Our work connects retrograde trafficking to luminal retention of the key rate-limiting protein required to restrict the tracheal tube length to the proper level15,16 and has identified a new regulatory process for tracheal tube size.
Previous works in mammalian cells revealed that recruitment of the cargo recognition subcomplex of retromer (Vps35, Vps29 and Vps26) to the endosomal membrane requires Rab5 and Rab7 (refs 38,39). Rab7 has been shown to bind directly to Vps35/29/26 complex38, but no evidence is available for association of Rab5 or Rab9 with those components38,39. Our analysis of the Drosophila counterparts have shown that conversion of early to LE is accompanied by gradual reduction of relative abundance of GFP-Rab5 to RFP-Rab9 signals (Supplementary Fig. S4). Throughout the process, Vps35-mRFP is present as distinct puncta associated with endosomes (yellow and white arrowheads in Fig. 5a). We propose the following order of Rab9-Vps35 assembly. In early endosome, Rab9 recruits Vps35 to the endosomal membrane through physical binding. This process requires Rab5. After initial recruitment of Vps35, endosomal maturation proceeds with exchange of Rab5 with Rab7, which promotes retromer assembly and cargo concentration, followed by membrane scission induced by WASH and F-actin. Together, our results indicate that Rab5, Rab9 and Rab7 acts on retromer assembly at different stages of endosomal maturation and tubular membrane formation, where Serp and other cargos are retrieved for retrograde pathway (Fig. 7o).
In contrast to the tracheal diameter expansion, which is triggered by a cell autonomous burst of exocytosis6,7, axial elongation is a slow and continuous process spanning stage 14–16. Therefore, any mechanism that restricts elongation is expected to be active throughout the elongation process. Previous studies showed that the two chitin deacetylases Serp and Verm act additively in tube length control15,16 and the overexpression of either one causes the same tube length defects16, indicating that the amount of luminal chitin deacetylase must be precisely maintained. Furthermore, the expression of Serp mRNA in the trachea declines at stage 16 (ref. 15), when luminal Serp protein is still abundant (Fig. 2b), implying that Serp synthesized in the previous stage must be effectively retained and reused. Here we have shown that Serp is endocytosed and associates with GFP-Rab9 (Fig. 2). The requirement for Rab9 and Vps35 for the luminal retention of Serp suggests that the endocytosed Serp is sorted from LEs to the TGN for secretion into the lumen, and this recycling pathway actively maintains the steady-state level of Serp to optimize the tube elongation process. Moreover, the retrieval transport through the TGN might help promote the modification of the endocytosed Serp, to recover its activity or to bind to an adaptor for its subsequent polarized secretion41.
In rab9, vps35 and wash mutants, Serp was mislocalized at the apical cortex of tracheal cells. This mislocalization may have been due to the trapping of Serp in endosomes marked with Rab7 or Rab11 which are apically localized in a Rab9-independent manner (Supplementary Fig. S2g–j). Consistent with this idea, a recent report showed that the suppression of Vps35 expression in NLT cells and neurons causes the accumulation of its cargo protein β-secretase (BACE1) in endosomes42. The second possibility is that the loss of Rab9 diverts the trafficking route of Serp from the endosomes to the cell surface, as observed in Rab9-deficient HeLa cells43. In support of this idea, we observed an enhancement of Serp accumulation at the surface of the epidermis in rab9 mutants (yellow arrowheads in Supplementary Fig. S2k,l). The third possibility is that a defect in endocytosis arrested Serp at the apical membrane, because Vps35 has been shown to be involved in endocytosis in S2 cells44. Further analysis will be required to understand the diverse influences of retrograde trafficking on endosomal dynamics.
The apical localization of Crb depends on the retromer complex29,30, but it was unaffected in rab9 mutants (Supplementary Fig. S2). One possible explanation for this finding is that the alternative recycling pathway of Crb, which involves Rab1145, compensates for the defect in retrograde trafficking in rab9 mutants. Another possibility is that Crb-retromer and Serp-retromer complexes use different trafficking pathways distinguished by sorting nexins46,47, which organize endosomal membranes into distinct morphological and functional regions for transport to diverse destinations47,48,49. Further study of the different sorting nexins should uncover the role of Rab9 in retromer cargo specificity.
