Department of Biochemistry, Dartmouth Medical School, Hanover, New Hampshire 03755
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Abstract |
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COPII-coated ER-derived transport vesicles
from Saccharomyces cerevisiae contain a distinct set of
membrane-bound polypeptides. One of these polypeptides, termed Erv14p (ER-vesicle protein of 14 kD),
corresponds to an open reading frame on yeast chromosome VII that is predicted to encode an integral
membrane protein and shares sequence identity with
the Drosophila cornichon gene product. Experiments
with an epitope-tagged version of Erv14p indicate that
this protein localizes to the ER and is selectively packaged into COPII-coated vesicles. Haploid cells that lack
Erv14p are viable but display a modest defect in bud
site selection because a transmembrane secretory protein, Axl2p, is not efficiently delivered to the cell surface. Axl2p is required for selection of axial growth
sites and normally localizes to nascent bud tips or the mother bud neck. In erv14 strains, Axl2p accumulates
in the ER while other secretory proteins are transported at wild-type rates. We propose that Erv14p is required for the export of specific secretory cargo from
the ER. The polarity defect of erv14
yeast cells is reminiscent of cornichon mutants, in which egg chambers fail to establish proper asymmetry during early stages
of oogenesis. These results suggest an unforeseen conservation in mechanisms producing cell polarity shared
between yeast and Drosophila.
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Introduction |
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SECRETORY proteins destined for intracellular organelles or the plasma membrane are first synthesized and processed at the ER of eukaryotic cells.
Fully folded secretory proteins are then packaged into
ER-derived transport vesicles for export to the Golgi complex and beyond. Several lines of experimental evidence indicate mechanisms of protein retention and retrieval operate during ER-Golgi transport to maintain distinct organelle identity (Sato et al., 1996; Kaiser et al., 1997
). In
addition, secretory proteins that must move forward are
concentrated into ER-derived vesicles during export from
this compartment (Quinn et al., 1984
; Balch et al., 1994
;
Rexach et al., 1994
); however, the mechanisms of this selection procedure remain obscure. One component of this selective export process is a protein complex, termed
COPII, that forms ER-derived transport vesicles and selects secretory proteins by direct or indirect interaction
(Barlowe et al., 1994
; Kuehn et al., 1998
). In the yeast Saccharomyces cerevisiae, formation of ER-derived vesicles
has been reconstituted in a cell-free reaction with ER
membranes and purified COPII proteins (Salama et al., 1993
). We have proposed that additional components of
this selection machinery are contained on ER-derived vesicles, and we have undertaken a molecular analysis of
protein constituents on purified COPII-coated vesicles
(Belden and Barlowe, 1996
).
An uncoated form of ER-derived vesicles may be isolated after centrifugation on density gradients. These gradient-purified vesicles contain a set of tightly associated
polypeptides that are solubilized by detergents but not by
an elevated pH treatment. NH2-terminal polypeptide sequences have been determined from several of the abundant species contained on ER vesicles (Ervs),1 starting
with the lowest molecular weight species moving upward (Belden and Barlowe, 1996). In this report, we characterize Erv14p, an integral membrane protein that localizes to
the ER and Golgi compartments of yeast cells. Strains that
lack Erv14p (erv14
) are viable but display novel phenotypes in both haploid and diploid stages of growth. First,
haploid erv14
strains are defective in selecting the proper
bud site. Wild-type budding yeast are highly polarized
during vegetative growth, orienting cytoskeletal elements
and the secretory pathway toward the emerging bud tip (Drubin et al., 1991). Haploids select bud sites such that
mother and daughter cells bud toward each other and
therefore exhibit an "axial" budding pattern. Genetic
analyses in yeast have led to the identification of several
genes that are required for selection of axial growth sites
(Chant, 1996
). One of these gene products, Axl2p, is an integral membrane secretory protein that must be delivered
to the plasma membrane for establishment of the axial bud site (Halme et al., 1996
; Roemer et al., 1996
). In
erv14
strains, Axl2p is largely retained in the ER and the
yeast bud in a nonaxial manner. The accumulation of
Axl2p in the ER appears to be selective since other secretory proteins examined were transported at wild-type
rates. Second, diploid erv14
/erv14
strains display normal diploid budding patterns but do not sporulate when
deprived of nutrients. This sporulation defect does not appear to be related to transport of Axl2p and suggests that
Erv14p participates in the transport of additional secretory proteins.
Erv14p shares a high degree of amino acid identity
(36%) with the cornichon gene product from Drosophila
melanogaster. Mutations in the cornichon gene are known
to disrupt anterior-posterior pattern formation during
early stages of Drosophila oogenesis and ultimately lead
to misorientation of the oocyte cytoskeleton (Roth et al.,
1995). This phenotype is in some respects similar to the
erv14
phenotype. Therefore, experiments with the yeast homologue of cornichon may provide insight on the molecular mechanisms establishing polarity in the Drosophila
oocyte and perhaps in a variety of cell types.
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Materials and Methods |
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Yeast Strains and Media
The strains used in this study are listed in Table I. Cultures were grown in
either rich medium (1% Bacto-yeast extract, 2% Bacto-peptone, and 2%
dextrose [YPD]) or minimal medium (0.67% nitrogen base without amino
acids, 2% dextrose [YMD]) containing appropriate supplements. Cultures
were grown at 30°C unless indicated differently in figure legends. Standard yeast genetic methods used in these studies have been previously described (Sherman, 1991). Manipulation of recombinant DNA was performed as described (Ausubel et al., 1987
), and Escherichia coli strain
DH5
(Woodcock et al., 1989
) was used for these procedures.
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Plasmid Construction
The sequence of ERV14 and its upstream and downstream regions were
obtained from the yeast genome database for YGL054c (Feuermann et al.,
1997). ERV14 was isolated by PCR amplification of genomic DNA prepared from S. cerevisiae strain FY23 (Winston et al., 1995
) using the primers GP3 (5'-CGGAATTCCGGGGTTCGACTCCCCG-3') and GP4 (5'-CGGGATCCTATTTACCGATATTCACCGG-3'). The restriction sites
EcoRI and BamHI were used to subclone ERV14 (including 250 bp upstream and downstream of the open reading frame) into the EcoRI and
BamHI sites of pRS316 to produce pRS316-ERV14. This construct was
sequenced to confirm proper synthesis during amplification. An epitope
tag corresponding to the hemagglutinin (HA) peptide sequence YPYDVPDYA (Wilson et al., 1984
) was added on the COOH terminus of
Erv14p and was synthesized using the primers GP3 and JP11 (5'-TCCCCGCGGTTAAGCGTAGTCTGGGACGTCGTATGGGTAGAAGT- CATCACCACTTTCAGC-3 '). This primer anneals to the 3'-coding sequence of ERV14 and inserts the HA epitope followed by a stop codon
and a SacII restriction site. The resulting ~700-bp PCR product was treated with EcoRI and SacII and then ligated into the EcoRI/SacII site of
pRS316. The 3' untranslated region for ERV14 was restored by inserting
the 340-bp PCR product synthesized using the primers JP12 (5'-TCCCCGCGGTCCAACAAGACATTGAAATCC-3') and JP13 (5'-AGGCCGCGGATTTCACAGTCATGCTCACCC-3') into the SacII site. This
construct (pRS316-ERV14HA) was sequenced to confirm proper synthesis during amplification.
