1 Program in Cellular Biotechnology, University of Helsinki, Viikinkaari 9, 00710 Helsinki, Finland
2 Electron Microscopy Unit, Institute of Biotechnology, University of Helsinki, Viikinkaari 9, 00710 Helsinki, Finland
3 Department of Applied Chemistry and Microbiology, University of Helsinki, Viikinkaari 9, 00710 Helsinki, Finland
Author for correspondence (e-mail: marja.makarow{at}helsinki.fi)
Accepted 27 November 2003
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Summary |
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Key words: Hsp150, COPI, Yeast, Secretion, Membrane traffic
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Introduction |
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Sec24p has two homologs, Sfb2p (Iss1p/Sec24B) and Sfb3p (Lst1p/Sec24C), which have 56% and 23% identity with Sec24p, respectively (Kurihara et al., 2000; Roberg et al., 1999
). All homologs have been shown to serve as COPII components and operate in ER exit. Sec24p is essential, whereas deletion of either of the homologs individually or in combination does not compromise exocytic membrane traffic or viability (Pagano et al., 1999
). However, overexpression of Sfb2p rescued viability of cells lacking the SEC24 gene, and allowed intracellular transport of several cargo proteins, showing that Sfb2p can compensate for Sec24p in COPII coats (Kurihara et al., 2000
). Overexpression of Sfb3p could not complement the lack of SEC24, but Sfb3p could replace Sec24p in in vitro ER budding assays (Miller et al., 2002
). Deletion of SFB3 from sec24 mutants is lethal, but that of SFB2 is not (Roberg et al., 1999
; Peng et al., 2000
).
Here we show that Sec24p was not required for ER exit of Hsp150 in living yeast cells. Hsp150 was secreted to the medium in the absence of normal Sec24p function, albeit slowly. The signature on Hsp150 for selection to the Sec24p-independent ER exit route resided in the C-terminal domain of 114 amino acids. The determinant was an active mediator of ER exit occurring independently of Sec24p function. The C-terminal domain recruited Hsp150 specifically to ER exit sites lacking functional Sec24p, because it was completely dispensable for secretion in cells with wild-type Sec24p. Nonfunctional Sec24p was not compensated by the homolog Sfb2p in ER exit of Hsp150.
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Materials and Methods |
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Electron microscopy
Cells were fixed by adding an equal volume of 6% formaldehyde plus 1% of glutaraldehyde in 0.2 M sodium citrate, pH 4.8, to the growth medium for a 2 hour incubation at 37°C, followed by an overnight incubation at 4°C in 3% formaldehyde in 0.1 M sodium citrate. The cell wall was weakened by digestion with zymolyase (25 U/ml; Seikagaku, Japan) in TPC buffer (10 mM Tris-HCl, 10 mM CaCl2 and 1.2 M sorbitol) for 15 minutes at room temperature. A DAB treatment was adapted from Brown and Farquhar (Brown and Farquhar, 1989) as follows. The cells were washed three times for 5 minutes in 50 mM Tris-HCl buffer, pH 7.6, and incubated then for 10 minutes in the dark in 0.15% DAB/Tris-HCl buffer, and then for 30 minutes in 0.15% DAB/Tris-HCl containing 0.063% hydrogen peroxide. After three washes with Tris-HCl buffer and another three washes with distilled water, the cells were treated with 1% OsO4/1.5% K4Fe(CN)6 for 1 hour at 4°C. The cells were washed with water, and left overnight in water. The cell pellets were then dehydrated in an increasing gradient of ethanol, 3x20 minutes in 70%, 3x20 minutes in 94% and 3x20 minutes in 99.5% ethanol, followed by an overnight incubation in the last. The cells were finally embedded in Spurr resin (Agar Scientific, UK) as follows: 1 hour in 50% and then 1 hour in 67% Spurr in ethanol, and finally 14 hours in 100% Spurr. Polymerization was at 60°C. Sections were cut and picked on single-slot copper grids, post-stained with uranyl acetate and lead citrate, using the Leica EMSTAIN device. Sections were examined with an FEI Tecnai12 transmission electron microscope at 80 kV. Formaldehyde, glutaraldehyde and osmium tetroxide (OsO4) were obtained from Electronic Microscopic Sciences (Washington, PA); diaminobenzidine (DAB) was from TAAB Laboratories Equipment, UK. All reagents were EM grade.
