Transport of Storage Proteins to Protein Storage Vacuoles Is Mediated by Large Precursor-Accumulating Vesicles

Correspondence to: Ikuko Hara-Nishimura, ihnishi{at}nibb.ac.jp (E-mail), 81-564-55-7505 (fax).

	ABSTRACT

TOP ABSTRACT INTRODUCTION RESULTS DISCUSSION METHODS REFERENCES

Novel vesicles that accumulate large amounts of proprotein precursors of storage proteins were purified from maturing pumpkin seeds. These vesicles were designated precursor-accumulating (PAC) vesicles and had diameters of 200 to 400 nm. They contained an electron-dense core of storage proteins surrounded by an electron-translucent layer, and some vesicles also contained small vesicle-like structures. Immunocytochemical analysis revealed numerous electron-dense aggregates of storage proteins within the endoplasmic reticulum. It is likely that these aggregates develop into the electron-dense cores of the PAC vesicles and then leave the endoplasmic reticulum. Immunocytochemical analysis also showed that complex glycans are associated with the peripheral region of PAC vesicles but not the electron-dense cores, indicating that Golgi-derived glycoproteins are incorporated into the PAC vesicles. These results suggest that the unique PAC vesicles might mediate a transport pathway for insoluble aggregates of storage proteins directly to protein storage vacuoles.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION RESULTS DISCUSSION METHODS REFERENCES

Higher plants have two types of vacuoles. One type, protein storage vacuoles, develops mainly in storage organs, such as seeds, and the other type, lytic (vegetative) vacuoles, which contain various lytic enzymes, develops in the vegetative organs. Both types of vacuoles, however, are found in the same cells of barley roots (Okita and Rogers 1996 ; Paris et al. 1996 ) and of maturing pea cotyledons (Robinson et al. 1995 ). In these cells, vacuolar proteins synthesized on the rough endoplasmic reticulum (RER) are sorted and delivered to their respective vacuoles. Thus, different targeting machineries for each type of vacuole must be involved in the protein transport in these cells.

Kirsch et al. 1994 demonstrated that the clathrin-coated vesicles contain a potential receptor for a precursor of barley aleurain, which is a thiol proteinase. This implicated these vesicles in the transport of the proteinase precursor to lytic vacuoles. On the other hand, clathrin-coated vesicles isolated from maturing pea cotyledons contain no seed protein precursors (Hohl et al. 1996 ). Thus, the clathrin-coated vesicles may mediate the transport of lytic vacuolar proteins but not the transport of seed proteins to protein storage vacuoles. This raises the question of how seed proteins are sorted and delivered to protein storage vacuoles in the cells of maturing seeds.

Most storage proteins, including globulins and some prolamins, have been shown to be transported to protein storage vacuoles via the Golgi apparatus (Chrispeels 1985 ; Shotwell and Larkins 1988 ). Chrispeels 1983 reported the presence of electron-dense vesicles close to the Golgi stacks in maturing bean cotyledons. Recently, Hohl et al. 1996 demonstrated immunocytochemically in maturing pea cotyledons that electron-dense vesicles with a diameter of ~100 nm associated with any cis, medial, and trans cisternae of the Golgi apparatus contain storage proteins. These results suggest that the storage proteins are transported to protein storage vacuoles via the Golgi-derived dense vesicles. However, a Golgi-independent pathway for storage proteins has also been reported. Levanony et al. 1992 reported that wheat prolamins are transported to the protein storage vacuoles without any contribution by the Golgi apparatus. However, the mechanism responsible for such Golgi-independent transport has not been characterized or determined.

Cell fractionation of pulse–chase—labeled maturing seeds of pumpkin and castor bean has demonstrated that both proglobulin (Hara-Nishimura et al. 1985 ; Fukasawa et al. 1988 ) and pro2S albumin (Hara-Nishimura et al. 1993a ) are transported from the RER to the protein storage vacuoles via the vesicles having a density of 1.24 g/cm³. At the protein storage vacuoles, the precursors are converted to their mature forms (Hara-Nishimura and Nishimura 1987 ). This suggests that the vesicles with a density of 1.24 g/cm³ mediate the transport of major storage proteins to protein storage vacuoles in maturing seeds of pumpkin and castor bean. However, the origin of these vesicles remains unknown. The ultrastructure of these vesicles, which includes an electron-dense core surrounded by electron-translucent structures, is distinct from the ultrastructures of the clathrin-coated vesicles (Robinson 1996 ) and Golgi-derived vesicles (Hohl et al. 1996 ) in pea cotyledons.

Immunoelectron microscopy showed that electron-dense aggregates of storage proteins are present within the RER. This suggests that the vesicles with a density of 1.24 g/cm³ might be derived directly from the protein aggregates in the RER. If this is true, then it is unclear how seed proteins with complex glycans, such as ricin of castor bean, are transported to the protein storage vacuoles, because complex glycans would not be expected to originate in the RER. In this study, we prepared biochemically and electron microscopically pure vesicles from maturing pumpkin seeds and characterized them to answer the question of how seed protein precursors are accumulated in the vesicles to be delivered to protein storage vacuoles. We show here a unique transport pathway provided by the vesicles that we have designated as precursor-accumulating (PAC) vesicles.

	RESULTS

TOP ABSTRACT INTRODUCTION RESULTS DISCUSSION METHODS REFERENCES

Ultrastructural Analysis and Isolation of a Novel Transport Vesicle for Storage Proteins
Previously, we demonstrated that vesicles with a density of 1.24 g/cm³ mediate the transport of proprotein precursors of two major storage proteins, namely, proglobulin and pro2S albumin, from the RER to protein storage vacuoles in maturing seeds of pumpkin (Hara-Nishimura et al. 1985 , Hara-Nishimura et al. 1993a ) and castor bean (Fukasawa et al. 1988 ). To characterize these vesicles, we performed an ultrastructural analysis of pumpkin cotyledons at the middle stage of seed maturation. Electron microscopy of the cotyledons revealed numerous electron-dense vesicles ~300 to 400 nm in diameter in the cells, as indicated by arrowheads in Figure 1A. These vesicles are much larger than the clathrin-coated vesicles (Robinson 1996 ), with diameters of 50 to 70 nm, and Golgi-derived dense vesicles, with diameters of ~100 nm (Hohl et al. 1996 ). The vesicles were frequently observed close to the well-developed RER, and some were surrounded by ribosomes in the cotyledon cells at the middle stage of seed maturation (Figure 1B).

View larger version (109K): [in this window] [in a new window]   Figure 1. Electron Microscopy of Pumpkin Cotyledons at the Middle Stage of Seed Maturation. (A) Numerous PAC vesicles (PV, arrowheads) ~300 to 400 nm in diameter are visible in the cell. PAC vesicles contain an electron-dense core that is surrounded by an electron-translucent layer. (B) An electron-dense vesicle surrounded by ribosomes can be seen close to the ER in the cell. Immunoelectron microscopy with 2S albumin–specific antibodies shows that the vesicle was also labeled with gold particles. (C) Immunoelectron microscopy with 11S globulin–specific antibodies shows that gold particles are distributed on the electron-dense area of PAC vesicles (PV). Gold particles are also visible on a protein storage vacuole. The labeling density of the vesicles is similar to that of the protein storage vacuoles. CW, cell wall; ER, endoplasmic reticulum; Lb, lipid body; Mt, mitochondrion; P, plastid; V, protein storage vacuole. Bars in (A) to (C) = 500 nm.

Electron microscopy after immunogold labeling with 11S globulin–specific antibodies revealed gold particles on the vesicles as well as on the protein storage vacuoles (Figure 1C), which contain large amounts of 11S globulin, the most abundant storage protein. Immunocytochemistry with 2S albumin–specific antibodies gave a similar result (Hara-Nishimura et al. 1993a ). The gold particles were distributed uniformly on the electron-dense area of the vesicles, and the labeling density of the vesicles was similar to that of the protein storage vacuoles (Figure 1C).

To characterize the vesicles in greater detail, we isolated them from maturing pumpkin cotyledons by centrifugation on a self-generated Percoll gradient. The vesicles formed one band in the Percoll gradient. Further centrifugation of the isolated vesicles on a sucrose density gradient revealed a density of 1.24 g/cm³. This indicated that the purified vesicles are identical to those found in the previous pulse–chase experiments with the maturing seeds of pumpkin (Hara-Nishimura et al. 1985 , Hara-Nishimura et al. 1993a ) and castor bean (Fukasawa et al. 1988 ).

Figure 2A shows electron microscopy of the isolated vesicles. Microscopy revealed that the vesicle fraction was not contaminated with any other organelles or any microsomal membranes. The vesicles had the same diameter as those observed in the cells. They had a characteristic structure, with an electron-dense core surrounded by an electron-translucent layer. Some vesicles contained small electron-translucent vesicle–like structures, and the content of the vesicle-like structures was observed to be higher in the vesicles of the younger cotyledons (data not shown). Immunoelectron microscopy of the isolated vesicles with specific antibodies raised against either 11S globulin or 2S albumin revealed that electron-dense cores of all the vesicles were labeled uniformly with gold particles, as shown in Figure 2B and Figure 2C. This result indicates clearly that both 11S globulin and 2S albumin are localized in the electron-dense core of the vesicles.

View larger version (77K): [in this window] [in a new window]   Figure 2. Ultrastructures of Isolated PAC Vesicles and Immunolocalization of Storage Proteins in the Vesicles. (A) Highly purified PAC vesicles from pumpkin cotyledons at the middle stage of seed maturation after centrifugation on a self-generated Percoll gradient. PAC vesicles contain electron-dense cores that are surrounded by an electron-translucent layer and/or small electron-translucent vesicles. The PAC vesicle fraction was not contaminated with other cellular components. (B) Immunoelectron microscopy of isolated PAC vesicles with 11S globulin–specific antibodies. Electron-dense cores of all of the vesicles are labeled uniformly with gold particles. (C) Immunoelectron microscopy of vesicles with 2S albumin–specific antibodies. Electron-dense cores of all the vesicles are uniformly labeled with gold particles. Bars in (A) to (C) = 500 nm.