Strain Construction
The ERV14 locus was targeted for disruption with the HIS3 gene (Baudin
et al., 1993). A PCR method was used to amplify an erv14::HIS3 disruption fragment using the primers GP1 (5'-TGCAATTAAAGTAAAGTAAAAAAATTAAGAATAAAAAGAAAAGGCCTCCTCTAGTACACT-3') and GP2 (5'-CTTGGCCCTTCAGTCTTCTTTGGATTTC-
AATGTCTTGTTGGAGCGCGCCTCGTTCAGAATG-3') with pHISKO
as a template. The resulting product has the HIS3 gene flanked by 45 bp
of the ERV14 gene directly before the ATG start and directly after the
stop codon. Transformation of strain YPH501 (Sikorski and Heiter, 1989)
to histidine prototrophy and subsequent screening identified several isolates that were heterozygous at the ERV14 locus. Several of these heterozygous diploids were grown under conditions to induce sporulation,
and dissection of these asci produced four viable spores. A haploid disruptant (CBY251) was also constructed in strain FY834 and used in subsequent studies. Disruption of the ERV14 locus was confirmed by two independent PCR analyses. First, the GP3 primer and a primer internal to the HIS3 gene (5'-GCCTCATCCAAAGGCGC-3') generated a product (650 bp) of the expected size, and second, primers that flank the ERV14 gene
(GP3 and GP4) produced a single product (1,500 bp) of the expected size.
An Erv14p homologue that shares 63% amino acid identity is defined
by open reading frame YBR210w on chromosome II (Feldmann et al.,
1994), referred to here as ERV15, and was also targeted for disruption
with the TRP1 gene in a multistep procedure. The primers EF4 (5'-AATCTAGAGCTCACTACTACTCTCTC-3') and EF3 (5'-AAACTCGAGCAAATACGAGGGAGATCG-3'), which correspond to regions
that are ~210 bp upstream and ~300 bp downstream of the open reading
frame, were used to amplify ERV15 from genomic DNA. These primers
contain the restriction sites XbaI (EF4) and XhoI (EF3) to facilitate insertion into the homologous sites of pRS305 (Sikorski and Heiter, 1989). This
plasmid, pREF305, was modified to disrupt the open reading frame of
ERV15 with TRP1. A unique PstI site located 29 bases upstream of the ERV14 start codon and a partial digest of DraI (site is located 328 bp
downstream from the ATG start) were used to insert the TRP1 gene. A
PstI/SmaI digest of pJJ248 (Jones and Prakash, 1990
) liberates a 955-bp
fragment containing the TRP1 gene that was then inserted into pREF305
treated with PstI and DraI. The resulting plasmid, pEFT305, was digested
with NotI/XboI, and the 1.6-kbp fragment containing the TRP1 gene
flanked by ERV15 sequence was isolated. This disruption fragment was
used to transform strain FY833. Tryptophan prototrophs were screened
using the primers EF7, 5'-CTGAACGACAAAGTGAAGC-3' (anneals
404 bp downstream of the ERV15 stop codon) and JP7, 5'-TCACCTGTCCCACCTGC-3' (anneals 500 bp downstream from the TRP1 start
codon), which produce a 1.1-kbp amplification product if integration has
occurred at the ERV15 locus. One of these isolates, CBY347, was used in
subsequent experiments and was mated with CBY251 to generate the
double erv14::HIS3 erv15::TRP1 strain, CBY348. This strain was placed in
media to induce sporulation, and an isogenic set of strains containing the
single and double disruptions (CBY353, CBY354, CBY355, and CBY356)
were isolated for use in these studies. To prepare diploids homozygous for
erv14::HIS3, CBY356 was mated with CBY358, and zygotes were picked
by their distinctive morphology under the microscope.
Antibodies and Immunoblotting
Antibodies directed against Sec61p (Stirling et al., 1992), Sec22p
(Bednarek et al., 1995
), Erv25p (Belden and Barlowe, 1996
), Emp47p
(Schröder et al., 1995
), Sec23p (Hicke and Schekman, 1989
), Kar2p
(Brodsky and Schekman, 1993
), CPY (Rothblatt et al., 1989
), Gas1p
(Frankhauser and Conzelmann, 1991
), Vph1 (Kane et al., 1992
), and
plasma membrane ATPase (Carolyn Slayman, Yale University, New Haven, CT) were used in these studies. Anti-HA monoclonal antibody
(HA.11) raised against the peptide CYPYDVPDYASL was obtained from Berkeley Antibody Co. (Richmond, CA). Polyclonal antiserum specific for Sec12p was raised against the NH2-terminal domain of Sec12p
(amino acid residues 1-354) fused to protein A. Fusion protein was expressed from the plasmid pRIT33 (Nilsson and Abrahmsen, 1990
) and purified by IgG affinity chromatography as described by the manufacturer
(Pharmacia Biotech, Piscataway, NJ). Antigen (0.25 mg) was mixed with
Freund's complete adjuvant and injected into rabbits followed by monthly
boosts with 0.12 mg of antigen in Freund's incomplete adjuvant. Serum
isolated from immunized rabbits cross-reacted with a 70-kD species that
was overproduced when transformed with a GAL1-regulated version of
SEC12 (d'Enfert et al., 1991
). For immunoblots, proteins were resolved by
SDS-PAGE (Laemmli, 1970
) and transferred to nitrocellulose (Towbin et
al., 1979
), and filter-bound primary antibodies were detected by peroxidase-catalyzed chemiluminescence (ECL method; Amersham Corp., Arlington Heights, IL).
In Vitro Vesicle Budding
Microsomes were isolated from strain CBY409 and incubated in the presence or absence of proteins required for reconstitution of vesicle formation as described (Barlowe et al., 1994). A 15-µl portion of the total reaction and 150 µl of a supernatant fluid containing vesicles released from
200-µl budding reactions were centrifuged at 100,000 g (model TLA100.3
rotor; Beckman Coulter, Inc., Fullerton, CA) to collect membranes. The
pellet fractions were dissolved in 30 µl of SDS-PAGE buffer, and 7-10 µl
of this material was resolved on 12.5% polyacrylamide gel and immunoblotted for Sec22p, Erv25p, Sec12p, and anti-HA for Erv14p-HA detection.
