| HOME | HELP | FEEDBACK | SUBSCRIPTIONS | ARCHIVE | SEARCH | TABLE OF CONTENTS |
|
|
|
|||||||
|
|||||||||
|
Plant Physiology 147:1493-1503 (2008) © 2008 American Society of Plant Biologists What Is Moving in the Secretory Pathway of Plants?1Departamento de Genética Molecular de Plantas, Centro Nacional de Biotecnología-Consejo Superior de Investigaciones Científicas, E–28049 Madrid, Spain (E.R.); and Centre for Plant Sciences, Faculty of Biological Sciences, The University of Leeds, Leeds LS2 9JT, United Kingdom (J.D.)
The secretory pathway of eukaryotic cells is a fascinating system of membrane compartments in dynamic equilibrium from the constant budding and fusion of vesicles and other membrane-enclosed transport carriers. Compared to yeasts, the plant protein machinery controlling vesicle budding, tethering, and fusion appears to be more complex and comparable to that of multicellular metazoans, confirming prior conceptions about the great complexity of the secretory pathway in plants. Moreover, phylogenetic analysis of trafficking components from plants, fungi, and animals suggest that many of those components were derived from duplications occurring after the last common eukaryotic ancestor, implying that numerous features of the endomembrane system evolved separately in the different kingdoms (Vernoud et al., 2003 In this Update, we will first review the ongoing efforts to genetically characterize the machinery involved in biosynthetic trafficking in plants. In recent years, many new genes implicated in different steps of trafficking in the plant biosynthetic pathway have been discovered (Table I). We will then discuss how the functional analysis of these components has allowed more detailed characterization of the trafficking pathways for soluble and membrane proteins in this route. Finally, we will discuss the recent data on the convergence/intersection of the biosynthetic and endocytic pathways in plants and comment on the current debate regarding the existence of two fundamentally different trafficking routes to vacuoles within the same cell.
Relatively few trafficking components have been genetically characterized through analysis of loss-of-function mutants. Redundancy within the large gene families encoding many of these components may account for this and, indeed, this has already been shown in a number of cases. Arabidopsis (Arabidopsis thaliana) has three genes homologous to the yeast retromer component VPS35, and trafficking phenotypes can be observed by combining null alleles in AtVPS35b and AtVPS35c, or null alleles in AtVPS35a and AtVPS35c and a weak allele in AtVPS35b. These double and triple mutants showed defects in growth and in the vacuolar targeting of storage proteins in seeds (Yamazaki et al., 2008  ). The VTI11 and VTI12 SNAREs are a well-characterized example of conditional redundancy. VTI11 and VTI12 have distinct localizations, interacting SNARE partners, and functions. However, in the absence of one of them, the other takes over in the respective complex and substitutes it functionally, albeit only partially (Surpin et al., 2003; Sanmartin et al., 2007). Moreover, a single amino acid change in VTI12 enhances its capacity to substitute for VTI11, probably by increasing its affinity for the corresponding SNARE complex (Niihama et al., 2005). Another interesting example of redundancy was recently reported between GNL1 and GNOM, two Arabidopsis ARF-GEFs (Richter et al., 2007; Teh and Moore, 2007). Through mutant analysis and engineering of brefeldin A-resistant and -sensitive forms of these proteins, it was demonstrated that GNL1 and GNOM are redundantly involved in COPI-coated vesicle formation at the Golgi stacks. Moreover, GNL1 functions with an unidentified brefeldin A-sensitive ARF-GEF in endocytosis of pin-formed (PIN) efflux carriers, whereas GNOM functions in their recycling from endosomes to the plasma membrane (PM).