Other methods
Metabolic labeling with 35S-methionine/cysteine (1000 Ci/mmol; Amersham International, Buckinghamshire, UK) and immunoprecipitation with antisera against Hsp150 (1:400), ß-lactamase (1:100), CPY (1:100) and HRP (1:200, RDI), and SDS-PAGE (8% gels) were as described previously (Paunola et al., 1998). Internal and cell wall activities of invertase were determined as described in Simonen et al. (Simonen et al., 1994
). Activity staining of invertase in nondenaturing gels was according to Novick et al. (Novick et al., 1980
). Endoglycosidase H (Boehringer, Mannheim, Germany) digestion (20 mU/50 µl of 80 mM sodium acetate buffer, pH 5.2) was performed for 4 hours at 37°C on immunoprecipitated substrate protein adhering to protein A-Sepharose beads. Trichloroacetic acid (TCA) precipitation was performed with 10% acid, followed by washing of the precipitate with ice-cold acetone.
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Results |
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We used pro-CPY and invertase as internal controls for nonfunctional Sec24p in the above experiment; both are shown to require all structural components of the COPII coat for ER exit (Novick et al., 1980; Stevens et al., 1982
). In the same sec24-1 cells where Hsp150 continued to be slowly secreted at restrictive temperature, newly synthesized vacuolar CPY remained in the ER-specific p1 form (Fig. 2B, lanes 1-4), indicating that it could not leave the ER (Stevens et al., 1982
), whereas at permissive temperature 24°C pro-CPY was rapidly converted via the Golgi form p2, to the mature vacuolar form (Fig. 2B, lanes 5-8). When the sec24-1 mutant was preincubated for 15 minutes at 38°C and then derepressed for invertase synthesis in low glucose medium at the same temperature, electrophoresis under nondenaturing conditions and activity staining revealed molecules (Fig. 2C, lane 3) that comigrated with the ER form accumulating in the ER in the sec18-1 mutant (lane 2). When invertase was synthesized at 24°C in the sec24-1 mutant (lane 4), it comigrated with mature invertase with extended N-glycans expressed in control cells (lane 1). In this experiment 38°C was used as restrictive temperature, but similar results were obtained at 37°C. Our data show that Hsp150 was secreted to the culture medium under conditions in which the COPII component Sec24p was nonfunctional to an extent that it prevented pro-CPY and invertase from leaving the ER.
Mapping of the domain responsible for ER exit of Hsp150 in the absence of normal Sec24p function
We showed previously that the C-terminal domain of Hsp150 (see Fig. 1A) was slowly secreted to the medium in the absence of normal Sec13p function (Fatal et al., 2002). This data provided us with a starting point to map the fragment guiding Hsp150 to the ER exit pathway that does not require normal Sec24p function. Subunit I of Hsp150, flanked by an authentic C-terminal recognition site for Kex2p located in the late Golgi (Wilcox et al., 1992
), was joined directly to the N-terminus of the C-terminal domain of Hsp150, creating SUI-Cterm (see Fig. 1C). Cells expressing SUI-Cterm were preincubated for 15 minutes, pulse-labeled for 5 minutes and chased up to 1 hour at 37°C, followed by immunoprecipitation of cell lysates and respective media samples, and SDS-PAGE analysis. In the case of control cells, very little if any SUI-Cterm could be detected in the lysates (Fig. 3C, lanes 1-4). After the 5-minute pulse, very little protein was detected in the medium (Fig. 3C, lane 5), but after 15-60 minutes of chase, proteins of 16.5 and 14 kDa could be immunoprecipitated from the medium (lanes 6-8). Apparently, SUI-Cterm was difficult to detect from the lysate after the pulse because of heterogeneity in glycosylation, which resulted in heterogeneity in electrophoretic migration. The 14 and 16.5 kDa bands represent the C-terminal fragment, released from subunit I by Kex2p. The two forms apparently arose from different degrees of processing of the C-terminus by other peptidases after the Kex2p cleavage. In the control cells, secretion of the C-terminal fragment to the medium was completed within 15 minutes of chase. In the sec24-1 mutant, uncleaved SUI-Cterm could be detected after the pulse in the lysate (Fig. 3A, lane 1). Thereafter, the fusion protein disappeared from the cells (lanes 2-4), and the released C-terminal fragment appeared in the medium (lanes 5-8). An apparently maximal amount of Cterm was in the medium in 30 minutes. For comparison, we show a similar experiment performed on sec13-1 cells. In this case, more of the intracellular uncleaved form was detected (Fig. 3B, lanes 1-4), and some uncleaved form appeared also in the medium (lanes 5-8). The secretion of released Cterm in sec24-1 cells (H1500) was also compared at permissive and restrictive temperature. Similar relative amounts of Cterm could be detected in the medium after a 30-minute chase both at 37°C and 24°C (data not shown).