Subcellular Fractionation
Subcellular fractionation was performed as described by Antebi and Fink
(1992) with modifications by Schimmöller et al. (1995)
. Strains were
grown to exponential phase and converted to spheroplasts by lyticase
treatment (Baker et al., 1988
). Spheroplasts were centrifuged and resuspended in a sucrose solution (10 mM Hepes, pH 7.5, 12.5% sucrose, 1 mM
EDTA, 1 mM PMSF) and subjected to 10 strokes in a Dounce homogenizer. Two clearing spins were performed, and the resulting supernatant
fluid was placed on a sucrose gradient consisting of nine steps from 22 to
60% (wt/vol) in 10 mM Hepes, pH 7.4, 1 mM MgCl2. The gradients were
centrifuged at 35,000 rpm (model SW40 rotor; Beckman Instruments, Palo
Alto, CA) for 2.5 h at 4°C. 15 fractions of 0.77 ml each were taken sequentially from the top of the gradient to the bottom. Fractions were diluted in
SDS-PAGE sample buffer, and proteins were resolved on polyacrylamide gels and immunoblotted for Sec61p (ER marker), Emp47p (Golgi
marker), plasma membrane ATPase (PMA), Vph1 (vacuolar marker),
and anti-HA monoclonal antibody to detect Erv14p-HA or Axl2-HA.
Relative levels of specific proteins in each fraction were quantified by
densitometry of immunoblots. GDPase activity was determined as described (Yanagisawa et al., 1990) using CDP to subtract nonspecific phosphatase activity. Sucrose concentrations of individual fractions were determined by measuring the refractive index with an Abbe Refractormeter (American Optical, Buffalo, NY).
For subcellular fractionation under conditions of divalent cation chelation, the method of Kölling and Hollenberg (1994) was followed. Cells
were grown and spheroplasted as described above; however, lysates were
prepared by agitation with glass beads in buffer containing 10 mM Hepes,
pH 7.5, 12.5% sucrose, 10 mM EDTA, 1 mM PMSF. The cleared lysate
was loaded onto a similar 22-60% sucrose gradient as described above,
except gradients contained 10 mM EDTA, and samples were centrifuged
at 30,000 rpm (model SW40 rotor; Beckman Instruments) for 14 h at 4°C.
Fractions were collected and analyzed as described above for magnesium-containing gradients.
To characterize the membrane association of Erv14p, yeast cell membranes were isolated and treated with various agents as follows. Spheroplasts were prepared as indicated above and resuspended in buffer 88 (20 mM Hepes, pH 6.8, 250 mM sorbitol, 150 mM KOAc, 5 mM MgOAc) containing 1 mM DTT and 1 mM PMSF. After Dounce homogenization, a low-speed supernatant fraction was prepared by centrifugation at 5,000 rpm (model SS34 rotor; Sorvall, Newtown, CT). Aliquots from the supernatant fraction were treated with buffer 88, 0.5 M NaCl, 2.5 M urea, 0.1 M sodium carbonate, or 1% Triton-X 100 in buffer 88. These samples were mixed and incubated 20 min on ice followed by centrifugation at 60,000 rpm (model TLA 100.3 rotor; Beckman Instruments) for 15 min. Equivalent amounts of supernatant and pellet fractions were diluted in SDS-PAGE buffer and resolved on a 12.5% polyacrylamide gel. Blots were probed with anti-Emp47p (integral membrane protein), anti-Sec23p serum (peripheral membrane protein), or anti-HA monoclonal antibody to detect Erv14p-HA.
Calcofluor Staining of Bud Scars
Yeast strains in a logarithmic stage of growth were diluted into YPD medium to an OD600 of 0.002. When cultures reached an OD600 of 0.5-0.8, an
aliquot (1.5 ml) of cells was harvested and resuspended in calcofluor stain
at a concentration of 0.1 mg/ml, as described (Pringle, 1991). After incubation for 5-10 min at room temperature, the cells were washed three times
in distilled water and resuspended in a final volume of 50 µl. Stained yeast were viewed under a fluorescence microscope, and cells possessing six or
more bud scars were examined for an axial or nonaxial budding pattern.
Haploid cells that displayed one or more bud scars at opposite poles were
scored as nonaxial.
Sporulation and Cell Survival Experiments
Sporulation efficiency and cell survival studies were performed as follows. Diploid strains were cultured for 8 h at 30°C in YPD to an exponential phase of growth. Cells were then harvested, washed twice with water, and resuspended to an OD600 of 1 in spmD, a nitrogen-deficient medium composed of 1% potassium acetate, 0.1% yeast extract, and 0.05% dextrose. To assess sporulation efficiency, samples from these cultures were microscopically examined daily to determine the number of tetrads per 300 cells. Cell viability from these cultures was assessed over a 7-d period by spreading an equivalent amount of OD600 units on YPD plates. After 4 d of growth on YPD plates, the colonies were counted to determine cell viability.
Indirect Immunofluorescence
Yeast strains were grown in 25 ml of YPD to an OD600 of 0.3 and fixed
with 5% formaldehyde for 1 h. Fixed cells were then centrifuged for 3 min
in a clinical centrifuge, washed three times in PBSS (PBS, pH 7.4, and 0.7 M
sorbitol) and resuspended in a final volume of 400 µl PBSS. -Mercaptoethanol (20 mM final) and lyticase were added and incubated at room
temperature for 30 min to digest cell walls. The fixed spheroplasts were
washed twice and resuspended in 400 µl of PBSS, and 15 µl was applied to
polylysine-coated multiwell slides (Pringle et al., 1991
). Cells were adhered for 10 min, washed, and incubated with blocking buffer (PBSS with 1% BSA and 0.5% Triton X-100) for 10 min. Wells were washed twice with PBSS followed by the addition of primary antibodies (anti-Kar2p at
1:500 and anti-HA at 1:200) diluted in blocking buffer. After incubation at
room temperature for 90 min, cells were washed five times with PBSS and
then incubated with secondary antibodies that had been diluted in blocking buffer at 1:500 (anti-rabbit IgG conjugated to fluorescein or anti-
mouse IgG conjugated to Texas red). After 90 min, cells were washed four
times with PBSS followed by a 1-min incubation in PBSS containing 1 µg/
ml diamidophenylindole. Cells were then washed four times with PBSS,
and mounting medium (FITC guard; Testog, Inc., Chicago, IL) was layered on wells before sealing with coverslips. For all fluorescence microscopy, images were obtained using a cooled CCD camera, and composites
were prepared with Adobe Photoshop (San Jose, CA) software.
In Vivo Labeling
Pulse-chase experiments were performed as previously described (Belden
and Barlowe, 1996). In brief, cells were grown at 30°C (25°C for the sec12-4
strain) in selective medium containing 2% dextrose to an OD600 of 0.5. Cultures were harvested, washed, and resuspended at one-tenth the original volume in selective medium lacking sulfate. After culturing for 10 min
at 30°C (37°C for sec12-4 strain), cultures were pulsed for 10 min by the
addition of [35S]Express label (NENTM Life Science Products, Boston,
MA) and chased by the addition of excess methionine and cysteine. Cell
samples were taken at the end of the pulse period and after 10 and 20 min
of chase. Cell lysates were prepared by bead-beat lysis, and labeled species were precipitated from a common extract with specific antibodies for
CPY, Gas1p, or anti-HA monoclonal antibody that recognizes Axl2p-HA.
