Identification of Novel Vesicles in the Cytosol to Vacuole Protein Degradation Pathway

doi:10.1083/jcb.136.4.803

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© The Rockefeller University Press, 0021-9525/1997//803 $5.00
The Journal of Cell Biology, Volume 136, Number 4, , 1997 803-810

Article

Identification of Novel Vesicles in the Cytosol to Vacuole Protein Degradation Pathway

Pei-Hsin Huang and Hui-Ling Chiang

Department of Cell Biology, Harvard Medical School, Boston, Massachusetts 02115

The key gluconeogenic enzyme, fructose1,6-bisphosphatase (FBPase),is induced when Saccharomyces cerevisiae are starved of glucose.FBPase is targeted from the cytosol to the yeast vacuole fordegradation when glucose-starved cells are replenished withfresh glucose. Several vid mutants defective in the glucose-induceddegradation of FBPase in the vacuole have been isolated. Insome vid mutants, FBPase is found in punctate structures inthe cytoplasm. When extracts from these cells are fractionated,a substantial amount of FBPase is sedimentable in the highspeed pellet, suggesting that FBPase is associated with intracellularstructures in these vid mutants. In this paper we investigatedwhether FBPase association with intracellular structures alsoexisted in wild-type cells. We report the purification of novelFBPase-associated vesicles from wild-type cells to near homogeneity.Kinetic studies indicate that FBPase association with thesevesicles is stimulated by glucose and occurs only transiently,suggesting that these vesicles are intermediate in the FBPasedegradation pathway. Fractionation analysis demonstrates thatthese vesicles are distinct from known organelles such as thevacuole, ER, Golgi, mitochondria, peroxisomes, endosomes, COPI,or COPII vesicles. Under EM, these vesicles are 30–40nm in diam. Proteinase K experiments indicate that the majorityof FBPase is sequestered inside the vesicles. We propose thatFBPase is imported into these vesicles before entering the vacuole.

Abbreviations used in this paper: API, aminopeptidase I; CPY, carboxypeptidase Y; ECL, enhanced chemiluminescence; FBPase, fructose-1,6bisphosphatase.

The key regulatory enzyme in the gluconeogenesis pathway, fructose-1,6-bisphosphatase(FBPase)¹, is induced when Saccharomyces cerevisiae are grown in medium containing poor carbon sources (Gancedo, 1971). When cells are transferred to medium containing fresh glucose,FBPase is rapidly inactivated and degraded (Gancedo, 1971; Chiang and Schekman, 1991).Regulated degradation of FBPase is mediated by a selective targetingof FBPase from the cytosol to the lysosome (vacuole) for degradation(Chiang and Schekman, 1991, 1994; Chiang et al., 1996). Theglucose-induced FBPase redistribution into the vacuole hasbeen demonstrated by cell fractionation, immunofluorescencemicroscopy, and immunoelectron microscopy (Chiang and Schekman, 1991,1994; Chiang et al., 1996).

Glucose also inactivates peroxisomal enzymes in Hasenula polymorpha,Pichia pastoris, Candida boidinii, or S. cerevisiae (Bormann and Sahm, 1978;Veenhuis et al., 1983; Tuttle and Dunn, 1995; Chiang et al., 1996).Peroxisomes are taken up by the vacuole by autophagy. In P.pastoris, two modes of autophagy operate to deliver peroxisomesto the vacuole for degradation (Tuttle and Dunn, 1995). Peroxisomescan be taken up by the vacuole by microautophagy when cellsare transferred from methanol to glucose. When cells are shiftedfrom methanol to ethanol, peroxisomes are surrounded by a layerof membrane, and then internalized by the vacuole by macroautophagy(Tuttle and Dunn, 1995). In addition to FBPase and peroxisomes, the maltose transporter and the galactose transporter are also degraded in the vacuole in response to glucose (Riballo et al., 1995;Chiang et al., 1996). These transporters are delivered to thevacuole by the endocytic pathway, as mutants defective in theendocytic process impair the glucoseinduced degradation of thesesugar transporters (Riballo et al., 1995; Chiang et al., 1996).Accumulation of autophagic bodies inside the vacuole has beenobserved when S. cerevisiae are starved of nitrogen (Takeshige et al., 1992).