Genetic redundancy may lead to subtle phenotypes difficult to discover through the reverse-genetic approaches that are commonly used in plants such as Arabidopsis. In cases where redundancy is not present, knockout of trafficking genes may result in early lethality (Rojo et al., 2001
Moore and collaborators reported a genetic assay to detect Arabidopsis mutants blocked in secretion based on the enhanced stability and fluorescence of a secreted GFP construct (secGFP) when retained in intracellular compartments. With this assay, two genes necessary for export of cargo (including secGFP) from the endoplasmic reticulum (ER) have been identified: RDH3, which encodes a GTP binding protein, and GNL1, which encodes an ARF-GEF (Zheng et al., 2004
Several genetic assays to dissect trafficking to plant vacuoles have also been described. A laborious screen for maigo (mag) mutants that accumulate seed storage protein precursors, which is indicative of a block in their vacuolar targeting, led to the isolation of a number of Arabidopsis mutants. MAG1 encodes the retromer component VPS29 (Shimada et al., 2006
MAG2 encodes a protein related to Rint1/TIP20 (Li et al., 2006
Recently, Hara-Nishimura and collaborators developed a more efficient method for isolating mutants in vacuolar sorting. This screen is based on detection of the SP-GFP-CT24 vacuolar marker in the apoplasm, where the marker is stabilized, leading to a great increase in fluorescence. In this way, more than 100 green fluorescent seed (gfs) mutants were isolated. Analysis of 10 of those mutants showed that they corresponded to seven complementation groups (Fuji et al., 2007
Another vacuolar mutant screen has recently been described (Sanmartin et al., 2007 It will be important to devise further screens with more elaborate reporter systems to study plant-specific phenomena, such as Golgi morphology and motility, and to discover those key players of the pathway that evolved after the last common eukaryotic ancestor.
In addition to mutants, a large body of genetic data on the function of different trafficking components has been attained through expression of dominant transgenes. Although loss-of-function mutants are a first step toward gene identification, further knowledge can often be gained through the use of gain-of-function mutants. These can range from dominant-negative mutants to simply overexpressed wild-type proteins, which lead to titration of other components of the system and shed light on the network of possible interactions within a living cell.
Through the available trafficking assays, three major gene families have been studied by transient expression of dominant constructs: GTPases of the Rab and ARF families, ATPases of chaperones and other key regulators of organelle traffic, and SNAREs. In the case of the GTPases, it is possible to engineer mutated versions of a particular Rab or ARF locked in the GTP or GDP bound forms. Nucleotide-free mutants have also been instrumental with Rab GTPases and are thought to titrate their exchange factors, although this has not been formally tested in plants. In the case of ER export, it was experimentally shown that overdose of the exchange factor Sec12 titrates its target GTPase Sar1 and prevents ER export of soluble cargo (Phillipson et al., 2001
Curiously, nucleotide-free rab mutants are expected to exhibit a dominant effect and reveal their role in membrane trafficking even in the presence of the wild-type gene (Table I) because they lead to stable complexes with their nucleotide exchange factors, thus titrating those and preventing wild-type Rabs from functioning even when these are overexpressed (Jones et al., 1995
In the case of SNAREs, overexpression of truncated molecules lacking the transmembrane domain (Sp2 fragment) can exhibit dominant-negative effects (Tyrrell et al., 2007
Expression of engineered forms of a protein that have an altered sensitivity to a drug is a very powerful system to study gene function. This approach was used to prove the specific function of the ARF-GEFs GNOM and GNL1 in ER-Golgi trafficking and in endocytosis and recycling to the PM (Geldner et al., 2003
An advantage of transient expression experiments is the possibility of testing particular constructs that would be deleterious to stable transformed plants. Moreover, the speed of the assays permits much deeper characterization of the particular trafficking steps studied. An example of this is the thorough functional analysis of the Bp80/VSR1 protein, which demonstrated that recycling of VSR1 to the PVC is essential for efficient transport of vacuolar cargo and saturable (daSilva et al., 2005
It is interesting to note that silencing techniques, such as RNA interference (RNAi) or virus-induced gene silencing (VIGS), have not been widely used yet to analyze trafficking, although they could prove very helpful, especially in transient assays. Similar to the titration of a gene product by a permanently binding mutant molecule, this technique simulates loss-of-function mutations and can be timed by the inducible expression of RNAi. Recently, evidence linking Syp132 to secretion of pathogenesis-related proteins and resistance to pathogens was obtained through VIGS silencing of the tobacco (Nicotiana tabacum) gene (Kalde et al., 2007
A caveat to many of the genetic data available is that only one or, at best, a few trafficking markers were tested for each mutant or transgenic line analyzed. This is particularly relevant for experiments using transient expression because, in that case, there is no previous selection against deleterious side effects, as in the case of stable mutants. Analyzing multiple markers increases the chances to dissect between a general block in endomembrane trafficking and specific branches of a pathway, even if a specific effector influences more than one pathway (Pimpl et al., 2003