For endoglycosidase H (Endo H) experiments, 20-min chase time points
were taken, and Axl2p-HA was immunoprecipitated in duplicate from indicated strains. Washed immunoprecipitates were equilibrated with 100 mM
sodium citrate, pH 5.5, and one tube of each duplicate was incubated with
5 mU of Endo H (Sigma Chemical Co., St. Louis, MO) for 12 h at 37°C.
Samples were resolved on 7.5 or 10% polyacrylamide gels, and labeled
species were visualized by fluorography.
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Results |
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Identification of Erv14p
Uncoated ER-derived vesicles were isolated, and vesicle
proteins were resolved on a 15% polyacrylamide gel as
previously described (Belden and Barlowe, 1996). Approximately 0.02 mg of the 14-kD protein was purified and
subjected to automated NH2-terminal sequencing. The sequence GAWLFILAVVVNXINLFG was obtained from
the polypeptide corresponding to Erv14p (X represents a
residue that could not be unambiguously determined).
The NH2-terminal sequence of Erv14p (Fig. 1 A, underlined) aligns with an unidentified open reading frame on
chromosome VII (YGL054c) reported by the yeast genome sequencing project (Feuermann et al., 1997
). Conceptual translation of YGL054c produces a 138-amino acid
protein that contains three segments of sufficient length
and hydrophobicity to span a lipid bilayer. Based on this
sequence information and further data presented in this
report, Erv14p is likely an integral membrane protein. A
search of the current protein database identified a 142-
amino acid unidentified open reading frame in S. cerevisiae, YBR210w (Feldmann et al., 1994
), which shares 63%
identity with Erv14p, and the predicted 144-amino acid
cornichon gene product from Drosophila melanogaster,
which shares 36% identity. Other than these sequence homologies, Erv14p does not contain consensus sites for
N-linked glycosylation or any characterized sequence motifs to provide insight into molecular function.
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Erv14p Is an Integral Membrane Protein Localized to the ER and Golgi
To investigate Erv14p function and location, the molecular clone was modified to express a nine-amino acid influenza HA-epitope at the extreme COOH terminus that is
recognized by a monoclonal antibody HA.11 (see Materials and Methods). Yeast cells harboring this Erv14p-HA
expression vector on a centromere (CEN)-based plasmid produced an ~15-kD immunoreactive species that was absent in untransformed strains (Fig. 2 A). Experiments described in later sections (for example Table I) demonstrate
that Erv14p-HA complements the phenotypes displayed
by an erv14 strain and indicate that this tagged version is
fully functional. For the experiments described in this section, CBY409 was constructed such that Erv14p-HA is expressed from a CEN plasmid in an erv14
strain to keep the
concentration of Erv14p-HA near normal cellular levels.
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First, we isolated COPII vesicles from in vitro reactions
using ER membranes prepared from the Erv14p-HA-
tagged strain CBY409. If Erv14p is an authentic Erv protein, it should be selectively packaged into vesicles only when
COPII proteins are included in the incubation. Under reconstituted budding conditions (Fig. 2 B), ER-derived vesicles incorporated Erv14p-HA at a level (~12%) comparable to other characterized vesicle proteins, such as
Sec22p (Barlowe et al., 1994; Rexach et al., 1994
) and
Erv25p (Belden and Barlowe, 1996
). Resident ER proteins, such as Sec12p and Sec61p (not shown), were not
packaged into COPII-coated vesicles under these conditions. In this experiment, [35S]glycopro-
-factor was released at an efficiency of 23% in the presence of COPII
proteins and 3% in their absence. Thus, Erv14p satisfies
the initial criteria of an Erv protein such that this species is
selectively exported from ER membranes under conditions that reconstitute vesicle budding.
Next, we investigated the nature of Erv14p association
with membranes. The predicted amino acid sequence for
Erv14p suggests this protein spans the lipid bilayer three
times and is consistent with the result that several of the
Erv proteins (including an ~14-kD species) partition to a
carbonate inextractable pellet fraction (Rexach et al.,
1994). The fractionation behavior of Erv14p-HA was
monitored (Fig. 3) under conditions that extract peripherally bound membrane proteins (2 M urea), release lumenal proteins (0.1 M Na2CO3, pH 11), or solubilize integral
membrane proteins (1% Triton X-100). The fractionation
profile of Erv14p-HA was identical to an integral membrane protein such as Emp47p (Schröder et al., 1995
) and
not the peripheral membrane protein Sec23p (Hicke and
Schekman, 1989
). We conclude that Erv14p is an integral
membrane protein. Application of the "positive inside"
rule (von Heijne and Gavel, 1988
) suggests a topology
such that the NH2 terminus is oriented toward the cytoplasm and the COOH terminus is oriented toward the lumenal compartment.
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Previous experiments demonstrated that cycloheximide
pretreatment does not diminish the level of abundant Erv
proteins contained on COPII-coated vesicles (Yeung et al.,
1995). This condition depletes ER membranes of known
secretory proteins but does not inhibit in vitro synthesis
of COPII-coated vesicles. Based on this observation, we
hypothesize that the abundant Erv proteins, including
Erv14p, are not newly made secretory proteins en route to
the Golgi complex. Instead, we propose that many of the
Erv proteins are structural components of COPII-coated
vesicles and cycle between the ER and Golgi, functioning
in aspects of vesicle budding or fusion (Belden and Barlowe, 1996
). The following experiments indicate Erv14p
localizes to the ER and Golgi compartments and suggest
that Erv14p is not an abundant secretory protein. First, whole-cell immunofluorescence (Fig. 4) with an Erv14p-HA strain (CBY409) revealed a distinct perinuclear staining pattern for Erv14p-HA, much of which was coincident
with that observed for the ER-resident protein Kar2p/BiP
(Rose et al., 1989
). A distinct staining pattern was not detected using the anti-HA antibody in strains lacking the
Erv14p-HA construct, indicating a specific signal from the
HA epitope (data not shown). Second, fractionation of
membranes isolated from CBY409 on sucrose gradients
(Antebi et al., 1992) showed that ~70% of Erv14p-HA
cosediments with the ER marker Sec61p and ~30%
cosedimented with the Golgi marker Emp47p (Fig. 5).
This subcellular distribution is similar to other vesicle proteins (Emp24p and Erv25p) that appear to cycle between
the ER and Golgi compartments (Schimöller et al., 1996;
Belden, W.J., and C. Barlowe, manuscript in preparation).
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Erv14p Is Required for an Axial Budding Pattern in Haploid Cells
To characterize the function of Erv14p, we analyzed a
yeast strain bearing a null allele at the ERV14 chromosomal locus. Oligonucleotides corresponding to 3' and 5'
regions of ERV14 and HIS3 were used to direct HIS3 to
the ERV14 locus, thereby replacing the open reading
frame of Erv14p from start to stop codons. A heterozygous diploid (ERV14/erv14) was obtained and sporulated, and dissection of individual asci produced four viable spores. Analysis of these spores by growth on different
selective media and PCR amplification to confirm disruption indicated that ERV14 was dispensable for vegetative
growth (data not shown). Strains carrying the null allele
grew at rates identical to wild-type strains and were not thermosensitive. Although the logarithmic phase growth
rate of erv14
strains was wild-type, we found that erv14
strains exhibited a prolonged lag phase when diluted from
stationary phase cultures into standard rich media such as
YPD (see Materials and Methods). The lag phase delay
was further exacerbated when diluted into yeast minimal
media such as YMD. This growth phenotype was linked to
the HIS3 disruption of ERV14 and was corrected when
transformed with a plasmid containing the ERV14 gene.