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A construction in which the C-terminal fragment was replaced by ß-lactamase (SUI-ß-lactamase, Fig. 1D) served as a control to confirm that it was the C-terminal fragment rather than subunit I that was responsible for ER exit in the absence of normal Sec24p function. A similar pulse-chase experiment as above showed that SUI-ß-lactamase remained intracellular at 37°C in a sec24-1 background, and comigrated in SDS-PAGE with the form retained in the ER in a sec18-1 mutant (not shown). We conclude that the C-terminal fragment harbored a signature recruiting Hsp150 to the Sec24p-independent ER exit pathway.
If the C-terminal domain in full-length Hsp150 is alone responsible for ER exit in the absence of normal Sec24p function, the remainder of the protein, Hsp150 (see Fig. 1B), should remain in the ER in the absence of Sec24p function. We showed that this indeed is the case. Pulse-chase experiments on sec24-1 cells lacking the endogenous HSP150 gene detected an intracellular form of about 90 kDa after pulse at 37°C (Fig. 4, lane 1). Its electrophoretic migration slowed down to correspond to 170 kDa during the chase (lanes 3, 5 and 7), whereas no protein could be detected in the media samples (lanes 2, 4, 6 and 8). The intracellular form detected after 60 minutes of chase (lane 7) comigrated with the ER form detected at 37°C in a sec18-1 mutant (lane 21). At 24°C, the mature form of Hsp150
migrating like a protein of more than 200 kDa appeared in the medium by 15 minutes of chase (lanes 9-16). Mature Hsp150
, as well as its biosynthetic intermediates, migrate anomalously slowly in SDS-PAGE, probably because of extensive O-glycosylation, as described previously (Jämsä et al., 1995
). In control cells, similar amounts of the mature form were in the media samples after 60 minutes of chase both at 24°C (lane 18) and 37°C (lane 20), whereas no intracellular forms could be detected at either temperature (lanes 17 and 19). This data shows that the C-terminal domain is dispensable for ER exit in the presence of normal Sec24p. Thus, the C-terminal domain appears to recruit authentic Hsp150 specifically to ER exit sites that lack functional Sec24p.
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Electron microscopic localization of Hsp150-HRP
Next we sought for morphological evidence that an Hsp150 variant lacking the C-terminal domain is retained in the ER in the absence of Sec24p function. To this end, the C-terminal portion was exchanged to horseradish peroxidase (HRP; see Fig. 1E). The chimera was expressed in sec mutants under the HSP150 promoter, which drives a basal level of expression at 24°C, and is upregulated at 37°C (Russo et al., 1993). The fusion protein migrating in SDS-PAGE like a 170 kDa protein was recognized by antisera against Hsp150 and HRP in western blotting and immunoprecipitation experiments (not shown). For EM, the cells were incubated for 1 hour at 37°C to impose the secretion block, fixed and processed as described in Materials and Methods. Fig. 5A shows in sec24-1 cells membranous structures, reminiscent of ER membrane, containing HRP reaction product (large black arrows), as well as unstained membrane (large open arrow). A sec23-1 mutant served as a control for ER. Stained ER membrane close to the plasma membrane and in the cytosol (Fig. 5C, large black arrows), as well as stained nuclear envelope (small arrows), were observed. The plasma membrane appeared not to be stained, at least not uniformly. The cell wall contained some reaction product, which was apparently due to the basal expression of secretory Hsp150
-HRP at 24°C before shift to 37°C. Endogenous peroxidases were responsible for reaction product in the vacuoles. For reference we show the Golgi-specific sec7-1 mutant (Fig. 5D), where multiple stained cisternae were detected (large black large), whereas the nuclear envelope was unstained (small arrow). In the absence of the HSP150
-HRP gene, no deposit was observed, except for the vacuole harboring endogenous peroxidases (Fig. 5B).