PAC Vesicles Are Packed with a Significant Amount of Proprotein Precursors of Storage Proteins
Our previous study showed that maturation of storage proteins occurs in protein storage vacuoles by the action of a vacuolar processing enzyme (Hara-Nishimura and Nishimura 1987 ; Hara-Nishimura et al. 1993a ). Therefore, if it is true that the vesicles with a density of 1.24 g/cm³ function as the transport vesicles for storage proteins to the protein storage vacuoles, then the vesicles should contain proprotein precursors of storage proteins but not mature proteins.

To examine the protein composition of the vesicles, we subjected the pure vesicle preparation to SDS-PAGE and then either to staining with Coomassie blue or to immunoblotting with specific antibodies against each of three major storage proteins. Figure 3 shows that the vesicles accumulated considerable amounts of three proteins that stained with Coomassie blue (lane 2). The immunoblot showed that these proteins corresponded to proprotein precursors of 11S globulin (lane 3), 2S albumin (lane 4), and the 51-kD protein (lane 5), respectively. No mature forms of these proteins were detected in the vesicles, indicating that the vesicle fraction was not contaminated by protein storage vacuoles. Thus, the vesicles accumulate proprotein precursors of all the major storage proteins and transport them to protein storage vacuoles. Accordingly, the vesicles were designated PAC vesicles.

View larger version (44K): [in this window] [in a new window]   Figure 3. Accumulation of the Proprotein Precursors of All Major Storage Proteins of Pumpkin in PAC Vesicles. Isolated PAC vesicles were subjected to SDS-PAGE and subsequent staining with Coomassie blue (CBB; lanes 1 and 2) or immunoblot analysis (lanes 3 to 5). Lane 1 (M) contains molecular mass markers (labeled in kilodaltons at left); lane 2 (PV), isolated PAC vesicles; and lanes 3 to 5, immunoblots with antibodies raised against the specified protein. Lane 3 contains 11S globulin; lane 4, 2S albumin; and lane 5, the 51-kD protein. Labeling at right identifies the major protein components of PAC vesicles, which are all proprotein precursors to storage proteins: pro51-kD protein (p51kD), proglobulin (pG), and pro2S albumin (p2S).

The results indicate that the major storage proteins are transported to protein storage vacuoles via PAC vesicles. This raised the question of whether each PAC vesicle contains all three precursors that are to be transported or whether there are PAC vesicles that are specific to each storage protein. To answer these questions, we performed double immunogold labeling of the isolated vesicles by using protein A conjugated with gold particles 10 and 15 nm in diameter. Double immunogold labeling using specific antibodies raised against various pairs of storage proteins resulted in gold particles of both 10 and 15 nm in each PAC vesicle, as shown in Figure 4A to C. This finding strongly suggests that each PAC vesicle mediates the transport of all three major storage proteins of pumpkin.

View larger version (48K): [in this window] [in a new window]   Figure 4. Double Immunogold Labeling of the Isolated PAC Vesicles by Using Protein A Conjugated with Gold Particles of Different Sizes. (A) Immunolocalization of proglobulin (15-nm gold) and pro2S albumin (10-nm gold). (B) Immunolocalization of proglobulin (15-nm gold) and pro51-kD protein (10-nm gold). (C) Immunolocalization of pro2S albumin (15-nm gold) and pro51-kD protein (10-nm gold). Bar in (C) = 500 nm for (A) to (C).

The Electron-Dense Core of a PAC Vesicle Originates from a Storage Protein Aggregate That Is Formed within the ER
The next issue to be resolved was the origin of the PAC vesicles. Are they derived from the ER or the Golgi apparatus? Most storage proteins are actively synthesized in the cells of pumpkin cotyledons at the middle stage of seed maturation (Hara-Nishimura et al. 1987 ; Inoue et al. 1995a ). Ultrastructural analysis of the cells of maturing pumpkin cotyledons at this stage revealed that Golgi stacks are less in these cells, in contrast to the extensive development of the RER, as shown in Figure 1 and Figure 5.

View larger version (112K): [in this window] [in a new window]   Figure 5. Electron Microscopy of Maturing Pumpkin Cotyledons Showing Numerous Electron-Dense Aggregates within the ER. (A) Electron-dense core aggregates (arrows) formed within the ER in cells at the middle stage of seed maturation. The electron-translucent space between the aggregate and the ER membrane is loaded with ribosomes. PAC vesicles (PV) are also visible. (B) Immunoelectron microscopy with 2S albumin–specific antibodies. The aggregates within the ER (arrows) are labeled with gold particles. PAC vesicles (PV) and a protein storage vacuole (V) are also visible. CW, cell wall; Lb, lipid body. Bars in (A) and (B) = 500 nm.

Electron microscopy of pumpkin cotyledons at the middle stage revealed numerous electron-dense aggregates within the RER, as indicated by arrows in Figure 5A. Immunocytochemical analysis with 2S albumin–specific antibodies demonstrated that the ER aggregates contained 2S albumin, as shown in Figure 5B. Similar immunogold labeling of the ER aggregates with 11S globulin–specific antibodies was observed (data not shown), indicating that these ER aggregates are composed of both pro2S albumin and proglobulin. This result indicates that the proprotein precursors, which are synthesized and translocated into the lumenal side of the ER, form core aggregates. The diameters of the ER aggregates ranged from 100 to 300 nm, suggesting that the aggregates might increase in size by incorporating newly synthesized storage proteins in the lumen of the RER.

Most aggregates were not surrounded directly by the ER membrane. There was an electron-translucent space between each aggregate and the ER membrane, as indicated by arrows in Figure 5A and Figure 5B. The structure of the aggregates is analogous to that of the PAC vesicles, although the ER aggregates were smaller than the PAC vesicles. It seems possible that the aggregates might bud out of the ER to be transformed into PAC vesicles.

Golgi-Derived Glycoproteins Are Localized in the Peripheral Region of PAC Vesicles
The next question is whether the PAC vesicles are involved in a transport of storage proteins with complex glycans to protein storage vacuoles. Such glycoproteins must be passed through the Golgi apparatus so that their oligosaccharide chains can be modified. However, the major storage proteins of pumpkin, namely, 11S globulin and 2S albumin, are not glycosylated. Recently, we isolated a cDNA of the third major storage protein of pumpkin, the 51-kD protein. The cDNA encodes the 100-kD precursor with no possible N-linked glycosylation site (data not shown). Thus, it is not necessary for these pumpkin storage proteins to pass through the Golgi apparatus.

In contrast to pumpkin seeds, castor bean seeds contain glycoproteins, ricin, and Ricinus communis agglutinin, with complex glycans. Previously, we reported that 11S globulin of the maturing endosperm of castor bean, like pumpkin storage proteins, was transported from the ER to protein storage vacuoles via the vesicles with a density of 1.24 g/cm³ (Fukasawa et al. 1988 ). We also observed vesicles identical to pumpkin PAC vesicles in the endosperm cells of castor bean at the middle stage of seed maturation (Hiraiwa et al. 1993 ). Except for the glycoproteins, the compositions of soluble proteins and membrane proteins of castor bean protein storage vacuoles are similar to those of pumpkin (Inoue et al. 1995a , Inoue et al. 1995b ; Hiraiwa et al. 1997a ). Therefore, we used the endosperm of maturing castor bean seeds to study the transport pathway of glycoproteins.

We prepared complex glycan-specific antibodies that recognized mainly ricin and R. communis agglutinin (data not shown) and used them for immunocytochemical analysis. Immunoelectron microscopy revealed the presence of gold particles on the peripheral region of PAC vesicles but not on the electron-dense area of PAC vesicles, as shown in Figure 6A and Figure 6B. Gold particles were also distributed on the periphery of the protein deposits in a protein storage vacuole, a cell wall, and a Golgi stack. This result suggests that Golgi-derived glycoproteins might be incorporated into the mature PAC vesicles after the vesicles are released from the ER.

View larger version (134K): [in this window] [in a new window]   Figure 6. Immunoelectron Microscopy of Castor Bean Endosperm at the Middle Stage of Seed Maturation with Complex Glycan-Specific Antibodies. (A) Gold particles are visible at the peripheral region of the PAC vesicles (PV) but not inside the area of the PAC vesicles. A Golgi stack (G) and cell wall (CW) are also labeled with gold particles. (B) Gold particles are also visible on the peripheral region of PAC vesicles (PV) as well as on the peripheral region of storage protein deposits in a protein storage vacuole (V, arrows). Lb, lipid body. Bar in (B) = 500 nm for (A) and (B).

An ER-Resident Protein BiP Is Trapped in the ER Aggregates and Is Transported to Protein Storage Vacuoles via PAC Vesicles
To confirm that the storage protein cores of PAC vesicles are derived directly from the ER, we measured the content of BiP, an ER-resident molecular chaperone, in the vesicles. If BiP were detected in the vesicles, it would suggest that BiP is trapped in the protein aggregates of ER and then transported to the vesicles, as discussed by Levanony et al. 1992 . To compare the BiP content in vesicles with that in the ER, the ER was prepared from maturing pumpkin cotyledons by sucrose density gradient centrifugation. The specific activity of NADH–cytochrome c reductase, an ER marker enzyme, was 104 milliunits per mg of protein in the ER preparation. In contrast, no activity was detected in the isolated PAC vesicles by using this assay, indicating that the specific activity in the vesicles was estimated to be <0.3 milliunits per mg of protein. Thus, the isolated vesicles were barely contaminated with the ER. The ER and PAC vesicles (15 µg of protein each) were subjected to SDS-PAGE on a 5 to 20% gradient polyacrylamide gel with subsequent Coomassie blue staining. The protein composition of the PAC vesicles was different from that of the ER, as shown in Figure 7A (lanes 1 and 2).