Proteins can be sorted to the vacuole through the secretorypathway. The vacuolar protein carboxypeptidase Y (CPY) is synthesized,processed, and transported from the ER to the Golgi (Hasilik and Tanner, 1978;Hemmings et al., 1981; Rothman and Stevens, 1986; Banta et al., 1988;Jones, 1991). Sorting occurs in the late Golgi by the Pep1p/Vps10p (CPY receptor protein). CPY is delivered to the vacuolethrough the prevacuolar compartments, and the CPY receptorrecycles back to the Golgi compartment (Marcusson et al., 1994;Cooper and Stevens, 1996). Other vacuolar proteins such asaminopeptidase I (API) and ${alpha}$ -mannosidase are transported directlyfrom the cytosol to the vacuole, independent of the secretorypathway (Yoshihisa and Anraku, 1990; Klionsky et al., 1992).Mutants defective in API targeting to the vacuole have been isolated. They process and sort CPY normally, suggesting thatthe API targeting pathway is different from the CPY sortingpathway (Harding et al., 1995).

In mammalian cells, serum starvation induces protein degradationby lysosomes (Dice, 1990; Haynes and Dice, 1996). This proteindegradation pathway requires a pentapeptide sequence (Chiang and Dice, 1988;Chiang et al., 1989; Terlecky et al., 1992). Proteins are translocatedto the lysosomal lumen by a heat shock protein–mediatedprocess (Terlecky and Dice, 1993; Cuervo et al., 1994). Thereceptor protein for the selective uptake of RNase A and glyceraldehyde-3-phosphatedehydrogenase by lysosomes has been identified to be the lysosomalglycoprotein LGP96 (Cuervo and Dice, 1996). Overexpressionof LGP96 increases the activity of the selective lysosomal degradation pathway both in vivo and in vitro (Cuervo and Dice, 1996).

To study the pathway of FBPase degradation in S. cerevisiae,mutants defective in the glucose-regulated degradation of FBPasewere isolated using a colony blotting procedure (Hoffman and Chiang, 1996).The vid (vacuolar import and degradation) mutations are allrecessive. They process and sort CPY normally, suggesting thatthey are distinct from the mutants affecting vacuolar proteolysis (pep), protein secretion (sec), and vacuolar protein sorting (vps). FBPase is inactivated by the cAMP-dependent signal transductionpathway (Lamponi et al., 1987; Toyoda et al., 1987). Sincevid mutants all inactivate FBPase at rates indistinguishablefrom wild-type cells, the vid mutants appear to transduce signalproperly. Immunolocalization experiments demonstrated that FBPaseis found in the cytosol in most vid mutants. In some vid mutants, FBPase is found in punctate structures in the cytoplasm (Hoffman and Chiang, 1996).When extracts from these cells are further fractionated, asubstantial amount of FBPase is sedimentable in the high speedpellet, suggesting that FBPase is associated with intracellularstructures in these mutants (Hoffman and Chiang, 1996).

We investigated whether FBPase association with intracellularstructures also existed in wild-type cells. Since this associationmight occur rapidly at 30°C, we monitored FBPase distributionafter transfer of wild-type cells to glucose at timed intervalsat 22°C, based on our earlier observation that FBPase targetingto the vacuole is delayed at this temperature. We report thepurification of FBPase-associated vesicles to near homogeneityfrom wild-type cells. Proteinase K experiments demonstrate thata substantial amount of FBPase is sequestered inside the vesicles.We propose that FBPase is imported into the vesicles beforeentering the vacuole.