Transport of soluble proteins in the biosynthetic pathway is probably the best-characterized trafficking process in the endomembrane system of plants. It is now widely accepted that the default destination for soluble proteins in the secretory pathway is the apoplasm and that no export signals are required to achieve transport rates of native secretory proteins like amylase (Denecke et al., 1990 ; Crofts et al., 1999; Phillipson et al., 2001; Pimpl et al., 2006). To be retained in intracellular compartments, proteins require positive sorting information in their sequence. Signals for retention in the ER and for targeting to the vacuole have been thoroughly characterized (Vitale and Hinz, 2005). In contrast, soluble proteins retained in the Golgi or in endosomal compartments have not been reported. Moreover, very little is known about the process of secretion of soluble cargo to the PM. For example, the secretory vesicles have not been characterized, nor is it known whether the last compartment that soluble proteins pass before reaching the PM is the Golgi apparatus or the TGN. In fact, it cannot even be ruled out that the PVC can serve as a sorting station for transport to the PM during certain conditions. An added level of complexity of secretion in plants is that cell wall polysaccharides appear to use different pathways than proteins (Leucci et al., 2007).
Due to the agronomic importance of storage proteins accumulated in vacuoles and protein bodies of plants, many studies have been focused in this process. Comparatively, a lot of data in plant vacuolar trafficking have been generated and fueled intense debate. An important point of discussion in the field of vacuolar trafficking is the nature of the receptors that recognize the vacuolar sorting determinants in soluble cargo to package them into vesicles destined for the vacuole. Two families of proteins have been put forward as candidates to fulfill that role. The VSR family of proteins, made up of seven members in Arabidopsis, has many of the characteristics expected for sorting receptors. They are type I transmembrane proteins with a large lumenal domain that interacts with vacuolar sorting determinants. The small cytosolic tail harbors motifs that are involved in interaction with adaptor complexes of vesicle coats. Moreover, VSRs are present on the TGN and PVC (Sanderfoot et al., 1998
Initially, progress in investigating the transport of plant membrane proteins was slow compared to soluble proteins, mainly due to the lack of good markers and simple assays. With the development of live imaging with GFP fusions and other spectral variants, advances on understanding the sorting of membrane-spanning proteins within the plant secretory pathway is now fast and furious and many principles are starting to emerge. Whereas secretion appears to be the default for soluble proteins, the rules regarding the exit of membrane-spanning proteins from the ER and subsequent sorting to other locations appear to be more complex, as suggested by conflicting reports. It was first suggested that the tonoplast is the default membrane (Hofte and Chrispeels, 1992 ). This hypothesis was further tested with type I membrane-spanning reporter fusions constructed from ER residents and mutagenesis of the known ER retention signals. One of these studies confirmed the tonoplast as default (Barrieu and Chrispeels, 1999), whereas the other suggested the PM (Benghezal et al., 2000).
Further complexity was introduced by a study that suggested a critical role of the length of the transmembrane domain in the sorting of type I membrane-spanning proteins (Brandizzi et al., 2002
Most recently, a systematic analysis of the sorting of p24 proteins revealed that deletion of a di-Lys motif for COPI-mediated ER retention led to transport to the PVC and a soluble degradation product was detected in the vacuole lumen (Langhans et al., 2008
The problem with many of these studies is that the reporter fusion is proteolytically cleaved and leads to the detection of the soluble reporter in either the vacuole (Barrieu and Chrispeels, 1999
As part of a systematic analysis of the sorting of the plant VSR BP80, the lumenal portion of BP80 was replaced by GFP and the C-terminal tail was mutagenized (daSilva et al., 2005
Rules regarding the sorting of membrane-spanning proteins are thus far from established in plants. It should also be noted that comparable BP80 transmembrane domains were used in two studies, but different results were obtained (Brandizzi et al., 2002
Finally, results obtained with type I membrane-spanning proteins could not necessarily apply to all membrane-spanning proteins. For instance, the sorting of type II membrane-spanning proteins could be dependent on both the transmembrane length and on motifs exposed in the cytosolic peptides (Saint-Jore-Dupas et al., 2006
Compared to the knowledge on the early secretory pathway in plants and the route to the vacuole, much less is known about endocytic transport routes or the route taken by secretory proteins. Where do secretory proteins segregate from vacuolar proteins? Are there several routes to the PM? One of the difficulties with research on endocytosis is related to the fact that much of the research was inspired by analogy from processes in animals and yeasts. For instance, the Rab5 group was initially assumed to label the early endosome (EE), and colocalization with endocytic tracers, such as FM4-64, was taken for granted as evidence for endocytic compartments. Later evidence demonstrated that the Rab5 group labels the PVC or the multivesicular body (Kotzer et al., 2004 ; Haas et al., 2007), the suggested plant equivalent of the late endosome (LE).