View larger version (38K): [in this window] [in a new window]   Figure 7. Association of an ER-Resident Molecular Chaperone, BiP, with PAC Vesicles. (A) ER and PAC vesicles were subjected to SDS-PAGE and subsequent staining with Coomassie blue (CBB; lanes 1 and 2) or immunoblot analysis with pumpkin BiP-specific antibodies (anti-BiP; lanes 4 and 5). Lane 1 (E) contains the ER protein (15 µg of protein); lane 2 (PV), PAC vesicles (15 µg of protein); lane 3 (M), molecular mass markers (labeled in kilodaltons at left); lane 4 (E), ER protein (0.4 µg of protein); and lane 5 (PV), PAC vesicles (40 µg of protein). Arrowhead indicates BiP. (B) Immunogold labeling of isolated PAC vesicles with BiP-specific antibodies shows localization of BiP in PAC vesicles. ER and PAC vesicles were prepared from pumpkin cotyledons at the middle stage of seed maturation. Bar = 500 nm.

To examine the presence of BiP in the PAC vesicles, ER (0.4 µg of protein) and vesicles (40 µg of protein) were subjected to SDS-PAGE and subsequent immunoblotting with BiP-specific antibodies. The intensity of the BiP signal in the PAC vesicles was equal to that in the ER, as shown in Figure 7A (lanes 4 and 5). BiP content in the PAC vesicles, on the basis of the amount of protein, was ~1% of that in the ER. This result indicates that BiP is present at a significant level in the vesicles. This is supported by the results of the immunogold labeling analysis of vesicles with BiP-specific antibodies, as shown in Figure 7B. These results support the possibility that the electron-dense cores of the PAC vesicles might have been derived directly from the aggregates in the ER.

BiP found in PAC vesicles could be transported to protein storage vacuoles together with proprotein precursors of storage proteins. Further analysis was performed to determine how much BiP accumulated in protein bodies of dry seeds. Protein bodies have been shown to be directly converted from protein storage vacuoles at the late stage of seed maturation (Hara-Nishimura et al. 1987 ). We isolated protein bodies from dry pumpkin seeds by using glycerol, as described previously (Hara-Nishimura et al. 1982 ). The specific activity of NADH–cytochrome c reductase in the whole homogenate of the tissues was 0.29 milliunits per mg of protein, whereas the activity in the protein bodies was only 0.0028 milliunits per mg of protein. Thus, contamination of the protein bodies with the ER was estimated to be <1%.

Each 200 µg of protein of the whole homogenate and the protein bodies was subjected to SDS-PAGE and then to staining with Coomassie blue or immunoblot analysis with BiP-specific antibodies. Approximately 20% of the total amount of BiP in the whole homogenate was detected in the protein bodies, as shown in Figure 8A (lanes 5 and 6). A significant amount of BiP accumulated in the protein bodies. To examine the suborganellar localization of BiP, the protein bodies were separated further into a soluble fraction and an insoluble crystalloid that was composed of 11S globulin. Figure 8A shows that most of the BiP was located in the soluble matrix (lane 7) of the protein bodies but not in the crystalloid (lane 8). Immunocytochemical labeling of maturing pumpkin cotyledons with BiP-specific antibodies resulted in labeling of protein storage vacuoles with gold particles, as shown in Figure 8B and Figure 8C. This result supports the proposed association of BiP with the protein storage vacuoles. Taken together, these results suggest that BiP is trapped in the ER aggregates and is transported to protein storage vacuoles via PAC vesicles in the cells of maturing pumpkin cotyledons.

View larger version (50K): [in this window] [in a new window]   Figure 8. Association of BiP with Both Protein Bodies from Dry Pumpkin Seeds and Protein Storage Vacuoles in Maturing Pumpkin Seeds. (A) Protein bodies and the suborganellar fractions were subjected to SDS-PAGE and subsequent staining with Coomassie blue (CBB; lanes 1 to 4) or immunoblot analysis with pumpkin BiP-specific antibodies (anti-BiP; lanes 5 to 8). Lane 1 (W) contains whole protein (0.2 mg of protein) of dry seeds; lane 2 (PB), whole protein (0.2 mg of protein) of protein bodies; and lanes 3 (m) and 4 (c), suborganellar fractions of matrix and crystalloids of 11S globulin, respectively, prepared from protein bodies (0.2 mg of protein) by centrifugation. Lanes 5 to 8 show the results of the immunoblot analysis with BiP-specific antibodies (anti-BiP) of the same fractions as given for lanes 1 to 4. The arrowhead indicates BiP. G indicates 11S globulin subunits; 2S, 2S albumin; and 51kD, the 51-kD protein. (B) and (C) Immunoelectron microscopy of pumpkin cotyledons at the middle stage of seed maturation with anti-BiP antibodies shows localization of BiP together with storage proteins in protein storage vacuoles (V). Lb, lipid body; arrowheads, endoplasmic reticulum. Bars = 1 µm.

	DISCUSSION

TOP ABSTRACT INTRODUCTION RESULTS DISCUSSION METHODS REFERENCES

Formation of Core Aggregates of Storage Protein Precursors within the ER
Proprotein precursors of storage proteins are synthesized on the RER and translocated into the lumenal side of the RER. There, they might form core aggregates, similar to those shown in Figure 5A and Figure 5B. Active synthesis of storage proteins might facilitate formation of protein aggregates within the ER. We previously demonstrated that trimeric oxidized proglobulin molecules are produced within the ER (Hara-Nishimura et al. 1985 ; Hara-Nishimura 1987 ) and that the increased accumulation of storage proteins parallels the increase in the amount of BiP during seed maturation of pumpkin (Hatano et al. 1997 ). It seems likely that BiP might play some role in the formation of the aggregates in the ER of pumpkin cotyledons. Li et al. 1993 showed that BiP retains prolamins, alcohol-soluble storage proteins, in the lumen of the ER by facilitating their folding and assembly into protein bodies of rice. In the case of rice (Okita and Rogers 1996 ) and maize (Larkins and Hurkman 1978 ), prolamin aggregates that are formed within the ER are converted directly to protein bodies but are not transported to protein storage vacuoles.

The electron-dense aggregate structures surrounded by a ribosome-studded membrane also were observed in maturing pea cotyledons (Craig 1988 ). The ER-derived aggregates of pea should be transported to the protein storage vacuoles. However, the mechanism of transport is unknown. Levanony et al. 1992 reported that the wheat prolamin aggregates forming in the ER might be transported to the vacuoles, bypassing the Golgi apparatus, via protein bodies that are surrounded by electron-translucent vesicles. These protein bodies could be structurally analogous to the PAC vesicles in pumpkin, even though the protein components are different in each case: the wheat aggregates are composed of insoluble prolamin, and the pumpkin aggregates are composed of proglobulin and pro2S albumin. It seems likely that the PAC vesicles are targeted to protein storage vacuoles by a mechanism similar to that for the wheat protein bodies. These results suggest that plant cells might have a common machinery for the delivery of protein aggregates produced within the ER to the vacuoles.

PAC Vesicle–Mediated Transport of Storage Proteins to Protein Storage Vacuoles
Robinson and Hinz 1996 reported that a type of pea protein body, PB₃, has a density of 1.19 to 1.22 g/cm³ and might contain a proprotein precursor of legumin. They also reported that PB₃ is formed at the late stage of pea seed maturation and is derived from the cisterna, whose origin is unclear. These characteristics of pea PB₃ are similar to those of PAC vesicles. PAC vesicles, like pea PB₃, are observed more frequently in the cotyledon cells at the later stage of pumpkin seed maturation (data not shown). The increase in the number of PAC vesicles might be correlated with the disappearance of Golgi stacks in the cell from the middle to late stages of seed maturation.

PAC vesicle–mediated transport of aggregates implies the existence of a Golgi-independent pathway for storage proteins in maturing pumpkin cotyledons. This is supported by our previous results with maturing pumpkin cotyledons treated with the carboxylic ionophore monensin (Hayashi et al. 1988 ). Monensin has been reported to inhibit Golgi-dependent transport of -amylases in the rice scutellum cells (Mitsui et al. 1985 ) and in the barley aleurone cells (Heupke and Robinson 1985 ). However, monensin did not inhibit the transport of proglobulin into protein storage vacuoles at the middle stage of pumpkin seed maturation (Hayashi et al. 1988 ). This result indicates that at this stage, proglobulin synthesized on the RER is transported to the vacuoles, bypassing the Golgi apparatus. The majority of storage proteins in pumpkin are not glycosylated and need not pass through the Golgi apparatus. A pathway bypassing the Golgi apparatus is presumed to have evolved for the efficient transport of unglycosylated proteins in maturing seeds that synthesize a large amount of storage proteins. On the other hand, glycoproteins of castor bean seeds that pass through the Golgi apparatus can be incorporated into the mature PAC vesicles and then transported to protein storage vacuoles together with the other storage proteins (Figure 6). Further analysis of the sorting of storage proteins with or without complex glycans will give us a detailed mechanism of the vacuolar targeting machineries in maturing seeds.

Multiple Transport Pathways for Vacuolar Proteins to Protein Storage Vacuoles
Elucidation of these machineries for the targeting of proteins to protein storage vacuoles requires biochemical analyses of isolated vesicles. Recently, we found two homologous proteins, PV72 and PV82, in the membrane fraction of isolated PAC vesicles and showed that PV72 and PV82 bind to peptides derived from pumpkin pro2S albumin (Shimada et al. 1997 ). Both PV72 and PV82 are type I integral membrane proteins with epidermal growth factor–like motifs and homologs of a potential vacuolar targeting receptor in pea, BP-80 (Paris et al. 1997 ), and an epidermal growth factor receptor–like protein in Arabidopsis, AtELP (Ahmed et al. 1997 ). Further investigations of the PV72 and PV82 proteins should help us to clarify the molecular mechanisms responsible for sorting within the cisternae of ER and/or Golgi apparatus.