Materials and Methods

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Abstract
Materials and Methods
Results
Discussion
References

Strains, Media, and Antibodies
The strain used in this study was W303 (MAT ${alpha}$ leu2-3,112 ade2his3-200 trp1-1 ura3-52). YPD contained 1% yeast extract (DifcoLaboratories, Inc., Detroit, MI), 2% peptone (Difco Laboratories,Inc.), and 2% glucose. YPKG contained 1% yeast extract, 2%peptone, 1% potassium acetate, and 0.5% glucose. Anti-FBPaseantibodies were produced by injecting rabbits with affinity-purifiedFBPase. Anti-Sec21p and Sec22p antibodies were kindly providedby Dr. C. Barlowe (Dartmouth Medical School, Hanover, NH),anti-Sec62p by Dr. T. Rapoport (Harvard Medical School, Boston,MA), anti-Mnn1p by Dr. T. Graham (Vanderbilt University, Nashville,TN), and anti-Pep12p by Dr. S. Emr (University of California at San Diego). Antibodies were used at 2,000 dilution for Sec21p,Sec22p, Mnn1p, and Pep12p, and 10,000 dilution for Sec62p,Pma1p, 3-oxoacyl CoA thiolase, cytochrome C, and FBPase. Antibodiesdirected against plasma membrane ATPase, 3-oxoacyl CoA thiolasewere produced as described (Chiang et al., 1996). Anti-CPY andcytochrome C were produced by injecting rabbits with CPY (SigmaChemical Co., St. Louis, MO) and cytochrome C (Sigma ChemicalCo.).

Cell Fractionation
Yeast cells were grown in 1 liter of YPKG for 2 d at 30°Cin an environmental shaker (300 rpm). Cells (OD₆₀₀ = 10,000)were harvested by centrifugation at 500 g for 5 min and divided.Cells were shifted to YPD for 0, 30, 60, or 90 min at 22°C.At the end of incubation, 10 mM NaN₃ was added to the culturemedium and yeast cells were collected by centrifugation. Spheroplastswere prepared as described (Hoffman and Chiang, 1996). Spheroplastswere homogenized using a Dounce homogenizer with 20 strokeson ice. Cell lysates were centrifuged first at 15,000 g for20 min. The supernatant was further centrifuged at 100,000g for 2 h to obtain the high speed supernatant and pellet.The pellet was resuspended in 1 ml of TEA buffer (10 mM triethanolamine,pH 7.5, 100 mg/ml PMSF, 10 mM NaF, 10 mM NaN₃, 1 mM EDTA, and0.8 M sorbitol), loaded on a 90 cm x 1.5 cm Sephacryl S-1000(Pharmacia Fine Chemicals, Piscataway, NJ) column, and elutedwith 200 ml of TEA buffer with a flow rate of 8 ml/h. Fractions(4 ml) were collected, and 1.5 ml of samples was precipitated with TCA at the final concentration of 10% at 4°C for 1h on ice. Samples were centrifuged at 13,000 g for 10 min at4°C, and pellets were washed once with 1 ml ice-cold acetoneand resuspended in 50 µl of SDS sample buffer. Proteins(15 µl) were separated on SDS-PAGE gels and immunoblottedwith antibodies directed against FBPase and organelles, followed by 1:10,000 dilution of HRP-conjugated anti–rabbit antibodiesand exposure on x-ray films after enhanced chemiluminescence(ECL) reactions. For the detection of CPY, Sec21p, plasma membraneATPase, and Mnn1p, 7.5% SDS-PAGE gels were used; 12.5% SDS-PAGEgels were used for Sec22p and Sec62p, and 15% SDS-PAGE gelswere used for cytochrome C. For the detection of FBPase, 3-oxoacylCoA thiolase, and Pep12p, 10% SDS-PAGE gels were used. Fractionsare shown from 16–30.