Erv14p shares amino acid identity with the Drosophila
cornichon gene product over the entire open reading
frame, and their hydrophobicity profiles are superimposable. The cornichon gene is necessary for establishment of
anterior-posterior asymmetry during early stages of oogenesis (Ashburner et al., 1990; Roth et al., 1995
); however, a molecular determination of cornichon gene product function has not been reported. We used this clue of
cornichon function in generating cellular asymmetry to explore a possible role for Erv14p in yeast cell polarity. S.
cerevisiae undergoes polarized cell growth such that the
plane of cell division is determined by the site of bud formation and is dependent on cell type. Haploid yeast bud in
an axial manner, placing each new bud adjacent to the previous bud site. Genetic analysis of bud site selection has
revealed a group of bud and axl mutants defective in the
haploid axial budding pattern. The phenotypes of these
mutants fall into distinct categories, with one group that
displays a random bud site selection pattern and a second group that exhibits bipolar patterns instead of the normal
axial pattern (Bender and Pringle, 1989
; Chant and Herskowitz, 1991
; Chant et al., 1991
; Fugita et al., 1994
; Chant
and Pringle, 1995
; Halme et al., 1996
; Roemer et al., 1996
;
Sanders and Herskowitz, 1996
). A history of bud site selection in yeast may be visualized by staining with calcofluor, a fluorophore that binds to chitin and reveals previous bud scars as chitin-rich rings (Hayashibe and Katohda,
1973
). Logarithmic-stage cultures of wild-type and erv14
strains were grown in rich medium and stained with calcofluor. Strikingly, erv14
haploid strains displayed a nonaxial budding phenotype that was not observed in an
isogenic wild-type strain (Fig. 6). In a quantitative analysis
of bud site selection, the penetrance of this phenotype was
incomplete, but a significant fraction of mothers exhibited
nonaxial budding patterns (see Table II). Transformation
of erv14
strains with a CEN-based plasmid expressing
Erv14p or Erv14p-HA reversed the nonaxial budding
phenotype and confirmed that this defect was caused by
deletion of Erv14p (Table II). Furthermore, these results
indicated ERV14-HA is functional and complements as effectively as unmodified ERV14.
|
|
We also examined the influence of disrupting YBR210w
on bud site selection. This predicted open reading frame
on chromosome II shares 63% amino acid identity with
Erv14p and could be functionally redundant. Disruption
of this gene (ERV15) produced viable haploids (CBY347
and CBY353) that displayed no apparent phenotypes. Furthermore, combination of erv14 with erv15
(CBY354)
did not exacerbate the nonaxial budding pattern displayed
by a single erv14
strain (not shown). We also designed a
construct to express an epitope tag on the COOH terminus of Erv15p, an approach that had proven successful for
detection of Erv14p. Although DNA sequencing indicated correct synthesis of this construct, we failed to detect a
tagged species under our standard growth conditions (data
not shown). To rationalize these observations, we speculate that ERV15 is not functionally redundant with ERV14
when cells are grown in rich medium and that ERV15 expression may be restricted to specific stages of the yeast
life cycle.
Wild-type a/ diploids exhibit a bipolar budding pattern
such that a mother cell may produce a new bud at either
pole from the previous bud site. We examined the budding
pattern in homozygous diploid strains lacking Erv14p
(CBY410) and in strains lacking both Erv14p and Erv15p
(CBY411). These strains did not exhibit any alterations in
the bipolar positioning of the bud site (data not shown).
Therefore, erv14
strains possess haploid-specific defects
in establishing cell polarity, as reported for a subset of the
axl and bud mutants (Chant et al., 1995
; Roemer et al., 1996
).
Axl2p Accumulates in the ER of erv14 Mutants
Because Erv14p is localized to the early compartments of
the secretory pathway, and this pathway is responsible for
the delivery of proteins to the plasma membrane, we considered the possibility that Erv14p was required for transport of factors to the cell surface for establishment of cell
polarity. Combined molecular/genetic approaches have
provided a wealth of information on the proteins involved
in bud site selection in yeast (for review see Chant, 1996).
Axl2p is one of the characterized proteins that is required for an axial budding pattern and displays a bipolar phenotype when disrupted in haploid cells. Axl2p is also an integral membrane glycoprotein with a predicted type I topology and is known to traverse the secretory pathway en
route to the cell surface (Roemer et al., 1996
). During the
biogenesis of Axl2p, N-linked core oligosaccharides are
added in the ER and are further extended during passage
through Golgi compartments. We tested if Axl2p was efficiently transported in strains carrying an erv14
allele and
used a triple-HA-tagged version of Axl2p (known to complement an axl2
strain) to monitor transport of Axl2p
(Roemer et al., 1996
). In an initial experiment, we immunoblotted whole-cell extracts from wild-type and mutant strains expressing Axl2p-3HA (Fig. 7). In an erv14
null
strain, an ~150-kD HA-tagged species that was not detected in wild-type strains was apparent. In contrast, wild-type strains expressed an ~220-kD form that was a very
minor species in erv14
null strains. We reasoned that the
150-kD form of Axl2p-3HA that was unique to the erv14
strain represented a core-glycosylated form of this secretory protein that may accumulate in the ER. The next series of experiments are focused on this hypothesis.
|
The temperature-sensitive sec12-4 allele blocks ER to
Golgi transport when shifted to a restrictive temperature,
and ER forms of secretory proteins accumulate (Novick
et al., 1980; Stevens et al., 1984
). Sec12p is an integral
membrane glycoprotein localized to the ER, and it is required for the formation of transport vesicles from this
compartment (Nakano et al., 1988
; d'Enfert et al., 1991
). We transformed a sec12-4 strain with the Axl2p-3HA expression construct to monitor the ER form of Axl2p-3HA
that accumulates when shifted to a restrictive temperature.
Under steady-state conditions (Fig. 7, lane 3), the 150-kD
form of Axl2p-3HA was not detected; however, after a
shift to 37°C for 2 h, a small amount of this species became
apparent in a sec12-4 strain (Fig. 7, lane 4).
The above experiments suggest that Axl2p-3HA accumulates in the ER as a 150-kD core-glycosylated form in
erv14 and sec12-4 strains. The immunoblot experiments
provide a steady-state view of Axl2p-3HA in these strains.