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The C-terminal domain of Hsp150 harbors an active signal recruiting invertase for Sec24p-independent ER exit
Next we studied whether the C-terminal fragment of Hsp150 was able to recruit invertase to the Sec24p-independent ER exit pathway. Invertase was used as cargo, as in authentic form it requires functional Sec24p for ER exit. Invertase was fused to the C-terminus of subunit I, and the C-terminal Hsp150 domain was joined to the C-terminus of invertase, creating SUI-invertase-Cterm (see Fig. 1F). A Kex2p recognition site joined subunit I to invertase. Cleavage at the Kex2p site would indicate that the fusion protein had exited the ER and reached at least the late Golgi, where the Kex2 protease resides. The chimera was placed under the control of the HSP150 promoter. Thus, in full glucose (2%) medium, at either temperature, invertase activity would be due only to the recombinant gene, and not to endogenous invertase expressed only in low (0.1%) glucose medium.
The invertase portion acquired a catalytically active conformation and the fusion protein acquired a transport-competent form, because high levels of invertase activity were detected in control (H1577), sec24-1 (H1579), sec13-1 (H1578) and sec18-1 (H1575) cells after growth at 24°C in full glucose medium. At least 75% of the total activity was in the cell wall and the rest was in spheroplast lysates in each strain, with no activity in the medium (data not shown). Immunoprecipitation of 35S-labeled control cell lysates, followed by endoglycosidase H digestion to remove the heterogenous N-glycans of the invertase portion, revealed in SDS-PAGE analysis a protein migrating at 73 kDa (Fig. 6A, lane 4). In a sec18-1 mutant, labeled at 37°C, a protein migrating at 81 kDa was detected (lane 6). The difference in electrophoretic migration, 9 kDa, corresponds to the 54 amino acid O-glycosylated subunit I. Thus, we expect that the 81 kDa form was SUI-invertase-Cterm, retained in the pre-Golgi in the sec18-1 mutant, whereas in control cells subunit I had been removed by Kex2p in the late Golgi, resulting in invertase-Cterm. In sec24-1 cells both forms were detected (lane 5). When the same experiment was performed for reference in sec13-1 cells, similar results were obtained (lane 7). We suggest that in the sec24-1 and sec13-1 mutants about half of SUI-invertase-Cterm had left the ER at 37°C during a 40-minute chase, and reached at least the late Golgi. Similar results were obtained when the C-terminal fragment was placed to the N-terminus of invertase (SUI-Cterm-invertase, Fig. 1G), as shown in Fig. 6A, lanes 1-3. Parallel immunoprecipitations with CPY antiserum showed that CPY remained in the ER form in the three mutant strains (Fig. 6B, lanes 1, 3 and 4), but was converted to the mature form in the control cells (lane 2). We conclude that the C-terminal domain of Hsp150 served as an active mediator of ER exit for proteins, which in authentic form were dependent on functional Sec24p for recruitment to ER-derived COPII-coated vesicles.
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Role of Sec24p homologs in ER exit of Hsp150
Deletion of either of the SEC24 homologs, SFB2 or SFB3 alone or in combination from a normal cell (strains H1141-H1143, see Table 1), did not affect Hsp150 secretion (not shown). Hsp150 appeared in the culture medium with a half time of 5 minutes as described previously for normal cells (Jämsä et al., 1995; Fatal et al., 2002
). Disruption of the SFB3 gene from thermosensitive sec24 mutants is lethal (Roberg et al., 1999
; Peng et al., 2000
). Thus, we disrupted the SFB2 gene from the sec24-1 mutant. Pulse-chase experiments showed that Hsp150 was secreted to the medium at 37°C in this double mutant (Fig. 7B), with similar kinetics as in the sec24-1 mutant carrying a normal SFB2 gene (Fig. 7A). Thus, Sfb2p did not compensate for nonfunctional Sec24p in ER exit of Hsp150.