It is clear that colocalization with FM4-64 alone is totally insufficient as an indication for involvement in endocytosis, because, depending on the time of incubation, cell type, and experimental conditions, the tracer can label almost any compartment of the cell (Bolte et al., 2004
During the last decade, it has been a popular concept to single out plants for their extraordinary complexity of the vacuolar transport. This was inspired by published evidence suggesting that soluble and membrane-spanning proteins reach the vacuoles by different routes (Gomez and Chrispeels, 1993 ), by a difference in sensitivity to wortmannin when comparing two soluble vacuolar cargos (Matsuoka et al., 1995), and by reports showing that compartments containing lumenal and membrane markers characteristic of lytic and storage vacuoles can be differentiated in certain cell types (Hoh et al., 1995; Paris et al., 1996; Di Sansebastiano et al., 2001; Park et al., 2004). Moreover, in Mesembryanthemum crystallinum, functionally different vacuoles within a single leaf mesophyll cell can be clearly recognized (Epimashko et al., 2004), and in pea (Pisum sativum) cotyledon parenchyma cells from embryos PSV and lytic vacuoles are also morphologically distinguishable (Hoh et al., 1995). However, recent work has not found evidence of distinct vacuoles in Arabidopsis embryos, pea, and barley (Hordeum vulgare) roots (Otegui et al., 2006; Hunter et al., 2007; Olbrich et al., 2007). It is as yet unclear whether this reflects species differences, but further work should be carried out to investigate this in more detail. Even if plant cells contain a single vacuole type, different routes to that vacuole may exist, similarly to the situation in yeast or mammals. Indeed, there is evidence of segregation of vacuolar cargo to different subdomains of the Golgi and distinct vesicles (Otegui et al., 2006). Differences in the sensitivity to drugs (Matsuoka et al., 1995) or to dominant-negative inhibitors, such as GTP-trapped ARF1 (Pimpl et al., 2003), could be used as arguments to justify different routes. However, the results could also be explained if two different vacuolar sorting signals bind the same receptor, but with different affinities. Under impaired transport conditions, strong ligands might still reach the vacuole while weak ligands are secreted. This may explain why some in vitro binding studies are above or below the detection limit (Kirsch et al., 1996) and also why inhibition of transport leads to differential dose-response characteristics (Pimpl et al., 2003). In addition, the knockdown of Arabidopsis BP80 has led to secretion of some storage proteins, but not all vacuolar cargo (Shimada et al., 2003), but this could be due to the fact that storage proteins are more abundant and have a lower affinity to BP80 because they can use alternative ways to target the vacuoles (i.e. by aggregation and incorporation into DVs). Indeed, an alternative study using artificial ligands and expressed at more equivalent levels revealed that BP80 knockdown leads to induced secretion of different types of vacuolar cargo without discrimination between different classes of sorting signals (Craddock et al., 2008). In summary, if two different vacuolar transport routes exist, it is important to identify reciprocal specificity of inhibitors or mutations so that one route can be inhibited without affecting the other and vice versa. This has not been accomplished yet.