However, we sought to characterize the kinetics of Axl2p-3HA transport in wild-type and erv14
strains through
a pulse-chase analysis. In these experiments, cells were grown in minimal medium and pulsed with [35S]methionine and cysteine for 10 min to label newly synthesized proteins. Excess cold methionine and cysteine were then
added to initiate the chase phase, and the fate of specific
secretory proteins (Axl2p-3HA, CPY, and Gas1p) were
monitored by selective immunoprecipitation of these species from whole-cell lysates (Fig. 8). CPY is first detected
in the ER as the P1 precursor (67 kD), then modified upon
arrival to the Golgi complex producing the P2 form (69 kD),
and finally processed to the mature form (67 kD) in the
vacuole (Stevens et al., 1984
). As shown in Fig. 8, wild-type strains and the erv14
strain exhibited similar kinetics for CPY transport to the vacuole, whereas the sec12-4
temperature-sensitive mutation accumulated the ER form
(P1) of CPY when shifted to a restrictive temperature.
Similar results were observed for transport of the glycosylphosphatidylinositol-anchored plasma membrane protein Gas1p. Newly synthesized Gas1p appeared in the ER
as a 105-kD glycosylphosphatidylinositol-anchored precursor that carries N- and O-linked oligosaccharide. As
Gas1p traverses the Golgi complex, outer chain glycosylation residues are added, generating the 125-kD mature
form (Nuoffer et al., 1991
). Gas1p was transported out of
the ER in wild-type and erv14
strains; however, we see a
subtle delay in Gas1p transport (note the ratio of ER form
to mature form after a 10-min pulse in the Gas1p panel in
Fig. 8). This delay was not as severe as seen in strains bearing deletions of other Erv proteins, such as Emp24p and
Erv25p (Belden and Barlowe, 1996
). In sec12-4 cells, the
ER form of Gas1p accumulated but displayed a reduced
electrophoretic mobility during the chase period, as has
been previously observed (Schimmöller et al., 1995
;
Belden and Barlowe, 1996
). Based on these results, we
conclude that the ERV14 gene is not required for transport of CPY and Gas1p from the ER to the Golgi complex, in contrast to sec mutant strains such as sec12-4 (Novick et al., 1980
; Stevens et al., 1984
). This result is also
consistent with the wild-type growth rate for erv14
since
cell surface expansion (i.e., growth rate) was not impeded in these strains, again in contrast to typical sec mutations
that are lethal and prevent expansion of the plasma membrane.
|
Transport of Axl2p was also examined in these strains.
Strikingly, the transport block observed in an erv14 stain
was as complete as seen in a sec12-4 strain (Fig. 8). We
could not detect the mature form of Axl2p in the erv14
strain even after the 20-min chase period. This result is
consistent with the steady-state analysis in an erv14
strain conveyed though immunoblotting in Fig. 7, where
the 150-kD form accumulated and the level of mature species was depleted. Furthermore, the 150-kD form of Axl2p
that accumulated in an erv14
strain was relatively constant during the 20-min chase period, indicating that this
species is not rapidly degraded. The transport of Axl2p
from the ER to the Golgi appeared to occur rapidly. Several attempts were made to detect earlier secretory forms
of Axl2p-3HA using shorter pulse time periods in larger-scale reactions, but we failed to detect ER and Golgi forms
of this protein under these conditions. We speculate that a
short transitory time coupled with the heterogeneity of
modifications on Axl2p-3HA as it is transported though
the secretory pathway prevents detection of these intermediates.
We proposed that Axl2p is not exported from the ER in
erv14 strains and sought additional lines of evidence in
support of this proposal. Axl2p acquires N-linked oligosaccharide in the ER of yeast cells (Roemer et al., 1996
),
and if the form that accumulates in an erv14
strain is
trapped in the ER, treatment with Endo H should liberate
this covalently linked carbohydrate and produce a faster
migrating polypeptide on polyacrylamide gels (Orlean et al.,
1991
). After immunoprecipitation of Axl2p-3HA from
various strains, treatment with Endo H produced an alteration in the mobility of the labeled polypeptide (Fig. 9).
The forms of Axl2p-3HA that accumulated in an erv14
and a sec12-4 strain displayed identical properties upon
treatment with Endo H, shifting the ~150-kD ER-form to
an ~125-kD species. Based on an approximation of each
core oligosaccharide contributing 2 kD in mass (Orlean et al.,
1991
), we estimate the attachment of ~13 N-linked chains on Axl2p, which was predicted to contain 16 potential
N-linked glycosylation sites (Roemer et al., 1996
). Treatment of the mature form of Axl2p-3HA with Endo H also
produced a distinct shift in size from ~220 to ~145 kD,
but clearly not to the 125-kD species that appears after removal of N-linked residues from the ER form. We speculate that Axl2p acquires O-linked oligosaccharides in the
ER that are then extended upon transport through the
Golgi (Tanner and Lehle, 1987
). Indeed, preliminary data
indicate that Axl2p contains O-linked oligosaccharide
(Sanders, S., and M. Gentzsch, personal communication),
which would also explain the difference between the predicted size (~90 kD) and the Endo H-treated ER form
(~125 kD). Regardless, the form of Axl2p-3HA that accumulates in an erv14
strain behaves identically to the ER
form that accumulates in a sec12-4 strain, a well-characterized mutant representative of mutants blocked in export
from the ER (Novick et al., 1980
; Stevens et al., 1984
; Nakano et al., 1988
). This observation, coupled with the fact
that CPY and Gas1p are transported and modified correctly, make it unlikely that the erv14
mutation alters the glycosylation machinery producing modification defects
on Axl2p.
|
As an independent method to evaluate Axl2p location
in erv14 strains, we performed immunofluorescence experiments to visualize Axl2p-3HA in wild-type and erv14
strains. Axl2p is reported to localize to discrete sites at the
cell periphery depending on the phase of the cell cycle and
first appears in nascent buds as a crescent-shaped patch
that then diffuses and appears as a ring at the mother-
daughter bud neck (Roemer et al., 1996
). Immunofluorescence images generated from double staining wild-type
and erv14
strains with anti-HA and anti-Kar2p revealed
the expected localization pattern for Axl2p-3HA in wild-type strains (Fig. 10). In contrast, we did not detect this
staining pattern for Axl2p-3HA in erv14
strains after examination of several hundred stained cells. Axl2p-3HA appeared to colocalize with Kar2p in some images, but a
definitive ER localization for Axl2p remained equivocal
through this approach. The accumulation of Axl2p-3HA
in the ER may produce a stain that is too diffuse for detection in this compartment. The validity of our immunofluorescence procedure for erv14
cells was confirmed by observation of a characteristic ER-staining pattern for Kar2p (Fig. 10). We can conclude that the normal localization
pattern of Axl2p-3HA is blocked in an erv14
strain, and
this result is entirely consistent with a block in export from
the ER observed in the pulse-chase experiments.