Sucrose Equilibrium Gradients
Wild-type cells were shifted to glucose for 0, 30, 60, or 90min at 22°C. Fractions 25–30 were pooled from theS-1000 columns and centrifuged at 100,000 g for 4 h. The pelletswere resuspended in 0.5 ml of TEA buffer and loaded onto thetop of 20–50% sucrose gradients. The gradients were preparedby adding 3 ml of 50% sucrose, 3 ml of 40% sucrose, 3 ml of30% sucrose, and 2 ml of 20% sucrose sequentially. Sampleswere centrifuged at 100,000 g for 20 h at 4°C using a SorvallTH 641 rotor (Sorvall Instruments Division, DuPont Co., Newton,CT). Samples were collected from the top (0.8 ml), precipitatedwith TCA, and processed as described above. Proteins were resolvedon SDS-PAGE gels and detected by immunoblotting with antibodiesspecific to organelle markers and FBPase.

Electron Microscopy
Fractions 25–30 were pooled from the S-1000 columns andseparated on two sequential 20–50% sucrose gradients.Vesicles were isolated from the second sucrose gradient (fractions10 and 11) and examined directly by EM. Samples (5 µl)were adsorbed to a carbon-coated grid that was made hydrophilicby a 30-s exposure to a glow discharge in an Auto 306 vacuum evaporator (Edwards High Vacuum, Inc., Grand Island, NY). Aftera brief rinse with water to wash away excess sucrose, the sampleswere stained with 1% uranyl acetate for 1 min. The grids wereexamined using a 1200 EX transmission electron microscope (JEOLUSA, Peabody, MA). Micrographs were recorded at magnificationsof 40,000 or 60,000.

Proteinase K Treatment
The titration of proteinase K was performed using isolated vesicles(50 µg) incubated with increasing amounts of proteinaseK in the absence or presence of 2% Triton X-100 for 30 min onice. Proteinase K was added at the concentration of 0, 0.5,1, 1.5, 2, or 2.5 mg/ml in 100-µl reaction mixtures. Reactions were terminated by adding 10% TCA and processed asdescribed. To determine the time course of proteinase K sensitivity,vesicles (50 µg) were isolated from the sucrose gradientand treated with or without proteinase K (2 mg/ml) in the absenceor presence of 2% Triton X-100 for 0, 10, 20, 30, or 40 minon ice. Reactions (100 µl) were terminated by adding10% TCA, and samples were processed as described above. FBPasewas detected by immunoblotting. The 75-kD protein was detected by staining with Coomassie blue.

Results

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Abstract
Materials and Methods
Results
Discussion
References

FBPase Is Associated with Intracellular Structures after Glucose Shift
We investigated whether FBPase was associated with intracellularstructures in wild-type cells. Since the association may occurrapidly at 30°C, cells were shifted to glucose at 22°C,based on our earlier observation that FBPase targeting to thevacuole is delayed at this temperature. Wild-type cells wereshifted to glucose for 0, 30, 60, or 90 min at 22°C. Cellswere homogenized and centrifuged to obtain high speed pellets.The pellets were further fractionated on Sephacryl S-1000 columnsto separate intracellular organelles based on size. The distributionof FBPase on the S-1000 columns was followed by immunoblotting with anti-FBPase antibodies. We showed previously that FBPasewas found in two distinct peaks on the S-1000 columns in vidmutants (Hoffman and Chiang, 1996). A similar distribution ofFBPase was also found in wild-type cells. It remains to bedetermined whether two types of vesicles are involved in theFBPase degradation pathway; we focused on the second FBPasepeak and attempted to purify the vesicles from the second peak.Kinetic studies show that, at t = 0 min, very little FBPasewas detected on the S-1000 columns in wild-type cells (Fig.1 a). However, 30 min after glucose shift, FBPase appearedin fractions 26–30 (Fig. 1 b). The amount of FBPase wasfurther increased at t = 60 min (Fig. 1 c), and then decreasedat t = 90 min (Fig. 1 d). Under the same conditions, the amountof the vacuolar CPY was constant before and after glucose shift (Fig. 1, e–h).