The secretory pathway of plants is an important production platform of important biomolecules and deserves our full attention in the current climate of depleting energy resources that are easy to exploit. In addition, the complexity of the pathway is particularly challenging from a fundamental perspective because it contains many circular processes that require molecular switches, signal transduction, and feedback loops. Finally, it has now become clear that the plant secretory pathway is by no means identical to the pathway in yeasts or mammals and that many plant-specific features remain to be explored. This is best documented by a comparison of Rab GTPases and their subcellular localizations. Mammalian Rab11 is localized on the recycling endosomes, but plant Rab11 is found on the TGN (Chow et al., 2008 ). Mammalian Rab5 is a key molecule of EE, whereas in plants this group is found on the PVC (Kotzer et al., 2004; Dettmer et al., 2006; Haas et al., 2007) and contains a unique plant-specific N-myristoylated Rab5 derivative (Ueda et al., 2001). Finally, mammalian Rab7 is found on LEs, whereas in plants it decorates the tonoplast (Saito et al., 2002). If Rab GTPases would be used as signatures for organelle identities, we could thus suggest that the phragmoplast is not a derivative of the PM, but simply a specialized form of TGN (Chow et al., 2008) that perhaps later matures into a PM. Likewise, plant vacuoles may be equivalents of mammalian LEs rather than lysosomes. Clearly, we still have much to learn about the intricacies of the plant secretory pathway. Received June 11, 2008; accepted June 25, 2008; published August 6, 2008.
1 This work was supported, in part, by the Spanish Ministerio de Educación y Ciencia (grant no. BIO2006–11150 to E.R.) and by the U.K. Biotechnology and Biological Sciences Research Council.  The author responsible for distribution of materials integral to the findings presented in this article in accordance with the policy described in the Instructions for Authors (www.plantphysiol.org) is: Jurgen Denecke (j.denecke{at}leeds.ac.uk). www.plantphysiol.org/cgi/doi/10.1104/pp.108.124552 * Corresponding author; e-mail j.denecke{at}leeds.ac.uk.
Anders N, Nielsen M, Keicher J, Stierhof YD, Furutani M, Tasaka M, Skriver K, Jurgens G (2008) Membrane association of the Arabidopsis ARF exchange factor GNOM involves interaction of conserved domains. Plant Cell 20: 142–151 Barbante A, Irons S, Hawes C, Frigerio L, Vitale A, Pedrazzini E (2008) Anchorage to the cytosolic face of the endoplasmic reticulum membrane: a new strategy to stabilize a cytosolic recombinant antigen in plants. Plant Biotechnol J (in press) Barrieu F, Chrispeels MJ (1999) Delivery of a secreted soluble protein to the vacuole via a membrane anchor. Plant Physiol 120: 961–968 Batoko H, Zheng HQ, Hawes C, Moore I (2000) A Rab1 GTPase is required for transport between the endoplasmic reticulum and Golgi apparatus and for normal Golgi movement in plants. Plant Cell 12: 2201–2218 Benghezal M, Wasteneys GO, Jones DA (2000) The C-terminal dilysine motif confers endoplasmic reticulum localization to type I membrane proteins in plants. Plant Cell 12: 1179–1201 Bolte S, Talbot C, Boutte Y, Catrice O, Read ND, Satiat-Jeunemaitre B (2004) FM-dyes as experimental probes for dissecting vesicle trafficking in living plant cells. J Microsc 214: 159–173[Medline] Brandizzi F, Frangne N, Marc-Martin S, Hawes C, Neuhaus JM, Paris N (2002) The destination for single-pass membrane proteins is influenced markedly by the length of the hydrophobic domain. Plant Cell 14: 1077–1092 Chatre L, Brandizzi F, Hocquellet A, Hawes C, Moreau P (2005) Sec22 and Memb11 are v-SNAREs of the anterograde endoplasmic reticulum-Golgi pathway in tobacco leaf