The Dia and motor protein Myosin V were shown to be required for the secretion of a number of markers, including 2A12 antigen, Pio and artificial ANF-GFP, into the tracheal lumen8. On the other hand, the secretion of Serp and Verm and the cell-surface localization of Crb are normal in Dia mutants, indicating that a Dia-independent secretory pathway regulates these protein localizations in the trachea8. The spectrum of secreted protein localizations affected in the rab9 and vps35 mutants was nearly complementary to that of Dia, suggesting that the Dia-dependent and retrograde trafficking-dependent mechanisms are the two major apical secretory pathways in the trachea (Fig. 7p). Verm localization was not affected in the rab9 and vps35 mutants, suggesting that this putative chitin deacetylase behaves differently from Serp50. The difference in cargo specificity for each pathway allows cells versatility in controlling the localization of different proteins according to distinct schedules, so that the secretory burst that triggers tube diameter expansion and the continuous recycling of chitin deacetylases in axial elongation are controlled separately. Our results provide a molecular basis for the roles of distinct trafficking pathways in controlling tubule growth and geometry.
Methods
Fly strains and genetics
rab9 deletion mutations were generated using Minos transposon imprecise excision37. Three lethal deletions (rab956, rab9199 and rab9366) were identified from 540 progenies. The region of each mutant encompassing the deletion was PCR amplified using genomic DNA from homozygous mutant embryos with the following primer pairs:
rab956, forward (f): 5′-CTGATGTTTAAGGCTAGTGCCTGC-3′, reverse (r): 5′-TGCAAGACTCAAAAACGTGTC-3′; rab9199, f: 5′-CCAATCGCTACGAGGAGAACAAC-3′, r: 5′-GAGCATCATTCCACGCTGTGTG-3′; and rab9366, f: 5′-TGAATGCGAGTGTTGACCTTGC-3′, r: 5′-CAATAGCGAAATCTGCCGAACCC-3′
The PCR products were subcloned into the pBluescript II KS vector for sequencing. rab956, rab9199, rab956/rab9199 and rab9366 showed similar tracheal tube length phenotypes; dvps351 was a kind gift from Xinhua Lin31; the vps35 rab9 double mutant was generated by crossing recombination. vps351 rab956, vps351 rab9199 and vps351 rab9366 showed similar tracheal tube-length phenotypes. Other strains used in this study included: washΔ185, UAS-GFP-Rab5, UAS-YFP-Rab7, UAS-GFP-KDEL, UAS-GFP-LAMP1, Df(2L)Exel8041, Mi{ET1}Rab9MB05612 and snaSco/SM6a P{hslLMiT}2.4 (all from the Bloomington Stock Center), UAS–galactosyltransferase (GalT)-CFP (a kind gift from Akiko Satoh, Hiroshima University), UAS-myc-Dvps35 (kindly provided by Xinhua Lin31) and UAS-Serp-CBD-GFP (generously provided by Stefan Luschnig15). btl-GAL4 was used to drive the expression of UAS transgenes in the tracheal system.
Molecular biology
Full-length rab9 cDNA was amplified using the primers Rab9-EcoRI (5′-GGGAATTCGATGACGAACATGCGGCCGCC-3′) and Rab9-BglII (5′-CCACCAATTATCGGCTATGAAGATCTCCC-3′). The PCR product was purified, digested and ligated to the C-terminus of EGFP (GFP) or tagRFP (RFP) and inserted into the pUAST vector to generate the pUAST-GFP-Rab9 and pUAST-RFP-Rab9 transgenes. pUAST-GFP-Rab9-S26N was generated by a point mutant kit (QuickChange). Full-length (1–499 aa) and truncated (1–394 aa, VCA domain deleted) WASH was amplified using a common 5′-terminal primer WASH5EcoRI (5′-TACAGAATTCGATGGAGGAGTCACCTTACCTGCACA-3′) and two 3′-terminal primers WASH3NotI (5′-TACAGCGGCCGCCTAGTTCCACCCATCCTCGTCGT-3′) and WASHΔVCA3NotI (5′-TACAGCGGCCGCCTACTCAGATCGCGGATCTTCAGTAGC-3′). The purified PCR products were ligased into pUAST-EGFP-C vector to make pUAST-EGFP-WASH and pUAST-EGFP-WASHΔVCA constructs, respectively. pUAST-lifeact-mEGFP was constructed by the amplification of Lifeact-mEGFP from a previously described Gateway expression plasmid51 using Lifeact-XhoI (5′-CCGCTCGAGCAACATGGGTGTCGCAGATTTGATCAAG-3′) and Lifeact-mEGFP-XbaI (5′-GCTCTAGATTACTTGTACAGCTCGTCCATGCC-3′), and the insertion of the digested product into the pUSATattB vector. All the constructs were confirmed by DNA sequencing. Transgenic strains were established by DNA microinjection. The pUAST-Serp-GFP plasmid was provided by Stefan Luschnig15; pUASp-GFP-Rab7, pUASp-GFP-Rab7-T22N and pUASp-GFP-Rab5 were kindly given by Tsubasa Tanaka and Akira Nakamura52; UAS-myc-Dvps35 was a gift from Xinhua Lin31 and pMT-blast-Vps35-mRFP was a kind gift from Cahir J O’Kane44.