|
Because immunofluorescence did not document the
subcellular location of Axl2p-3HA in an erv14 strain, we
performed cell fractionation experiments to determine
where Axl2p accumulates in this strain. A standard magnesium-containing sucrose gradient method (Antebi and
Fink, 1992
) that resolves several yeast organelles was used to monitor the subcellular distribution of Axl2p in a wild-type and an erv14
strain. In a wild-type strain (Fig. 11, A
and B), the mature form of Axl2p-3HA comigrates with
the PMA and is resolved from Golgi (GDPase) and vacuolar (Vph1) membranes. The 150-kD form of Axl2p-3HA
that accumulates in an erv14
strain (Fig. 11, C and D)
comigrates with ER membranes (Sec61p) and is resolved from Golgi and vacuolar membranes. However, the conditions of this gradient do not cleanly separate ER membranes (Sec61p) from plasma membranes (PMA), and we
chose another sucrose gradient fractionation procedure to
resolve these compartments. This method relies on a more
vigorous lysis procedure in the presence of EDTA, a condition that strips ribosomes from the ER and produces a
corresponding shift of ER membranes up in the gradient
to a lower buoyant density (Kölling and Hollenberg, 1994
;
Roberg et al., 1997
). As seen in Fig. 12, the 150-kD form of
Axl2p-3HA observed in an erv14
strain coincides with
the peak of Sec61p (Fig. 12, C and D) and is resolved from
the PMA. Based on the fractionation patterns observed in
Figs. 11 and 12, we conclude that Axl2p-3HA in erv14
strains is localized to the ER, a result that is entirely consistent with our pulse-chase and immunofluorescence experiments. Furthermore, these sucrose gradient analyses
indicate that additional secretory proteins (PMA, GDPase, and Vph1) are synthesized and localized correctly in
an erv14
strain.
|
|
Pleiotropic Effects of erv14 Mutations
To determine if ERV14 deletion produced altered budding patterns in diploid cells, we constructed the homozygous disruptant strain CBY410. This diploid strain does
not display a bud site selection defect (normal bipolar pattern), which is consistent with the observation that axl2
homozygous diploids are phenotypically bipolar (Roemer
et al., 1996
). However, we found that the homozygous erv14
disrupted strain would not sporulate under standard sporulation conditions (Sherman, 1991
). We tested if
erv14
/erv14
diploids became inviable under these conditions and found that the cell viability of wild-type
(CBY453) and mutant (CBY410) cultures were similar after several days in sporulation media. Further, the mutant
strains grew on nonfermentable carbon sources as efficiently as wild-type strains, indicating the carbon source
contained in sporulation media is adequate. Finally, transformation of CBY410 with the Erv14p-HA plasmid (strain
CBY433) restored sporulation competency to wild-type
levels (Table III). These results indicate Erv14p is required for some aspect of sporulation.
|
Previous studies have shown that Axl2p is expressed at
equal levels in both haploid and diploid cells, although this
protein does not appear to participate in bud site selection
in diploids (Roemer et al., 1996). We considered the possibility that delivery of Axl2p to the cell surface could also
be required for efficient sporulation. Our previous results
(Table II) demonstrated that overproduction of Axl2p
partially suppressed the nonaxial budding phenotype of
haploid erv14
strains. Therefore, we tested if overproduction of Axl2p could rescue the sporulation defect. However, the sporulation efficiency of homozygous erv14
disruptants was not affected by transformation with a
multicopy version of AXL2 (Table III). In summary, deletion of ERV14 leads to defects in haploid bud site selection, in recovery from stationary phase growth and in
sporulation of diploid cells. The nonaxial budding phenotype may be suppressed by overproduction of Axl2p,
whereas recovery from stationary phase growth and
sporulation were not affected by the expression level of
Axl2p. These pleiotropic effects suggest Erv14p functions
in other cellular processes besides transport of Axl2p and
that perhaps gene products involved in sporulation rely on
Erv14p for efficient transport.
![]() |
Discussion |
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---|
Organelles of the eukaryotic secretory pathway remain
distinct in spite of dynamic anterograde and retrograde
transport processes. Specific coat proteins that catalyze
transport between the ER and Golgi are thought to contribute to this organization (Schekman and Orci, 1996), although the molecular mechanisms that link coat proteins
with cellular sorting are not understood. Here we characterize a novel protein, termed Erv14p, that was discovered
on ER-derived transport vesicles and appears to participate in sorting during ER to Golgi transport. Erv14p is an
integral membrane protein that shares significant sequence identity (36%) and similarity (63%) over the entire length of the Drosophila cornichon gene product. Localization studies indicate that Erv14p resides in the ER
and Golgi compartments of cells and is selectively packaged into ER-derived vesicles in a COPII-dependent manner. Disruption of the ERV14 gene produces viable haploid cells that exhibit defects in axial bud site selection.
This phenotype correlates with the failure of erv14
strains to transport a bud site selection protein (Axl2p) to
the cell surface. We propose that Erv14p regulates export
of Axl2p and possibly other secretory proteins from the ER in COPII-coated vesicles as depicted in Fig. 13.
|
Erv14p is composed largely of hydrophobic amino acids
and possesses three linear segments of adequate hydrophobicity to span a lipid bilayer (Kyte and Doolittle,
1982). Application of the "positive inside" rule (von
Heijne and Gavel, 1988
) predicts a topology such that the
NH2 terminus is oriented toward the cytoplasm and the
COOH terminus is oriented toward the lumenal compartment. The first putative loop (amino acids 29-51) displays
a net negative charge, whereas positively charged residues
are enriched in loop two (amino acids 81-111). This charge
distribution is highly conserved between Erv14p and cornichon, lending some credence to this topology prediction,
but there are exceptions to the positive inside rule, and it is
not possible to draw a firm conclusion about the transmembrane arrangement of Erv14p at this time. Because
Erv14p is detected in the ER, ER-derived vesicles, and
Golgi membranes, it appears that this molecule cycles between early compartments of the secretory pathway, and
we speculate that amino acid residues in this protein impart selective packaging into COPII- and/or COPI-coated
vesicles. Characterized sequence motifs proposed to mediate incorporation into COPII-coated vesicles (Nishimura
and Balch, 1997
; Dominguez et al., 1998
) or COPI-coated
vesicles (Nilsson et al., 1989
; Cosson and Letourneur,
1994
) are not found in Erv14p. Therefore, selective incorporation of Erv14p into ER-derived vesicles could be
through direct interaction of COPII with novel signal(s)
contained on the cytoplasmic surface(s) of Erv14p or
through association of Erv14p with other proteins coupled
to the COPII budding machinery.
Surprisingly, deletion of ERV14 did not interfere with
bulk secretory function but instead produced defects in
yeast cell polarity. To comprehend this phenotype, we reviewed the literature concerning bud site selection in
yeast. Haploid yeast cells exhibit an axial budding pattern
whereby each new bud forms directly adjacent to the previous bud site. The selection of an appropriate bud site is
thought to rely on a series of integrated events: first, the
selected site for budding must be marked; second, components required for bud formation are assembled at this
site; and third, the actin cytoskeleton and secretory apparatus are directed toward the selected site for growth of
the emerging bud (Drubin, 1991). For the axial budding
pattern, it has been proposed that this first stage is accomplished through a landmark that persists after cytokinesis
and provides the cell with an assembly site for the next
round of budding (Chant and Herskowitz, 1991
; Snyder et
al., 1991
). Axl2p is unique among the characterized bud
site selection proteins because it must be delivered to the
plasma membrane via the secretory pathway. Once anchored in the plasma membrane, Axl2p may recruit additional components to the incipient bud site. In haploid
axl2
strains, the axial budding pattern is lost, and a bipolar phenotype is observed such that ~50% of the newly
formed buds are placed at the opposite pole from the previous bud site (Halme et al., 1996
; Roemer et al., 1996
).