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Figure 1 Glucose induces FBPase association with intracellular structures. Wildtype cells were shifted to 2% glucose for 0, 30, 60, and 90 min at 22°C. Cells were homogenized and centrifuged, and the high speed pellets were separated on S-1000 columns as described (Hoffman and Chiang, 1996). The second FBPase peak was analyzed (fractions 16–30). Aliquots from each fraction were TCA precipitated, washed, and electrophoresed on SDS-PAGE gels. Proteins were blotted onto nitrocellulose membranes. The positions of FBPase and CPY at t = 0, 30, 60, or 90 min were followed by ECL reactions with anti-FBPase (a–d) and anti-CPY antibodies (e–h).

Organelle Distribution on the S-1000 Columns
We examined the distribution of FBPase and organelles by immunoblottingwith antibodies directed against FBPase and organelle markers.We used CPY for the vacuole (Hasilik and Tanner, 1978; Hemmings et al., 1981;Rothman and Stevens, 1986; Banta et al., 1988; Jones, 1991)and Sec62p, an integral membrane on the ER membrane, for theER (Deshaies and Schekman, 1989, 1990). To detect the Golgicomplex, we used antibodies produced against Mnn1p ( ${alpha}$ -1,3-mannosyltransferase),a membrane protein that marks the medial Golgi compartment(Graham et al., 1994). We determined the positions of peroxisomesand mitochondria by using antibodies directed against 3-oxoacylCoA thiolase for peroxisomes, and cytochrome C for mitochondria.The plasma membrane was detected by the distribution of theplasma membrane ATPase (Pma1p). We also examined the positionsof transport vesicles by immunoblotting techniques. The COPIvesicles are involved in the retrograde and anterograde transportbetween the ER and the Golgi in yeast (Barlowe et al., 1994; Letourneur et al., 1994; Bednarek et al., 1995). These vesicleswere detected by antibodies directed against Sec21p (Bednarek et al., 1995).The ER-derived COPII vesicles were identified using antibodiesproduced against Sec22p (Barlowe et al., 1994; Bednarek et al., 1995).Endosomes were followed by immunoblotting of fractions withantibodies raised against Pep12p, a syntaxin homologue requiredfor sorting of luminal hydrolases to the vacuole (Becherer et al., 1996).Total protein profile was visualized by Coomassie blue staining.

Fig. 2 shows that, on the S-1000 columns, the fractions containingFBPase also contained most organelles such as the vacuole (CPY),ER (Sec62p), Golgi (Mnn1p), peroxisomes (3-oxoacyl CoA thiolase),and mitochondria (cytochrome C) (Fig. 2, a–f). Fractions26–30 also contained the COPI vesicles (Sec21p) and theCOPII vesicles (Sec22p) (Fig. 2, h and i). The FBPase-containingfractions showed some overlap with the endosomal marker Pep12p(Fig. 2 j). The plasma membrane ATPase (Pma1p) was partitionedprimarily in early fractions (Fig. 2 g). Protein staining demonstratedthat most proteins were distributed in fractions 25–30(Fig. 2 k). Therefore, FBPase overlaps significantly with manyorganelles on the S-1000 columns, with the exception of theplasma membrane marker Pma1p.

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Figure 2 Organelle distribution on the S-1000 columns. The distributions of FBPase and organelles were followed by immunoblotting with antibodies specific to the organelles. CPY for the vacuole (61 kD, b), Sec62p for the ER (30 kD, c), Mnn1p for the Golgi (106 kD, d), 3-oxoacyl CoA thiolase for peroxisomes (45 kD, e), cytochrome C for mitochondria (13 kD, f), Pma1p for the plasma membrane (106 kD, g), Sec21p for COPI vesicles (105 kD, h), Sec22p for COPII vesicles (24 kD, i), and Pep12p for endosomes (35 kD, j). Total protein was monitored by Coomassie blue R-250 staining (k). The cells had been shifted to glucose for 30 min.