RNAi-induced gene knockdown
Purified dsRNA products of Rab5, Rab7, Rab9, Vps35 and LacZ (control) were prepared according to the protocol previously described53. The primers used in the experiments were
Rab5fw: 5′-TAATACGACTCACTATAGGGCGGTACCACAGCTTAGCTCC-3′
Rab5res: 5′-TAATACGACTCACTATAGGGGTTCGTCGGTCGATTTGTTT-3′
Rab7fw: 5′-TAATACGACTCACTATAGGGTTCCTCATACAGGCCAGTCC-3′
Rab7res: 5′-TAATACGACTCACTATAGGGGACAGTTGTCAGGATTGCCA-3′
Rab9fw: 5′-TAATACGACTCACTATAGGGGCGATTCCGGGCTCTACGCACCCCG-3′
Rab9res: 5′-TAATACGACTCACTATAGGGTCGGCCACGCACTCCATGTGCC-3′
Vps35fw: 5′-TAATACGACTCACTATAGGGGGCAAAGGCTAAAGCATGTCCTA-3′
Vps35res: 5′-TAATACGACTCACTATAGGGCTTTCCACTCCAGAAAAGCGC-3′
LacZfw: 5′-TAATACGACTCACTATAGGGGCATAAACCGACTACACAAATCAG-3′
LacZres: 5′-TAATACGACTCACTATAGGGGGCTTCATCCACCACATACA-3′.
A total of 15 μg dsRNAs were added into 1 ml serum-free culture media for 45 min, then 2 ml normal S2 cell culture media containing serum was added into the wells and culture at 25 °C. After 72 h, the half cells were fixed for observation, another half was used for reverse transcription PCR to monitor the gene expression. Total RNA was prepared by using RNeasy mini kit (Qiagen) and RNase-Free DNase Set (Qiagen). Reverse transcription and PCR amplification were performed using SuperScript one-step reverse transcription PCR (Invitrogen). rp49 was chosen as internal control and the primers were as following: rp49_F: 5′-ATGACCATCCGCCCAGCATACAGG-3′ and rp49_R: 5′-TCGTTCTTCTTGAGACGCAGGCGA-3′.
Cell culture, transfection and immunostaining
Drosophila Schneider cells (S2 cells) were cultured in Schneider’s Insect Medium (Gibco) supplemented with 10% fetal calf serum and antibiotics at 25 °C. pUAS-vectors were co-transfected with actin5c-GAL4 drivers using Effectene (Qiagen) according to the manufacturer’s instructions. The expression of pMT-Vps35-mRFP was induced with 1 mM CuSO4 overnight. After 24–48 h, the transfected cells were fixed and immunostained following previously described procedures54.
GST pull-down experiment
pGEX, pGEX-Rab7 (gift from Akira Nakamura) and pGEX-Rab9 were expressed in Escherichia coli BL21, and protein expression was induced with 0.1 mM IPTG for 16 h at 20 °C. GST-Rab recombinant proteins were purified by glutathione-sepharose 4B beads (Amersham). GST and GST-Rab proteins were immobilized on glutathione-sepharose 4B beads, then loaded with GDP or GTPγS following the previously described procedures55. UAS-myc-Vps35 was expressed in S2 cells for 48 h. The cells were collected and lysed in buffer containing 50 mM Tris–HCl, pH7.5, 150 mM NaCl, 5 mM MgCl2 and 0.5% NP-40 for 30 min at 4 °C. Lysates were centrifuged and the supernatant was incubated with GST and GDP- or GTPγS-loaded GST and GST-Rabs for 2 h at 4 °C. The samples were subsequently washed five times with lysis buffer and eluted using SDS sample buffer and analysed by SDS–PAGE, immunoblotted with Mouse monoclonal anti-myc-HRP-DirecT and detected with ECL prime western blotting detection reagent (GE Healthcare).