Most proprotein precursors of storage proteins are converted into their respective mature forms by the action of the vacuolar processing enzyme after arrival at protein storage vacuoles (Hara-Nishimura et al. 1993a , Hara-Nishimura et al. 1995 ). We have shown that protein storage vacuoles contain the vacuolar processing enzyme (Hara-Nishimura et al. 1993b , Hara-Nishimura et al. 1995 ; Shimada et al. 1994a ) as well as an aspartic proteinase (Hiraiwa et al. 1997a ). This raises the question of how such hydrolytic enzymes are incorporated into protein storage vacuoles. We previously reported that the precursor of the vacuolar processing enzyme is localized in PAC vesicles in maturing castor bean endosperm (Hiraiwa et al. 1993 ) and is converted self-catalytically to an active enzyme after incorporation into the vacuoles (Hiraiwa et al. 1997b ). However, we could not detect the aspartic proteinase in PAC vesicles. To clarify the multiple transport pathway to protein storage vacuoles, the transport mechanism of these hydrolytic enzymes to the vacuoles should be established.

Targeting of PAC Vesicles to Protein Storage Vacuoles
The final step in the transport of a storage protein is the incorporation of the proprotein into a protein storage vacuole. There are two possible modes of incorporation: one is autophagy by the vacuoles, and the other is membrane fusion between PAC vesicles and the vacuoles. Autophagic engulfment by protein storage vacuoles has been observed in maturing seeds of pumpkin (data not shown) and pea (Robinson et al. 1995 ) and in seedlings of mung bean (Van der Wilden et al. 1980 ). Autophagy should be accompanied by the incorporation and breakdown of membrane proteins of protein storage vacuoles (Maeshima et al. 1994 ; Inoue et al. 1995a ; Strzalka et al. 1995 ). If such autophagy were to mediate the incorporation of PAC vesicles into the protein storage vacuoles, some of the tonoplast should remain inside the vacuoles. Detailed immunocytochemical studies about the tonoplast should answer the question of whether autophagic engulfment is involved in the incorporation of storage proteins into the protein storage vacuoles.

Alternatively, the incorporation of PAC vesicles into protein storage vacuoles could occur by membrane fusion. In yeast, distinct members of the Ras superfamily of small GTP binding proteins (Pryer et al. 1992 ) and members of the syntaxin family (Becherer et al. 1996 ) facilitate the targeting of vesicles to the appropriate membranes. We reported previously that two small GTP binding proteins are associated with the membrane of PAC vesicles (Shimada et al. 1994b ). Recently, two syntaxin homologs have been shown to be localized in specific compartments in Arabidopsis: AtPEP12 is localized on a post-Golgi compartment (da Silva Conceicao et al. 1997 ), and aVAM3 is localized on the contact sites between small vacuoles and large vacuoles (Sato et al. 1997 ). Thus, machinery analogous to that described in yeast could mediate the fusion of PAC vesicles with protein storage vacuoles. Further analysis is required to elucidate the involvement of members of these families in the transport of the storage proteins to protein storage vacuoles.

	METHODS

TOP ABSTRACT INTRODUCTION RESULTS DISCUSSION METHODS REFERENCES

Plant Materials
Pumpkin (Cucurbita sp cv Kurokawa Amakuri Nankin) seeds were purchased from Aisan Shubyo Seed Co. (Nagoya, Japan). The seeds were used directly for the isolation of protein bodies (protein storage vacuoles in dry seeds) and also were planted in the field during the summers of 1995 and 1996. The cotyledons of maturing seeds, freshly harvested 22 to 28 days after anthesis, were used for some of the experiments.

Castor bean (Ricinus communis) seeds were grown in a greenhouse during the summer of 1996. The maturing seeds were freshly harvested 25 to 30 days after anthesis, and the endosperm was used.

Isolation of Precursor-Accumulating Vesicles from Maturing Pumpkin Cotyledons
Precursor-accumulating (PAC) vesicles were isolated from pumpkin cotyledons at the middle stage of seed maturation by a method described previously (Hara-Nishimura et al. 1991 ; Shimada et al. 1994b ). The cotyledons (10 to 20 g) were homogenized in a solution (7 mL / g fresh weight of cotyledons) of 20 mM sodium pyrophosphate, pH 7.5, 1 mM EDTA, and 0.3 M mannitol with an ice-chilled mortar and pestle, and the homogenate was filtered through cheesecloth. The filtrate was centrifuged at 3000g for 15 min, and the supernatant was centrifuged again at 8000g for 20 min at 4°C. The resulting supernatant was used to isolate microsomes, as described below. The pellet was suspended in 1 mL of 10 mM Hepes-KOH, pH 7.2, 1 mM EDTA, and 0.3 M mannitol. The suspension was layered on a solution of 28% Percoll (Pharmacia LKB Biotechnology, Uppsala, Sweden) in 10 mM Hepes-KOH, pH 7.2, 1 mM EDTA, and 0.3 M mannitol on a cushion of 2 mL of 90% Percoll. Centrifugation was at 40,000g for 30 min at 4°C. The vesicle fraction was centrifuged again in a self-generated Percoll gradient. The resulting vesicle fraction was washed in the above-described Hepes-KOH buffer. The isolated PAC vesicles were subjected to either immunoelectron microscopy or immunoblot analysis.

Isolation of Microsomes from Maturing Pumpkin Cotyledons
Microsomes were also isolated from pumpkin cotyledons at the middle stage of seed maturation. An extract of cotyledons, prepared as described above, was centrifuged at 8000g and then at 100,000g for 30 min at 4°C. The pellet was suspended in 2 mL of 0.15 M Tricine-KOH, pH 6.8, 1 mM EDTA, and 13% (w/w) sucrose, and the suspension was layered on a step gradient of sucrose, which consisted of 50% (w/w) sucrose, 35% (w/w) sucrose, and 20% (w/w) sucrose. Centrifugation was at 21,000 rpm for 1 hr at 4°C in an SW 28 rotor (Beckman Instruments Ltd., Tokyo, Japan). Most microsomes formed a band between 20 and 35% (w/w) sucrose. The microsomal fraction was collected and diluted with the above-described Tricine-KOH buffer, and centrifugation was at 150,000g for 30 min at 4°C. The isolated microsomes were subjected to SDS-PAGE and then to an immunoblot analysis.

Isolation of Protein Bodies and Suborganellar Fractionation
Protein bodies were prepared from 5 g of dry pumpkin seeds by using a nonaqueous isolation method with 100% glycerol, as described previously (Hara-Nishimura et al. 1982 ). Both light microscopic examination and assays of marker enzymes indicated that the protein bodies were intact and were not contaminated with other cell organelles or cytoplasmic components. The protein bodies were lysed in 1 mL of a hypotonic buffer solution of 10 mM Tris-HCl, pH 7.5, and the lysate was centrifuged at 100,000g for 20 min at 4°C to separate it into a soluble matrix fraction and an insoluble crystalloid that was composed of the major seed protein 11S globulin. Aliquots of both the matrix and crystalloid fractions that had been prepared from protein bodies were equivalent to 200 µg of protein and were subjected to SDS-PAGE and then to immunoblot analysis with BiP-specific antibodies.

Preparation of Specific Antisera
The 51-kD protein is one of the major proteins in pumpkin seeds. To prepare polyclonal antibodies, we purified the 51-kD protein from the protein bodies that had been isolated as described above. Isolated protein bodies were burst in 10 mM Tris-Mes, pH 6.5, sonicated, and then centrifuged at 250g for 15 min to remove insoluble crystalloids as a pellet. A solution of NaCl was added to the supernatant to a final concentration of 1 M. During centrifugation at 100,000g for 1 hr, the 51-kD protein was sedimented. The pellet was subjected to SDS-PAGE with subsequent staining with Coomassie Brilliant Blue R 250. The band corresponding to the 51-kD protein was cut out from the gel and injected subcutaneously with complete Freund's adjuvant (Freund 1951 ) into a rabbit. After 3 weeks, two booster injections with incomplete adjuvant were given at 7-day intervals. One week after the second booster injection, blood was drawn and the antiserum was prepared.

Complex glycan-specific antibodies were purified from polyclonal antibodies raised against ß-xylosidase of sycamore (Acer pseudoplatanus) that had been raised previously (Tezuka et al. 1993 ). The ß-xylosidase contains xylose-containing N-linked oligosaccharides (Tezuka et al. 1993 ). To separate complex glycan-specific antibodies, we applied 5 mL of ß-xylosidase–specific antiserum to an affinity column of horseradish peroxidase–conjugated Sepharose 4B (Pharmacia LKB Biotechnology). After thoroughly washing the column, complex glycan-specific antibodies were eluted with glycine-HCl, pH 2.0. The affinity-purified antibodies recognized ricin, a major glycoprotein of castor bean (data not shown).

Previously prepared specific polyclonal antibodies specific to BiP (Hatano et al. 1997 ), 11S globulin (Hara and Matsubara 1980 ), or pro2S albumin (Hara-Nishimura et al. 1993a ) were also used for the experiments.

SDS-PAGE and Immunoblot Analysis
Both the PAC vesicles and the microsomes were subjected to SDS-PAGE on either a precast gradient gel (5 to 20% polyacrylamide; Atto Corporation, Tokyo, Japan) or a 12.5% polyacrylamide gel, and the protein body fractions were subjected to SDS-PAGE on a 12.5% polyacrylamide gel. Immunoblot analysis was performed essentially as described previously (Inoue et al. 1995a ). The separated proteins on gels were stained with Coomassie blue or were transferred electrophoretically to a GVHP membrane (0.22 µm; Nihon Millipore Ltd., Tokyo, Japan). The membrane blot was incubated with antibodies for 1 hr. Dilutions of specific antisera were as follows: anti-11S globulin (1:2000), anti-2S albumin (1:2000), anti–51-kD protein (1:500), and anti-BiP (1:2000 for the experimental results shown in Figure 7 and Figure 1:5000 for those shown in Figure 8). Horseradish peroxidase–conjugated antibodies raised in goat against rabbit IgG (Cappel, West Chester, PA) were diluted 10,000-fold and used as second antibodies. Immunodetection was performed with an enhanced chemiluminescence kit (Amersham Japan, Tokyo), according to the manufacturer's directions.