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Discussion |
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We showed recently that carrier vesicles can bud off the ER membrane and fuse with the Golgi membranes in the absence of normal Sec13p function, and that Hsp150 is able to leave the ER under these conditions. The signature required for selection to the Sec13p-independent ER exit pathway resided in the same C-terminal domain shown here to recruit Hsp150 for Sec24p-independent exit (Fatal et al., 2002). Whether these are in fact two different exit signatures within the C-terminal domain, each one specific for nonfunctional Sec13p and Sec24p, or a shared single signal, is not yet known.
Not only Sec24p, but also its homologs, Sfb2p and Sfb3p (Roberg et al., 1999; Pagano et al., 1999
; Kurihara et al., 2000
), function in ER exit. In cells lacking the SEC24 gene but overproducing Sfb2p, the soluble cargo molecules
-factor precursor and pro-CPY, and the membrane protein Gas1p, were shown to leave the ER. Purified Sfb2p/Sec23p complexes could replace Sec24p/Sec23p in vesicle budding in vitro, and the v-SNAREs (vesicular SNAP receptors) Bet1p and Sec22p could be identified in these vesicles (Kurihara et al., 2000
). Sfb3p could also compensate for Sec24p as COPII subunit in in vitro budding assays. However, such vesicles were deficient in SNAREs, suggesting that the Sec24 proteins function in cargo discrimination (Miller et al., 2002
). Sfb3p was already shown earlier to select a subset of cargo in vivo, and was suggested to function as a cargo-specific adaptor protein (Roberg et al., 1999
; Shimoni et al., 2000
). As shown here, the C-terminal domain of Hsp150 caused proteins to be selected specifically to ER exit sites lacking functional Sec24p under conditions where Sfb2p and Sfb3p were normal. Deletion of one or both Sec24p homologs did not inhibit the ER exit of Hsp150 when Sec24p was fully functional. Moreover, deletion studies showed that Sfb2p did not compensate for nonfunctional Sec24p in ER exit of Hsp150. Deletion of SFB3 is lethal in combination with mutations in any of the COPII genes SEC13/16/23/24/31 (Roberg et al., 1999
).
The exit of proteins from the yeast ER requires not only COPII traffic, but also ongoing retrograde traffic from the Golgi to the ER. The Golgi-derived vesicles are covered by the COPI coatomer consisting of seven different structural proteins (Hosobuchi et al., 1992). Retrograde transport has been suggested to return from the Golgi to the ER component(s), which are needed for forward traffic. Hsp150, as well as invertase and the C-tail anchored v-SNARE Sec22p, behave exceptionally, as they leave the ER in the absence of COPI traffic (Gaynor and Emr, 1997
; Ballensiefen et al., 1998
). The determinant selecting Hsp150 to the COPI-independent pathway was found to be in a region consisting mostly of a 19 amino acid peptide repeated 11 times in Hsp150 (see Fig. 1A) (Suntio et al., 1999
).
In summary, Hsp150 appears to have different determinants that drive ER exit. The repetitive region promotes ER exit in the absence of components that are normally returned from the Golgi to the ER by COPI traffic and required for the ER exit of many proteins. The determinant(s) in the C-terminal domain regulate ER exit in the absence of functional Sec24p or Sec13p. None of these determinants is required for ER exit of Hsp150 in cells, where all COPII components are available in functional form and COPI traffic operates. Thus, the different determinants guide soluble cargo proteins specifically and actively to ER exit sites covered with structurally and/or functionally different COPII coats. This suggests that in normal cells the ER gives rise to heterogeneous populations of vesicles, which are covered by different coat protein compositions, resulting in the recruitment of different sets of receptors, and consequently soluble cargo proteins, for intracellular transport.
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Acknowledgments |
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Footnotes |
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