In situ hybridization
Full-length rab9 cDNA was cloned into the pBluescript II KS vector and then digested with XhoI or EcoRI to create the template for in vitro transcription using T7 and T3, respectively, to produce sense and antisense probes for hybridization. Whole-mount wild-type and rab9-mutant embryos collected 14–15 h after egg laying at 25 °C were fixed using 4% paraformaldehyde in PBS. rab9-mutant homozygous embryos were collected from rab956, rab9199 or rab9366 balanced over the Cyo-Dfd-YFP fly. In situ hybridization was conducted using digoxigenin (DIG)-labelled sense and antisense probes, according to a standard protocol56.
Immunofluorescence staining and western blotting
The primary antibodies used in this study were: mAb directed against Crb protein (1:40) (Developmental Studies Hybridoma Bank (DSHB)); mAb 2A12 antigen (1:2) (DSHB); rabbit anti-Pio (1:100), a gift from Markus Affolter57; rabbit anti-Serp (1:300 and 1:1,000 for immunofluorescence and western blotting, respectively) and rabbit anti-Verm (1:300) generously provided by Stefan Luschnig15; guinea pig anti-Uninflatible (1:500) was a gift from Robert E Ward58; rabbit anti-Rab11 (1:8,000) and rabbit anti-Rab7 (1:3,000) were a kind gift from Tsubasa Tanaka and Akira Nakamura52; CBP (1:200); phalloidin (1:100); WASH (1:50)59 (DSHB); alpha-tubulin (DM1A) (1:8,000 for western blotting); and mouse monoclonal anti-Myc-HRP DirecT (1:5,000 for western blotting) (MBL). We were not able to obtain anti-Rab9 antibody that can be used for tissue staining, despite repeated attempts in raising polyclonal antibodies in mice and guinea pigs. For western blotting, 20 embryos were homogenized in loading buffer and heated for 10 min at 95 °C. The samples were loaded on 10% polyacrylamide gels for SDS-PAGE, and the proteins were transferred to polyvinylidene difluoride membranes. Immunoblotting and the detection of HRP-conjugated second antibodies with an ECL detection kit (GE Healthcare) were performed according to the manufacturer’s instructions.
Morphometric analysis and statistics
The DT was analysed in fixed stage-16 embryos (n=6–9) using CBP staining. The DT length and diameter were determined with ImageJ (NIH, http://rsbweb.nih.gov/ij/). The DT length was measured from the anterior in tracheal segment 1 to the junction of the DT and transverse connective in tracheal segment 10. The DT diameter measurements were performed on maximal projections of Z stacks. For each embryo, the DT diameter was determined as the average value of three independent measurements taken in the central region of tracheal segment 7. The DT length and diameter were expressed as the mean plus standard deviation (SD) Student’s two-sided unpaired t-test with equal variance was used to assess the statistical significance.
Author contributions
B.D., K.K. and S.H. perceived the project. K.K. created Rab9 fluorescent plasmids and fly strains. H.W. performed microinjection and dye injection experiments. B.D. performed rest of the experiments with help from T.O. on biochemical assay. B.D. and S.H. wrote the manuscript.
Additional information
How to cite this article: Dong, B. et al. Rab9 and retromer regulate retrograde trafficking of luminal protein required for epithelial tube-length control. Nat. Commun. 4:1358 doi: 10.1038/ncomms2347 (2013).
Supplementary Material
Acknowledgments
We thank S. Luschnig, C.J. O’Kane, X.H. Lin, M. Affolter, T. Tanaka, A. Nakamura, R.E. Ward, A. Satoh, the Bloomington Stock Center and the Developmental Studies Hybridoma Bank (DSHB) for generously providing antibodies, constructs and fly stocks; and K. Kato for image analysis; T. Nishimura and G. Sheng for critical reading of the manuscript; and members of Hayashi group for their discussion and valuable comments. This work was supported by a Grant-in-Aid for Scientific Research on Innovative Areas from MEXT Japan to S.H. and the RIKEN Foreign Postdoctoral Researcher programme to B.D.
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