Ultrastructural Analysis and Immunogold Labeling
The pumpkin cotyledons and the castor bean endosperm at the middle stage of seed maturation were vacuum infiltrated for 1 hr with a fixative that consisted of 4% paraformaldehyde, 1% glutaraldehyde, and 0.06 M sucrose in 0.05 M cacodylate buffer, pH 7.4. The tissues were then cut into slices <1 mm thick with a razor blade and treated for another 2 hr with freshly prepared fixative. The isolated PAC vesicles were fixed in 4% paraformaldehyde, 1% glutaraldehyde, 0.3 M mannitol, 1 mM EDTA, and 10 mM Hepes-KOH, pH 7.2, at 4°C for 1 hr. Procedures for ultrastructural studies were essentially the same as those described previously (Hara-Nishimura et al. 1993a ), except that the material was postfixed with 1% osmium tetroxide in 0.1 M cacodylate buffer, pH 7.4, at 4°C for 2 hr.

Immunogold labeling procedures were essentially the same as those described previously (Nishimura et al. 1993 ), except for the use of the appropriate antibodies raised against 11S globulin, 2S albumin, the 51-kD protein, BiP, and complex glycans. Postfixation was omitted for immunoelectron microscopy. The samples were dehydrated in a graded dimethylformamide series at -20°C and embedded in London Resin White (London Resin Co. Ltd., Basingstoke, Hampshire, UK). Blocks were polymerized under a UV lamp at -20°C for 24 hr. Ultrathin sections were cut with a diamond knife on a Reichert ultramicrotome (Leica, Heidelberg, Germany) and mounted on uncoated nickel grids. The sections were treated with blocking solution (1% BSA in PBS) for 1 hr at room temperature and then incubated overnight with antibodies raised against 11S globulin (diluted 1:5000), 2S albumin (1:2500), the 51-kD protein (1:250), BiP (1:100), and complex glycans (1:50) in blocking solution at 4°C. After washing with PBS, sections were incubated for 30 min at room temperature with a solution of protein A–gold (10 or 15 nm; Amersham Japan) that had been diluted 1:30 in the blocking solution. The sections were washed with distilled water and then were stained with 4% uranyl acetate and lead citrate. After staining, all sections were examined with a transmission electron microscope (model 1200EX; JEOL, Tokyo, Japan) at 80 kV.

Assay of a Marker Enzyme and Quantitation of Protein
The activity of NADH–cytochrome c reductase was measured as described previously (Hara-Nishimura et al. 1985 ). The reaction mixture consisted of 0.5 mL of 25 mM Hepes-KOH, pH 8.5, 0.05 mM NADH, 1 mM antimycin, 2.5 mM NaN₃, 0.05% bovine cytochrome c, and the sample solution. The reaction was started by the addition of NADH; the increase in absorbance at 550 nm was then measured. The NADH-independent increase in absorbance at 550 nm was measured as a control. The concentration of protein was determined by using a protein assay kit (Bio-Rad) with -globulin as the standard.

	ACKNOWLEDGMENTS

We thank Chiyeko Namba for growing castor bean and pumpkin plants. We are grateful to Maki Kondo for discussions concerning the ultrastructural analyses. This work was supported by Grants-in-Aid for the Research for the Future Program (JSPS-RFTF96L60407), Scientific Research (Nos. 08454262 and 08262220) from the Ministry of Education, Science, and Culture of Japan.

Received September 25, 1997; accepted March 16, 1998.

	REFERENCES

TOP ABSTRACT INTRODUCTION RESULTS DISCUSSION METHODS REFERENCES

Ahmed, S.U., Bar-Peled, M., and Raikhel, N.V. (1997) Cloning and subcellular location of an Arabidopsis receptor-like protein that shares common features with protein sorting receptors of eukaryotic cells. Plant Physiol. 114:325-336[Abstract].

Becherer, K.A., Rieder, S.E., Emr, S.D., and Jones, E.W. (1996) A novel syntaxin homologue, Pep12p, required for the sorting of lumenal hydrolases to the lysosome-like vacuole in yeast. Mol. Cell Biol. 7:579-594.

Chrispeels, M.J. (1983) The Golgi apparatus mediates the transport of phytohemagglutinin to the protein bodies in bean cotyledons. Planta 158:140-151[CrossRef][Web of Science].

Chrispeels, M.J. (1985) The role of the Golgi apparatus in the transport and post-translational modification of vacuolar (protein body) proteins. Oxf. Surv. Plant Mol. Cell Biol. 2:43-68.

Craig, S. (1988) Structural aspects of protein accumulation in developing legume seeds. Biochem. Physiol. Pflanz. 183:159-171.

da Silva Conceição, A., Marty-Mazars, D., Bassham, D.C., Sanderfoot, A.A., Marty, F., and Raikhel, N.V. (1997) The syntaxin homolog AtPEP12p resides on a late post-Golgi compartment in plants. Plant Cell 9:571-582[Abstract].

Freund, J. (1951) The effect of paraffin oil and mycobacteria on antibody formation and sensitization. Am. J. Clin. Pathol. 21:645-656[Medline].

Fukasawa, T., Hara-Nishimura, I., and Nishimura, M. (1988) Biosynthesis, intracellular transport and in vitro processing of 11S globulin precursor proteins of developing castor bean endosperm. Plant Cell Physiol. 29:339-345[Abstract/Free Full Text].

Hara, I., and Matsubara, H. (1980) Pumpkin (Cucurbita sp.) seed globulin. VII. Immunofluorescent study on protein bodies in ungerminated and germinating cotyledon cells. Plant Cell Physiol. 21:247-254[Abstract/Free Full Text].

Hara-Nishimura, I. (1987) Introduction of disulfide bond in proglobulin molecules during the 11S globulin biosynthesis in endoplasmic reticulum of developing pumpkin cotyledons. Agric. Biol. Chem. 61:2007-2008.

Hara-Nishimura, I., and Nishimura, M. (1987) Proglobulin processing enzyme in vacuoles isolated from developing pumpkin cotyledons. Plant Physiol. 85:440-445[Abstract/Free Full Text].

Hara-Nishimura, I., Nishimura, M., Matsubara, H., and Akazawa, T. (1982) Suborganellar localization of proteinase catalyzing the limited hydrolysis of pumpkin globulin. Plant Physiol. 70:699-703[Abstract/Free Full Text].

Hara-Nishimura, I., Nishimura, M., and Akazawa, T. (1985) Biosynthesis and intracellular transport of 11S globulin in developing pumpkin cotyledons. Plant Physiol. 77:747-752[Abstract/Free Full Text].

Hara-Nishimura, I., Hayashi, M., Nishimura, M., and Akazawa, T. (1987) Biogenesis of protein bodies by budding from vacuoles in developing pumpkin cotyledons. Protoplasma 136:49-55[CrossRef].

Hara-Nishimura, I., Inoue, K., and Nishimura, M. (1991) A unique vacuolar processing enzyme responsible for conversion of several proprotein precursors into the mature forms. FEBS Lett. 294:89-93[CrossRef][Web of Science][Medline].

Hara-Nishimura, I., Takeuchi, Y., Inoue, K., and Nishimura, M. (1993a) Vesicle transport and processing of the precursor to 2S albumin in pumpkin. Plant J. 4:793-800[CrossRef][Web of Science][Medline].

Hara-Nishimura, I., Takeuchi, Y., and Nishimura, M. (1993b) Molecular characterization of a vacuolar processing enzyme related to a putative cysteine proteinase of Schistosoma mansoni.. Plant Cell 5:1651-1659[Abstract].

Hara-Nishimura, I., Shimada, T., Hiraiwa, N., and Nishimura, M. (1995) Vacuolar processing enzyme responsible for maturation of seed proteins. J. Plant Physiol. 145:632-640[Web of Science].

Hatano, K., Shimada, T., Hiraiwa, N., Nishimura, M., and Hara-Nishimura, I. (1997) A rapid increase in the level of binding protein (BiP) is accompanied by synthesis and degradation of storage proteins in pumpkin cotyledons. Plant Cell Physiol. 38:344-351[Abstract/Free Full Text].

Hayashi, M., Akazawa, T., Nishimura, M., and Hara-Nishimura, I. (1988) Effect of monensin on intracellular transport and posttranslational processing of 11S globulin precursors in developing pumpkin cotyledons. FEBS Lett. 238:197-200[CrossRef].

Heupke, H.-J., and Robinson, D.G. (1985) Intracellular transport of -amylase in barley aleurone cells: Evidence for the participation of the Golgi apparatus. Eur. J. Cell Biol. 39:265-272.

Hiraiwa, N., Takeuchi, Y., Nishimura, M., and Hara-Nishimura, I. (1993) A vacuolar processing enzyme in maturing and germinating seeds: Its distribution and associated changes during development. Plant Cell Physiol. 34:1197-1204[Abstract/Free Full Text].

Hiraiwa, N., Kondo, M., Nishimura, M., and Hara-Nishimura, I. (1997a) An aspartic proteinase is involved in the maturation of storage proteins in concert with the vacuolar processing enzyme. Eur. J. Biochem. 246:133-141[Web of Science][Medline].

Hiraiwa, N., Nishimura, M., and Hara-Nishimura, I. (1997b) Expression and activation of the vacuolar processing enzyme in Saccharomyces cerevisiae.. Plant J. 12:819-829[CrossRef][Web of Science][Medline].

Hohl, I., Robinson, D.G., Chrispeels, M.J., and Hinz, G. (1996) Transport of storage proteins to the vacuole is mediated by vesicles without clathrin coat. J. Cell Sci. 109:2539-2550[Abstract].

Inoue, K., Motozaki, A., Takeuchi, Y., Nishimura, M., and Hara-Nishimura, I. (1995a) Molecular characterization of proteins in protein-body membranes that disappear most rapidly during transformation of protein bodies into vacuoles. Plant J. 7:235-243[CrossRef][Web of Science][Medline].