When we examined erv14 strains, we observed a nonaxial budding pattern and found that Axl2p accumulated
in the ER. The accumulation of Axl2p in the ER provides
a rational explanation for the nonaxial phenotype displayed by erv14
strains. Based on the following observations, however, we suspect that some Axl2p is slowly
transported to the cell surface in erv14
strains. First, immunoblot analysis indicated that a low level of the mature
form of Axl2p was detected in erv14
strains, although
this species appears to be synthesized at a slow rate since it
was not detected in pulse-chase experiments. Second, only
~16% of the erv14
cells exhibit budding from both poles
in contrast to a more typical bipolar pattern observed in axl2
strains (Halme et al., 1996
; Roemer et al., 1996
).
This may be explained if erv14
cells deliver some Axl2p
to incipient bud sites, but with suboptimal levels of plasma
membrane Axl2p, a nonaxial phenotype is displayed intermittently. Third, we find that overexpression of Axl2p
partially suppressed the nonaxial budding phenotype in
erv14
strains (Table II). Again, this observation may be
explained if some Axl2p trickles through the secretory pathway in an erv14
strain, and overexpression of Axl2p
increases the level of this flow.
Could the role of Erv14p in yeast trafficking provide insights on the function of cornichon? The cornichon mutants display phenotypes that are similar to torpedo (EGF
receptor) and gurken (TGF homologue and putative torpedo ligand) mutants. These three genes are components
of an intercellular signaling process between germ-line
cells and surrounding follicle cells that establishes anterior-posterior polarity during early stages of oogenesis. Both gurken and cornichon are required in germ-line cells,
whereas torpedo function is required in surrounding follicle cells of the developing egg chamber. The localized delivery of gurken protein to the plasma membrane of the
oocyte presumably activates the EGF receptor torpedo in
a subset of follicle cells and specifies their posterior fate.
In turn, the polarized arrangement of the surrounding follicle cells provides spatial information to the oocyte and is
critical for the reorganization of the microtubule network
at mid-oogenesis. In cornichon, gurken, and torpedo mutants, intercellular signaling between the oocyte and surrounding follicle cells fails. Anterior markers are abnormally expressed in the posterior follicle cells, producing
egg chambers that have the normal arrangement of oocyte
and nurse cells but have duplicated anterior follicle cells at
both poles. It is postulated that the gurken signal emanating from the oocyte represses anterior fates in adjacent
follicle cells and directs them to a posterior fate (Gonzáles-Reyes and St. Johnston, 1994
; Roth et al., 1995
). In cornichon mutants, gurken mRNA expression and perinuclear localization is normal. Examination of gurken protein reveals that the expression level is normal, but cornichon egg chambers display a diffuse staining pattern for
gurken protein at the oocyte membrane, unlike the tight
stripe-like distribution at the dorsal-anterior corner of the
oocyte observed in wild-type. Indeed, one explanation offered for this phenotype was that an altered polarity in
cornichon egg chambers would cause less efficient membrane targeting of vesicles transporting gurken protein
(Roth et al., 1995
).
In light of our findings with erv14 strains, it is plausible
that in cornichon mutants, a landmark on the oocyte cell
surface is not established to correctly orient the secretory
pathway. Much as the yeast cell uses Erv14p to export
Axl2p from the ER and mark the axial bud site, we speculate that cornichon is required for export of a polarity establishment factor from the oocyte ER in Drosophila. Although there are no candidates for this factor at present,
the high degree of homology shared between Erv14p and
the cornichon gene product suggests this molecule may be
related to Axl2p.
The mechanism by which Erv14p catalyzes Axl2p export from the ER remains to be determined, and we can
envision several possibilities to explain this transport
block. First, Erv14p could directly bind to Axl2p and escort this protein out of the ER, acting as an adaptor for incorporation of Axl2p into COPII-coated vesicles. Direct
binding could also be involved in the folding of Axl2p or
assembly of Axl2p into an oligomeric complex before exit
from the ER, although we do not favor this possibility because proteins involved in these processes (e.g., BiP) appear to remain in the ER and are not selectively packaged
into ER-derived vesicles (Salama et al., 1993; Barlowe et
al., 1994
; Rexach et al., 1994
). Furthermore, the forms of
Axl2p that accumulate in the ER of erv14
and sec12 strains are indistinguishable and are not rapidly degraded,
suggesting that Axl2p is stably folded but unable to depart
the ER. The erv14
phenotype resembles yeast strains
that lack Shr3p, a resident ER protein that is required for
the export of amino acid permease molecules in COPII-coated vesicles (Ljungdahl et al., 1992
; Kuehn et al., 1996
,
1998
). However, the activities of Erv14p and Shr3p appear
to be distinct because Erv14p is selectively packaged into COPII-coated vesicles, whereas Shr3p does not appear to
enter these vesicles (Kuehn et al., 1996
). Another set of
ER proteins that produce selective transport defects
(Vma12p, Vma21p, and Vma22p) are required for export
of integral membrane subunits of the vacuolar ATPase
(Hill and Stevens, 1994
, 1995
; Jackson and Stevens, 1997
).
It remains to be determined if these Vma proteins are selected for incorporation into COPII-coated vesicles. However, it has been proposed that Vma12p, Vma21p, and
Vma22p function in the assembly of V-ATPase subunits in
the ER and that assembly is a prerequisite for export from
the ER (Jackson and Stevens, 1997
). At present, we are
aware of only three proteins that when deleted produce
selective ER to Golgi transport defects and are enriched
on COPII-coated vesicles: Emp24p (Schimöller et al., 1995), Erv25p (Belden and Barlowe, 1996
), and Erv14p.
We continue to explore the protein-protein interactions
and mechanisms by which these molecules influence sorting during transport from the ER.
![]() |
Footnotes |
---|
Received for publication 29 April 1998 and in revised form 9 July 1998.
Address all correspondence to Charles Barlowe, Department of Biochemistry, Dartmouth Medical School, Hanover, NH 03755. Tel.: (603) 650-6516. Fax: (603) 650-1353. E-mail: barlowe{at}dartmouth.eduWe thank Bill Belden for help with strain construction, Terry Roemer and Michael Snyder for generously providing AXL2 constructs, Hannele Ruohola and Trudi Schüpbach for helpful discussions on Drosophila development, and Sylvia Sanders for advice and sharing her unpublished observations.
This work was supported by grants from the National Institute of General Medical Sciences and the Pew Scholars Program in the Biomedical Sciences.
![]() |
Abbreviations used in this paper |
---|
CPY, carboxypeptidase Y; Endo H, endoglycosidase H; Erv, ER vesicle; HA, hemagglutinin; PMA, plasma membrane ATPase.
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