Transient Association of FBPase with Dense Structures
To purify the FBPase vesicles, fractions 25–30 from the S-1000 columns were pooled and recentrifuged. High speed pelletswere centrifuged to equilibrium on 20–50% sucrose densitygradients. The positions of FBPase and CPY after glucose shiftwere detected by immunoblotting with antibodies directed againstFBPase and CPY. The kinetics of FBPase distribution in responseto glucose is shown in Fig. 3, a–d. FBPase was undetectableon the sucrose gradients at t = 0 min (Fig. 3 a); the amountwas increased at t = 30 min (Fig. 3 b). On the sucrose gradients, the FBPase antigen was in fractions 10–12, which correspondsto a density of $~$ 1.22 g/cm³. At t = 60 min, two peaks of FBPasewere found; one was in fractions 9–12, the other in fractions1–5 (Fig. 3 c). At t = 90 min, FBPase disappeared fromfractions 9–12; a smaller amount of FBPase was foundin fractions 2–5 (Fig. 3 d). In contrast with FBPase,the distribution of CPY was not affected by glucose (Fig. 3,e–h), nor the amount of CPY altered by the addition ofglucose for up to 90 min. Thus, FBPase distribution to highdensity fractions 9–12 is induced by glucose, occurs onlytransiently, and precedes the association with the vacuole.

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Figure 3 Transient association of FBPase with dense structures on the sucrose gradients. Wild-type cells were shifted to glucose for 0, 30, 60, or 90 min at 22°C. Fractions 25–30 were pooled from the S-1000 columns and centrifuged. The pellets were resuspended, loaded onto the top of 20–50% sucrose gradients, and centrifuged at 100,000 g for 20 h. Samples were collected from the top and treated as described in Materials and Methods. The positions of FBPase and CPY at t = 0, 30, 60, or 90 min were followed by immunoblotting with anti-FBPase (a–d) and CPY antibodies (e–h) using ECL reactions.

Purification of the FBPase-associated Vesicles
FBPase was associated transiently with high density structureson the sucrose density gradients. To determine which organellesFBPase was associated with, we examined the distribution oforganelle markers and FBPase in a sucrose gradient using immunoblottingwith antibodies directed against organelle markers and FBPase.Since FBPase was found in the denser part of the sucrose gradients,the sucrose gradients were designed to separate the FBPase peak away from most organelles. Fig. 4 shows that most organelleswere distributed in earlier fractions on the sucrose gradients.The vacuole (CPY), ER (Sec62p), Golgi (Mnn1p), peroxisomes(3-oxoacyl CoA thiolase), mitochondria (cytochrome C), COPI(Sec21p) and COPII (Sec22p) vesicles, and endosomes (Pep12p)were all found in early fractions (Fig. 4, b–i). Coomassie-stainedgels showed that most proteins were distributed in the first eight fractions; smaller amounts of proteins were found in the FBPase-containing fractions 9–12 (Fig. 4 j).

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Figure 4 Organelle distribution on the sucrose gradients. Wildtype cells were shifted to glucose for 30 min. Fractions 25–30 from t = 30 min were pooled from the S-1000 columns and resolved on 20–50% sucrose equilibrium gradients. The distributions of various organelles were detected by immunoblotting with antibodies directed against organelle markers described in Fig. 2. Total protein was visualized by staining with Coomassie blue R-250 (j).

Although the sucrose gradient was not optimal to separate mostintracellular organelles apart, it did separate the FBPasepeak from most organelles (Fig. 4). To minimize the contaminationof minor proteins that might be trailed off from other fractions,the FBPase-containing fractions (fractions 10 and 11) fromthe first sucrose gradient were pooled and refractionated ona second 20–50% equilibrium sucrose gradient. Proteinswere separated by SDSPAGE gel electrophoresis and stained withCoomassie blue. Fig. 5 shows that several protein bands wereenriched in the FBPase-containing fractions 10 and 11 on the second sucrose gradient, as compared with the protein patternsobtained from the S-1000 column (Fig. 2 k), or the first sucrosegradient (Fig. 4 j). When organelle markers were assayed, FBPasewas the only marker that appeared in fractions 10 and 11; theother organelle markers were undetectable on the second sucrosegradient (not shown).