Inoue, K., Takeuchi, Y., Nishimura, M., and Hara-Nishimura, I. (1995b) Characterization of two integral membrane proteins located in the protein bodies of pumpkin seeds. Plant Mol. Biol. 28:1089-1101[CrossRef][Web of Science][Medline].

Kirsch, T., Paris, N., Butler, J.M., Beevers, L., and Rogers, J. (1994) Purification and initial characterization of a potential plant vacuolar targeting receptor. Proc. Natl. Acad. Sci. USA 91:3403-3407[Abstract/Free Full Text].

Larkins, B.A., and Hurkman, W.J. (1978) Synthesis and deposition of protein bodies of maize endosperm. Plant Physiol. 62:256-263[Abstract/Free Full Text].

Levanony, H., Rubin, R., Altschuler, Y., and Galili, G. (1992) Evidence for a novel route of wheat storage proteins to vacuoles. J. Cell Biol. 119:1117-1128[Abstract/Free Full Text].

Li, X., Wu, Y., Zhang, D.-Z., Gillikin, J.W., Boston, R.S., Franceschi, V.R., and Okita, T.W. (1993) Rice prolamine protein body biogenesis: A BiP-mediated process. Science 262:1054-1056[Abstract/Free Full Text].

Maeshima, M., Hara-Nishimura, I., Takeuchi, Y., and Nishimura, M. (1994) Accumulation of vacuolar H⁺-pyrophosphatase and H⁺-ATPase during reformation of the central vacuole in germinating pumpkin seeds. Plant Physiol. 106:61-69[Abstract].

Mitsui, T., Akazawa, T., Christeller, J.T., and Tartakoff, A.M. (1985) Biosynthesis of rice seed -amylase: Two pathways of amylase secretion by the scutellum. Arch. Biochem. Biophys. 241:315-328[CrossRef][Web of Science][Medline].

Nishimura, M., Takeuchi, Y., De Bellis, L., and Hara-Nishimura, I. (1993) Leaf peroxisomes are directly transformed to glyoxysomes during senescence of pumpkin cotyledons. Protoplasma 175:131-137[CrossRef][Web of Science].

Okita, T.W., and Rogers, J.C. (1996) Compartmentation of proteins in the endomembrane system of plant cells. Annu. Rev. Plant Physiol. Plant Mol. Biol. 47:327-350[CrossRef][Web of Science].

Paris, N., Stanley, C.M., Jones, R.L., and Rogers, J.C. (1996) Plant cells contain two functionally distinct vacuolar compartments. Cell 85:563-572[CrossRef][Web of Science][Medline].

Paris, N., Rogers, S.W., Jiang, L., Kirsch, T., Beevers, L., Philips, T.E., and Rogers, J.C. (1997) Molecular cloning and further characterization of a probable plant vacuolar sorting receptor. Plant Physiol. 115:29-39[Abstract].

Pryer, N.K., Wuestehube, L.J., and Schekman, R. (1992) Vesicle-mediated protein sorting. Annu. Rev. Biochem. 61:471-516[CrossRef][Web of Science][Medline].

Robinson, D.G. (1996) Clathrin-mediated trafficking. Trends Plant Sci. 1:349-355[CrossRef][Web of Science].

Robinson, D.G., and Hinz, G. (1996) Multiple mechanisms of protein body formation in pea cotyledons. Plant Physiol. Biochem. 34:155-163.

Robinson, D.G., Hoh, B., Hinz, G., and Jeong, B.-K. (1995) One vacuole or two vacuoles: Do protein storage vacuoles arise de novo during pea cotyledon development? J. Plant Physiol. 145:654-664.

Sato, M.H., Nakamura, N., Ohsumi, Y., Kouchi, H., Kondo, M., Hara-Nishimura, I., Nishimura, M., and Wada, Y. (1997) The AtVAM3 encodes a syntaxin-related molecule implicated in the vacuolar assembly in Arabidopsis thaliana.. J. Biol. Chem. 272:24530-24535[Abstract/Free Full Text].

Shimada, T., Hiraiwa, N., Nishimura, M., and Hara-Nishimura, I. (1994a) Vacuolar processing enzyme of soybean that converts proprotein to the corresponding mature forms. Plant Cell Physiol. 35:713-718[Abstract/Free Full Text].

Shimada, T., Nishimura, M., and Hara-Nishimura, I. (1994b) Small GTP-binding proteins are associated with the vesicles targeting to vacuoles in developing pumpkin cotyledons. Plant Cell Physiol. 35:995-1001[Abstract/Free Full Text].

Shimada, T., Kuroyanagi, M., Nishimura, M., and Hara-Nishimura, I. (1997) Pumpkin 72-kDa membrane protein of precursor accumulating vesicles have characteristics for a vacuolar sorting receptor. Plant Cell Physiol. 38:1414-1420[Abstract/Free Full Text].

Shotwell, M.A., and Larkins, B.A. (1988). The biochemistry and molecular biology of seed storage proteins. In The Biochemistry of Plants, B.J. Miflin, ed (New York: Academic Press), pp. 297–345.

Strzalka, K., Hara-Nishimura, I., and Nishimura, M. (1995) Changes in physical properties of vacuolar membrane during transformation of protein bodies into vacuoles in germinating pumpkin seeds. Biochim. Biophys. Acta 1239:103-110[Medline].

Tezuka, K., Hayashi, M., Ishihara, H., Nishimura, M., Onozaki, K., and Takahashi, N. (1993) Purification and substrate specificity of ß-xylosidase from sycamore cell (Acer pseudoplatanus L.): Application for structural analysis of xylose-containing N-linked oligosaccharides. Anal. Biochem. 211:205-209[CrossRef][Medline].

Van der Wilden, W., Herman, E.M., and Chrispeels, M.J. (1980) Protein bodies of mung bean cotyledons as autophagic organelles. Proc. Natl. Acad. Sci. USA 77:428-432[Abstract/Free Full Text].

This article has been cited by other articles:

				T. Motoyama, N. Maruyama, Y. Amari, K. Kobayashi, H. Washida, T. Higasa, F. Takaiwa, and S. Utsumi {alpha}' Subunit of soybean {beta}-conglycinin forms complex with rice glutelin via a disulphide bond in transgenic rice seeds J. Exp. Bot., October 1, 2009; 60(14): 4015 - 4027. [Abstract] [Full Text] [PDF]

				K. Toyooka, Y. Goto, S. Asatsuma, M. Koizumi, T. Mitsui, and K. Matsuoka A Mobile Secretory Vesicle Cluster Involved in Mass Transport from the Golgi to the Plant Cell Exterior PLANT CELL, April 1, 2009; 21(4): 1212 - 1229. [Abstract] [Full Text] [PDF]

				Y. Saito, K. Kishida, K. Takata, H. Takahashi, T. Shimada, K. Tanaka, S. Morita, S. Satoh, and T. Masumura A green fluorescent protein fused to rice prolamin forms protein body-like structures in transgenic rice J. Exp. Bot., February 1, 2009; 60(2): 615 - 627. [Abstract] [Full Text] [PDF]

				F. Takaiwa, C. Sakuta, S.-K. Choi, Y. Tada, T. Motoyama, and S. Utsumi Co-Expression of Soybean Glycinins A1aB1b and A3B4 Enhances Their Accumulation Levels in Transgenic Rice Seed Plant Cell Physiol., October 1, 2008; 49(10): 1589 - 1599. [Abstract] [Full Text] [PDF]

				K. Yamada, A. J. Nagano, M. Nishina, I. Hara-Nishimura, and M. Nishimura NAI2 Is an Endoplasmic Reticulum Body Component That Enables ER Body Formation in Arabidopsis thaliana PLANT CELL, September 1, 2008; 20(9): 2529 - 2540. [Abstract] [Full Text] [PDF]

				E. Rojo and J. Denecke What Is Moving in the Secretory Pathway of Plants? Plant Physiology, August 1, 2008; 147(4): 1493 - 1503. [Full Text] [PDF]

				M. Yamazaki, T. Shimada, H. Takahashi, K. Tamura, M. Kondo, M. Nishimura, and I. Hara-Nishimura Arabidopsis VPS35, a Retromer Component, is Required for Vacuolar Protein Sorting and Involved in Plant Growth and Leaf Senescence Plant Cell Physiol., February 1, 2008; 49(2): 142 - 156. [Abstract] [Full Text] [PDF]

				F. Poustka, N. G. Irani, A. Feller, Y. Lu, L. Pourcel, K. Frame, and E. Grotewold A Trafficking Pathway for Anthocyanins Overlaps with the Endoplasmic Reticulum-to-Vacuole Protein-Sorting Route in Arabidopsis and Contributes to the Formation of Vacuolar Inclusions Plant Physiology, December 1, 2007; 145(4): 1323 - 1335. [Abstract] [Full Text] [PDF]

				K. Fuji, T. Shimada, H. Takahashi, K. Tamura, Y. Koumoto, S. Utsumi, K. Nishizawa, N. Maruyama, and I. Hara-Nishimura Arabidopsis Vacuolar Sorting Mutants (green fluorescent seed) Can Be Identified Efficiently by Secretion of Vacuole-Targeted Green Fluorescent Protein in Their Seeds PLANT CELL, February 1, 2007; 19(2): 597 - 609. [Abstract] [Full Text] [PDF]

				L. Li, T. Shimada, H. Takahashi, H. Ueda, Y. Fukao, M. Kondo, M. Nishimura, and I. Hara-Nishimura MAIGO2 Is Involved in Exit of Seed Storage Proteins from the Endoplasmic Reticulum in Arabidopsis thaliana PLANT CELL, December 1, 2006; 18(12): 3535 - 3547. [Abstract] [Full Text] [PDF]

				Y. Miao, P. K. Yan, H. Kim, I. Hwang, and L. Jiang Localization of Green Fluorescent Protein Fusions with the Seven Arabidopsis Vacuolar Sorting Receptors to Prevacuolar Compartments in Tobacco BY-2 Cells Plant Physiology, November 1, 2006; 142(3): 945 - 962. [Abstract] [Full Text] [PDF]

				T. Shimada, Y. Koumoto, L. Li, M. Yamazaki, M. Kondo, M. Nishimura, and I. Hara-Nishimura AtVPS29, a Putative Component of a Retromer Complex, is Required for the Efficient Sorting of Seed Storage Proteins Plant Cell Physiol., September 1, 2006; 47(9): 1187 - 1194. [Abstract] [Full Text] [PDF]

				G. Drakakaki, S. Marcel, E. Arcalis, F. Altmann, P. Gonzalez-Melendi, R. Fischer, P. Christou, and E. Stoger The Intracellular Fate of a Recombinant Protein Is Tissue Dependent Plant Physiology, June 1, 2006; 141(2): 578 - 586. [Abstract] [Full Text] [PDF]

				N. Maruyama, L. C. Mun, M. Tatsuhara, M. Sawada, M. Ishimoto, and S. Utsumi Multiple Vacuolar Sorting Determinants Exist in Soybean 11S Globulin PLANT CELL, May 1, 2006; 18(5): 1253 - 1273. [Abstract] [Full Text] [PDF]

				Y. Jou, C.-P. Chiang, G.-Y. Jauh, and H. E. Yen Functional Characterization of Ice Plant SKD1, an AAA-Type ATPase Associated with the Endoplasmic Reticulum-Golgi Network, and Its Role in Adaptation to Salt Stress Plant Physiology, May 1, 2006; 141(1): 135 - 146. [Abstract] [Full Text] [PDF]

				J. M. Pardo, B. Cubero, E. O. Leidi, and F. J. Quintero Alkali cation exchangers: roles in cellular homeostasis and stress tolerance J. Exp. Bot., March 1, 2006; 57(5): 1181 - 1199. [Abstract] [Full Text] [PDF]

				P. Pimpl, J. P. Taylor, C. Snowden, S. Hillmer, D. G. Robinson, and J. Denecke Golgi-Mediated Vacuolar Sorting of the Endoplasmic Reticulum Chaperone BiP May Play an Active Role in Quality Control within the Secretory Pathway PLANT CELL, January 1, 2006; 18(1): 198 - 211. [Abstract] [Full Text] [PDF]

				M. Oufattole, J. H. Park, M. Poxleitner, L. Jiang, and J. C. Rogers Selective Membrane Protein Internalization Accompanies Movement from the Endoplasmic Reticulum to the Protein Storage Vacuole Pathway in Arabidopsis PLANT CELL, November 1, 2005; 17(11): 3066 - 3080. [Abstract] [Full Text] [PDF]

				S.-J.-D. Claude, G. Marie-Agnes, R. Catalina, P. Nadine, K.-M. Marie-Christine, N. Jean-Marc, F. Loic, and G. Veronique Targeting of proConA to the Plant Vacuole depends on its Nine Amino-acid C-terminal Propeptide Plant Cell Physiol., October 1, 2005; 46(10): 1603 - 1612. [Abstract] [Full Text] [PDF]

				I. A. Sparkes, C. Hawes, and A. Baker AtPEX2 and AtPEX10 Are Targeted to Peroxisomes Independently of Known Endoplasmic Reticulum Trafficking Routes Plant Physiology, October 1, 2005; 139(2): 690 - 700. [Abstract] [Full Text] [PDF]

				M. Park, D. Lee, G.-J. Lee, and I. Hwang AtRMR1 functions as a cargo receptor for protein trafficking to the protein storage vacuole J. Cell Biol., August 29, 2005; 170(5): 757 - 767. [Abstract] [Full Text] [PDF]

				H. Takahashi, Y. Saito, T. Kitagawa, S. Morita, T. Masumura, and K. Tanaka A Novel Vesicle Derived Directly from Endoplasmic Reticulum is Involved in the Transport of Vacuolar Storage Proteins in Rice Endosperm Plant Cell Physiol., January 15, 2005; 46(1): 245 - 249. [Abstract] [Full Text] [PDF]

				L. L.P. daSilva, J. P. Taylor, J. L. Hadlington, S. L. Hanton, C. J. Snowden, S. J. Fox, O. Foresti, F. Brandizzi, and J. Denecke Receptor Salvage from the Prevacuolar Compartment Is Essential for Efficient Vacuolar Protein Targeting PLANT CELL, January 1, 2005; 17(1): 132 - 148. [Abstract] [Full Text] [PDF]

				P. Leivar, V. M. Gonzalez, S. Castel, R. N. Trelease, C. Lopez-Iglesias, M. Arro, A. Boronat, N. Campos, A. Ferrer, and X. Fernandez-Busquets Subcellular Localization of Arabidopsis 3-Hydroxy-3-Methylglutaryl-Coenzyme A Reductase Plant Physiology, January 1, 2005; 137(1): 57 - 69. [Abstract] [Full Text] [PDF]

				C. Carter, S. Pan, J. Zouhar, E. L. Avila, T. Girke, and N. V. Raikhel The Vegetative Vacuole Proteome of Arabidopsis thaliana Reveals Predicted and Unexpected Proteins PLANT CELL, December 1, 2004; 16(12): 3285 - 3303. [Abstract] [Full Text] [PDF]

				I. Hara-Nishimura, R. Matsushima, T. Shimada, and M. Nishimura Diversity and Formation of Endoplasmic Reticulum-Derived Compartments in Plants. Are These Compartments Specific to Plant Cells? Plant Physiology, November 1, 2004; 136(3): 3435 - 3439. [Full Text] [PDF]

				E. Herman and M. Schmidt Endoplasmic Reticulum to Vacuole Trafficking of Endoplasmic Reticulum Bodies Provides an Alternate Pathway for Protein Transfer to the Vacuole Plant Physiology, November 1, 2004; 136(3): 3440 - 3446. [Full Text] [PDF]

				E. Arcalis, S. Marcel, F. Altmann, D. Kolarich, G. Drakakaki, R. Fischer, P. Christou, and E. Stoger Unexpected Deposition Patterns of Recombinant Proteins in Post-Endoplasmic Reticulum Compartments of Wheat Endosperm Plant Physiology, November 1, 2004; 136(3): 3457 - 3466. [Abstract] [Full Text] [PDF]

				R. Matsushima, Y. Fukao, M. Nishimura, and I. Hara-Nishimura NAI1 Gene Encodes a Basic-Helix-Loop-Helix-Type Putative Transcription Factor That Regulates the Formation of an Endoplasmic Reticulum-Derived Structure, the ER Body PLANT CELL, June 1, 2004; 16(6): 1536 - 1549. [Abstract] [Full Text] [PDF]

				Y. C. Tse, B. Mo, S. Hillmer, M. Zhao, S. W. Lo, D. G. Robinson, and L. Jiang Identification of Multivesicular Bodies as Prevacuolar Compartments in Nicotiana tabacum BY-2 Cells PLANT CELL, March 1, 2004; 16(3): 672 - 693. [Abstract] [Full Text] [PDF]

				M. Park, S. J. Kim, A. Vitale, and I. Hwang Identification of the Protein Storage Vacuole and Protein Targeting to the Vacuole in Leaf Cells of Three Plant Species Plant Physiology, February 1, 2004; 134(2): 625 - 639. [Abstract] [Full Text] [PDF]

				E. Watanabe, T. Shimada, K. Tamura, R. Matsushima, Y. Koumoto, M. Nishimura, and I. Hara-Nishimura An ER-Localized Form of PV72, a Seed-Specific Vacuolar Sorting Receptor, Interferes the Transport of an NPIR-Containing Proteinase in Arabidopsis Leaves Plant Cell Physiol., January 15, 2004; 45(1): 9 - 17. [Abstract] [Full Text] [PDF]

				T. Shimada, K. Fuji, K. Tamura, M. Kondo, M. Nishimura, and I. Hara-Nishimura Vacuolar sorting receptor for seed storage proteins in Arabidopsis thaliana PNAS, December 23, 2003; 100(26): 16095 - 16100. [Abstract] [Full Text] [PDF]

				R. Matsushima, Y. Hayashi, K. Yamada, T. Shimada, M. Nishimura, and I. Hara-Nishimura The ER Body, a Novel Endoplasmic Reticulum-Derived Structure in Arabidopsis Plant Cell Physiol., July 15, 2003; 44(7): 661 - 666. [Abstract] [Full Text] [PDF]

				J. L. Hadlington, A. Santoro, J. Nuttall, J. Denecke, J. K-C. Ma, A. Vitale, and L. Frigerio The C-terminal Extension of a Hybrid Immunoglobulin A/G Heavy Chain Is Responsible for Its Golgi-mediated Sorting to the Vacuole Mol. Biol. Cell, June 1, 2003; 14(6): 2592 - 2602. [Abstract] [Full Text] [PDF]

				R. Matsushima, Y. Hayashi, M. Kondo, T. Shimada, M. Nishimura, and I. Hara-Nishimura An Endoplasmic Reticulum-Derived Structure That Is Induced under Stress Conditions in Arabidopsis Plant Physiology, December 1, 2002; 130(4): 1807 - 1814. [Abstract] [Full Text] [PDF]

				T. Shimada, E. Watanabe, K. Tamura, Y. Hayashi, M. Nishimura, and I. Hara-Nishimura A Vacuolar Sorting Receptor PV72 on the Membrane of Vesicles that Accumulate Precursors of Seed Storage Proteins (PAC Vesicles) Plant Cell Physiol., October 15, 2002; 43(10): 1086 - 1095. [Abstract] [Full Text] [PDF]

				N. Kutsuna and S. Hasezawa Dynamic Organization of Vacuolar and Microtubule Structures during Cell Cycle Progression in Synchronized Tobacco BY-2 Cells Plant Cell Physiol., September 15, 2002; 43(9): 965 - 973. [Abstract] [Full Text] [PDF]