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Figure 5 Protein staining on the second sucrose gradient. Fractions 10 and 11 from the first sucrose gradient were pooled, pelleted at high speed, and recentrifuged on a second equilibrium sucrose gradient. Fractions were collected from the top and processed as described. Proteins were separated by electrophoresis on 10% SDS-PAGE gels and stained by Coomassie blue R-250.

The purity of the FBPase-associated structures was examinedby EM. Fractions 10 and 11 from the second sucrose gradientwere isolated, stained with uranyl acetate, and visualizedby transmission electron microscopy. A homogeneous populationof vesicles of 30–40 nm in diam was found by EM (Fig.6, a and b). At higher magnification, these vesicles appearto be surrounded by a layer of membrane (Fig. 6 b). Since verylittle contamination of other structures was found under EM,these vesicles have been purified to near homogeneity. TableI summarizes the purification procedure for the isolation ofthe 30–40-nm vesicles from 10 liters of wild-type yeastculture. After differential centrifugation at 100,000 g andsubsequent separation on the S-1000 columns, 4.2% of the proteinswere recovered. Upon further purification on two sequentialsucrose gradients, 0.1% of the proteins were recovered. Vesiclesof the same size and protein composition have also been purifiedfrom a vid mutant (not shown).

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Figure 6 Electron micrograph of purified vesicles. Vesicles were isolated from the second sucrose gradient (fractions 10 and 11). Samples (5 µl) were adsorbed to a carbon-coated grid and examined using a JEOL 1200 EX transmission electron microscope. Bars: (a) 200 nm; (b) 100 nm.

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Table I Scheme for the Purification of the 30–40-nm Vesicles

FBPase Is Sequestered inside the Vesicles
FBPase is localized in the cytosol before transfer of cellsto glucose (Chiang and Schekman, 1991; Chiang et al., 1996). In the cytosol, FBPase is sensitive to proteinase K digestion(Chiang and Schekman, 1991). If these vesicles function as carriersto deliver FBPase to the vacuole for degradation, FBPase mightenter the lumen of the vesicles. To determine whether thiswas the case, we performed proteinase K experiments. If FBPasewas sequestered inside the vesicles, FBPase would be resistantto proteinase K digestion. By contrast, if FBPase was associatedwith the vesicles peripherally, FBPase would be sensitive toproteinase K digestion. Since FBPase was the only marker to detect the vesicles, we followed total protein bands by staininggels with Coomassie blue, before and after proteinase K treatment.We found that the 75-kD protein that copurified with FBPaseserved as a useful control, since the 75-kD protein was readilydigested by proteinase K. Fig. 7 a shows that the 75-kD proteinwas digested by proteinase K at concentrations ranging from0.5–2.5 mg/ml (Fig. 7 a, lanes 1–6); the sensitivitywas not affected whether or not Triton X-100 was present (Fig.7 a, lanes 7–12). By contrast, FBPase was stable whenincubated with 0.5–2.5 mg/ml proteinase K in the absenceof Triton X-100 (Fig. 7 a, lanes 1–6). However, when2% Triton X-100 was added to solubilize the membranes, FBPasebecame sensitive to proteinase K; it was digested completely by proteinase K at a concentration as low as 0.5 µg/ml (Fig. 7 a, lanes 7–12).