				M. H. Lee, M. K. Min, Y. J. Lee, J. B. Jin, D. H. Shin, D. H. Kim, K.-H. Lee, and I. Hwang ADP-Ribosylation Factor 1 of Arabidopsis Plays a Critical Role in Intracellular Trafficking and Maintenance of Endoplasmic Reticulum Morphology in Arabidopsis Plant Physiology, August 1, 2002; 129(4): 1507 - 1520. [Abstract] [Full Text] [PDF]

				Y.-B. Li, S. W. Rogers, Y. C. Tse, S. W. Lo, S. S. M. Sun, G.-Y. Jauh, and L. Jiang BP-80 and Homologs are Concentrated on Post-Golgi, Probable Lytic Prevacuolar Compartments Plant Cell Physiol., July 15, 2002; 43(7): 726 - 742. [Abstract] [Full Text] [PDF]

				F. Brandizzi, E. L. Snapp, A. G. Roberts, J. Lippincott-Schwartz, and C. Hawes Membrane Protein Transport between the Endoplasmic Reticulum and the Golgi in Tobacco Leaves Is Energy Dependent but Cytoskeleton Independent: Evidence from Selective Photobleaching PLANT CELL, June 1, 2002; 14(6): 1293 - 1309. [Abstract] [Full Text] [PDF]

				E. Watanabe, T. Shimada, M. Kuroyanagi, M. Nishimura, and I. Hara-Nishimura Calcium-mediated Association of a Putative Vacuolar Sorting Receptor PV72 with a Propeptide of 2S Albumin J. Biol. Chem., March 1, 2002; 277(10): 8708 - 8715. [Abstract] [Full Text] [PDF]

				L. Jiang, T. E. Phillips, C. A. Hamm, Y. M. Drozdowicz, P. A. Rea, M. Maeshima, S. W. Rogers, and J. C. Rogers The protein storage vacuole: a unique compound organelle J. Cell Biol., December 10, 2001; 155(6): 991 - 1002. [Abstract] [Full Text] [PDF]

				G. Shy, L. Ehler, E. Herman, and G. Galili Expression patterns of genes encoding endomembrane proteins support a reduced function of the Golgi in wheat endosperm during the onset of storage protein deposition J. Exp. Bot., December 1, 2001; 52(365): 2387 - 2388. [Abstract] [Full Text] [PDF]

				E. Torres, P. Gonzalez-Melendi, E. Stoger, P. Shaw, R. M. Twyman, L. Nicholson, C. Vaquero, R. Fischer, P. Christou, and Y. Perrin Native and Artificial Reticuloplasmins Co-Accumulate in Distinct Domains of the Endoplasmic Reticulum and in Post-Endoplasmic Reticulum Compartments Plant Physiology, November 1, 2001; 127(3): 1212 - 1223. [Abstract] [Full Text] [PDF]

				N. Mitsuhashi, Y. Hayashi, Y. Koumoto, T. Shimada, T. Fukasawa-Akada, M. Nishimura, and I. Hara-Nishimura A Novel Membrane Protein That Is Transported to Protein Storage Vacuoles via Precursor-Accumulating Vesicles PLANT CELL, October 1, 2001; 13(10): 2361 - 2372. [Abstract] [Full Text] [PDF]

				Y. Hayashi, K. Yamada, T. Shimada, R. Matsushima, N. K. Nishizawa, M. Nishimura, and I. Hara-Nishimura A Proteinase-Storing Body that Prepares for Cell Death or Stresses in the Epidermal Cells of Arabidopsis Plant Cell Physiol., September 1, 2001; 42(9): 894 - 899. [Abstract] [Full Text] [PDF]

				K. Tormakangas, J. L. Hadlington, P. Pimpl, S. Hillmer, F. Brandizzi, T. H. Teeri, and J. Denecke A Vacuolar Sorting Domain May Also Influence the Way in Which Proteins Leave the Endoplasmic Reticulum PLANT CELL, September 1, 2001; 13(9): 2021 - 2032. [Abstract] [Full Text] [PDF]

				J. B. Jin, Y. A Kim, S. J. Kim, S. H. Lee, D. H. Kim, G.-W. Cheong, and I. Hwang A New Dynamin-Like Protein, ADL6, Is Involved in Trafficking from the trans-Golgi Network to the Central Vacuole in Arabidopsis PLANT CELL, July 1, 2001; 13(7): 1511 - 1526. [Abstract] [Full Text] [PDF]

				L. Frigerio, A. Pastres, A. Prada, and A. Vitale Influence of KDEL on the Fate of Trimeric or Assembly-Defective Phaseolin: Selective Use of an Alternative Route to Vacuoles PLANT CELL, May 1, 2001; 13(5): 1109 - 1126. [Abstract] [Full Text]

				A. J. Kinney, R. Jung, and E. M. Herman Cosuppression of the {{alpha}} Subunits of {beta}-Conglycinin in Transgenic Soybean Seeds Induces the Formation of Endoplasmic Reticulum-Derived Protein Bodies PLANT CELL, May 1, 2001; 13(5): 1165 - 1178. [Abstract] [Full Text]

				L. Frigerio, N. A. Jolliffe, A. Di Cola, D. H. Felipe, N. Paris, J.-M. Neuhaus, J. M. Lord, A. Ceriotti, and L. M. Roberts The Internal Propeptide of the Ricin Precursor Carries a Sequence-Specific Determinant for Vacuolar Sorting Plant Physiology, May 1, 2001; 126(1): 167 - 175. [Abstract] [Full Text]

				D. K. Ro, N. Mah, B. E. Ellis, and C. J. Douglas Functional Characterization and Subcellular Localization of Poplar (Populus trichocarpa x Populus deltoides) Cinnamate 4-Hydroxylase Plant Physiology, May 1, 2001; 126(1): 317 - 329. [Abstract] [Full Text]

				S. Hillmer, A. Movafeghi, D. G. Robinson, and G. Hinz Vacuolar Storage Proteins Are Sorted in the Cis-Cisternae of the Pea Cotyledon Golgi Apparatus J. Cell Biol., January 8, 2001; 152(1): 41 - 50. [Abstract] [Full Text] [PDF]

				A. Vitale and G. Galili The Endomembrane System and the Problem of Protein Sorting Plant Physiology, January 1, 2001; 125(1): 115 - 118. [Full Text]

				L. Jiang, T. E. Phillips, S. W. Rogers, and J. C. Rogers Biogenesis of the Protein Storage Vacuole Crystalloid J. Cell Biol., August 21, 2000; 150(4): 755 - 770. [Abstract] [Full Text] [PDF]

				M. J. Chrispeels and E. M. Herman Endoplasmic Reticulum-Derived Compartments Function in Storage and as Mediators of Vacuolar Remodeling via a New Type of Organelle, Precursor Protease Vesicles Plant Physiology, August 1, 2000; 123(4): 1227 - 1234. [Full Text]

				K. Toyooka, T. Okamoto, and T. Minamikawa Mass Transport of Proform of a Kdel-Tailed Cysteine Proteinase (Sh-EP) to Protein Storage Vacuoles by Endoplasmic Reticulum-Derived Vesicle Is Involved in Protein Mobilization in Germinating Seeds J. Cell Biol., February 7, 2000; 148(3): 453 - 464. [Abstract] [Full Text] [PDF]

				M. Schmid, D. Simpson, and C. Gietl Programmed cell death in castor bean endosperm is associated with the accumulation and release of a cysteine endopeptidase from ricinosomes PNAS, November 23, 1999; 96(24): 14159 - 14164. [Abstract] [Full Text] [PDF]

				G. Hinz, S. Hillmer, M. Bäumer, and I. Hohl Vacuolar Storage Proteins and the Putative Vacuolar Sorting Receptor BP-80 Exit the Golgi Apparatus of Developing Pea Cotyledons in Different Transport Vesicles PLANT CELL, August 1, 1999; 11(8): 1509 - 1524. [Abstract] [Full Text]

				F. Barrieu and M. J. Chrispeels Delivery of a Secreted Soluble Protein to the Vacuole via a Membrane Anchor Plant Physiology, August 1, 1999; 120(4): 961 - 968. [Abstract] [Full Text]

				F. Marty Plant Vacuoles PLANT CELL, April 1, 1999; 11(4): 587 - 600. [Full Text]

				E. M. Herman and B. A. Larkins Protein Storage Bodies and Vacuoles PLANT CELL, April 1, 1999; 11(4): 601 - 614. [Full Text]

				A. Vitale and J. Denecke The Endoplasmic Reticulum—Gateway of the Secretory Pathway PLANT CELL, April 1, 1999; 11(4): 615 - 628. [Full Text]

				K. Yamada, T. Shimada, M. Kondo, M. Nishimura, and I. Hara-Nishimura Multiple Functional Proteins Are Produced by Cleaving Asn-Gln Bonds of a Single Precursor by Vacuolar Processing Enzyme J. Biol. Chem., January 22, 1999; 274(4): 2563 - 2570. [Abstract] [Full Text] [PDF]

				T. Okamoto, K. Toyooka, and T. Minamikawa Identification of a Membrane-associated Cysteine Protease with Possible Dual Roles in the Endoplasmic Reticulum and Protein Storage Vacuole J. Biol. Chem., January 5, 2001; 276(1): 742 - 751. [Abstract] [Full Text] [PDF]

This Article Abstract Full Text (PDF) Alert me when this article is cited Alert me if a correction is posted Services Email this article to a friend Similar articles in this journal Similar articles in Web of Science Similar articles in PubMed Alert me to new issues of the journal Download to citation manager Citing Articles Citing Articles via HighWire Citing Articles via CrossRef Citing Articles via Web of Science (137) Citing Articles via Google Scholar Google Scholar Articles by Hara-Nishimura, I. Articles by Nishimura, M. Search for Related Content PubMed PubMed Citation Articles by Hara-Nishimura, I. Articles by Nishimura, M. Agricola Articles by Hara-Nishimura, I. Articles by Nishimura, M.