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Figure 7 FBPase is sequestered inside the vesicles. (a) Isolated vesicles (50 µg) were incubated with increasing amounts of proteinase K in the absence (lanes 1–6) or presence of 2% Triton X-100 (lanes 7–12) for 30 min on ice. Proteinase K was added at the concentration of 0, 0.5, 1, 1.5, 2, or 2.5 mg/ml in 100-µl reaction mixtures. Reactions were terminated by adding 10% TCA and processed as described. FBPase was detected by immunoblotting. The 75-kD protein was detected by staining with Coomassie blue R-250. (b) Vesicles (50 µg) isolated from the sucrose gradient were incubated with or without proteinase K (2 mg/ml) in the absence or presence of 2% Triton X-100 on ice for 0, 10, 20, 30, or 40 min. Reactions (100 µl) were terminated by adding 10% TCA, and samples were processed as described above. (Lanes 1–5) Without proteinase K, without Triton X-100. (Lanes 6–10) Without proteinase K, with Triton X-100. (Lanes 11–15) With proteinase K, without Triton X-100. (Lanes 16–20) With proteinase K, with Triton X-100.

We determined the time course of proteinase K sensitivity inthe presence or absence of Triton X-100. Isolated vesicleswere incubated with or without 2 mg/ml proteinase K for 0–40min on ice in the absence or presence of 2% Triton X-100. Wefound that FBPase was stable in the absence of proteinase Kfor up to 40 min (Fig. 7 b, lanes 1–10). FBPase remainedresistant to proteinase K in the absence of Triton X-100 (Fig.7 b, lanes 11–15). It became sensitive to proteinaseK when Triton X-100 was added to solubilize the membranes (Fig.7 b, lanes 16–20); most FBPase was digested within 10min of treatment of proteinase K. The 75-kD protein was digestedwithin 10 min by proteinase K, either in the absence or thepresence of Triton X-100 (Fig. 7 b, lanes 11–20). Theseresults suggest that FBPase was sequestered inside the vesicles,and the 75-kD protein was not.

Discussion

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Abstract
Materials and Methods
Results
Discussion
References

We provide evidence for the importance of novel vesicles inthe degradation of the regulatory enzyme, FBPase, after transferof wild-type cells from poor carbon sources to glucose. We havepurified one type of FBPase-associated vesicles of 30–40nm in diam to near homogeneity. Kinetic studies indicate thatFBPase association with the vesicles is induced by glucoseand disappears as FBPase is delivered to the vacuole for degradation.These vesicles are distinct from the vacuole, peroxisomes,mitochondria, ER, Golgi, endosomes, COPI, or COPII vesiclesas shown by fractionation experiments. Morphological analysisalso demonstrates that the FBPase-associated vesicles are smaller than the early or late endosomes that are 100–400 nmin diam (Singer-Kruger et al., 1993), the COPI or COPII vesiclesthat are 50 nm in diam (Kaiser and Schekman, 1990; Bednarek et al., 1995),or the post-Golgi vesicles that are 100 nm in diam (Walworth and Novick, 1987).

A substantial amount of FBPase is sequestered inside the vesicles30 min after transfer of wild-type cells to glucose. If FBPasebinds to the surface of the 30–40-nm vesicles first andthen enters the lumen of the vesicles, it might be possibleto enrich for the vesicles containing FBPase on the surfaceusing mutants defective in FBPase degradation. The vesiclesmight fuse with the vacuole. After fusion, the sequestered FBPasecould be released directly into the lumen of the vacuole fordegradation. If a small amount of FBPase is present on thesurface of the vesicles, after fusion, FBPase would be distributedon the vacuolar membrane. The membrane-bound FBPase could thenbe internalized by autophagy. Cloning of VID genes and studiesof vid mutants may shed light onto the mechanisms of the FBPasedegradation pathway.

Acknowledgments

We thank Maria Ericsson for performing EM work, Kathleen J.Barrett for editing this manuscript, and members in the Chianglaboratory for helpful discussions.

This work was supported by American Cancer Society grant BE-212A to H.-L. Chiang.

Submitted: 2 October 1996

Revised: 10 December 1996

Address all correspondence to Hui-Ling Chiang, Department ofCell Biology, Harvard Medical School, 240 Longwood Avenue, Boston,MA 02115. Tel. and Fax: (617) 432-0140. e-mail: chiangne{at}warren.med.harvard.edu

References

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Abstract
Materials and Methods
Results
Discussion
References

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