epidermal cells. Plant Physiol 139: 1244–1254 Chow CM, Neto H, Foucart C, Moore I (2008) Rab-A2 and Rab-A3 GTPases define a trans-Golgi endosomal membrane domain in Arabidopsis that contributes substantially to the cell plate. Plant Cell 20: 101–123 Contreras I, Ortiz-Zapater E, Aniento F (2004a) Sorting signals in the cytosolic tail of membrane proteins involved in the interaction with plant ARF1 and coatomer. Plant J 38: 685–698[CrossRef][Web of Science][Medline] Contreras I, Yang Y, Robinson DG, Aniento F (2004b) Sorting signals in the cytosolic tail of plant p24 proteins involved in the interaction with the COPII coat. Plant Cell Physiol 45: 1779–1786 Cosson P, Schroder-Kohne S, Sweet DS, Demolliere C, Hennecke S, Frigerio G, Letourneur F (1997) The Sec20/Tip20p complex is involved in ER retrieval of dilysine-tagged proteins. Eur J Cell Biol 73: 93–97[Web of Science][Medline] Craddock CP, Hunter PR, Szakacs E, Hinz G, Robinson DG, Frigerio L (2008) Lack of a vacuolar sorting receptor leads to non-specific missorting of soluble vacuolar proteins in Arabidopsis seeds. Traffic 9: 408–416[CrossRef][Web of Science][Medline] Crofts AJ, Leborgne-Castel N, Hillmer S, Robinson DG, Phillipson B, Carlsson LE, Ashford DA, Denecke J (1999) Saturation of the endoplasmic reticulum retention machinery reveals anterograde bulk flow. Plant Cell 11: 2233–2248 Dacks JB, Poon PP, Field MC (2008) Phylogeny of endocytic components yields insight into the process of nonendosymbiotic organelle evolution. Proc Natl Acad Sci USA 105: 588–593 daSilva LL, Foresti O, Denecke J (2006) Targeting of the plant vacuolar sorting receptor BP80 is dependent on multiple sorting signals in the cytosolic tail. Plant Cell 18: 1477–1497 daSilva LL, Taylor JP, Hadlington JL, Hanton SL, Snowden CJ, Fox SJ, Foresti O, Brandizzi F, Denecke J (2005) Receptor salvage from the prevacuolar compartment is essential for efficient vacuolar protein targeting. Plant Cell 17: 132–148 Denecke J, Botterman J, Deblaere R (1990) Protein secretion in plant cells can occur via a default pathway. Plant Cell 2: 51–59 Dettmer J, Hong-Hermesdorf A, Stierhof YD, Schumacher K (2006) Vacuolar H+-ATPase activity is required for endocytic and secretory trafficking in Arabidopsis. Plant Cell 18: 715–730 Di Sansebastiano GP, Paris N, Marc-Martin S, Neuhaus JM (2001) Regeneration of a lytic central vacuole and of neutral peripheral vacuoles can be visualized by green fluorescent proteins targeted to either type of vacuoles. Plant Physiol 126: 78–86 Epimashko S, Meckel T, Fischer-Schliebs E, Luttge U, Thiel G (2004) Two functionally different vacuoles for static and dynamic purposes in one plant mesophyll leaf cell. Plant J 37: 294–300[Web of Science][Medline] Foresti O, Dasilva LL, Denecke J (2006) Overexpression of the Arabidopsis syntaxin PEP12/SYP21 inhibits transport from the prevacuolar compartment to the lytic vacuole in vivo. Plant Cell 18: 2275–2293 Frigerio G (1998) The Saccharomyces cerevisiae early secretion mutant tip20 is synthetic lethal with mutants in yeast coatomer and the SNARE proteins Sec22p and Ufe1p. Yeast 14: 633–646[CrossRef][Web of Science][Medline] Fuji K, Shimada T, Takahashi H, Tamura K, Koumoto Y, Utsumi S, Nishizawa K, Maruyama N, Hara-Nishimura I (2007) Arabidopsis vacuolar sorting mutants (green fluorescent seed) can be identified efficiently by secretion of vacuole-targeted green fluorescent protein in their seeds. Plant Cell 19: 597–609 Geldner N, Anders N, Wolters H, Keicher J, Kornberger W, Muller P, Delbarre A, Ueda T, Nakano A, Jurgens G (2003) The Arabidopsis GNOM ARF-GEF mediates endosomal recycling, auxin transport, and auxin-dependent plant growth. Cell 112: 219–230[CrossRef][Web of Science][Medline] Goh T, Uchida W, Arakawa S, Ito E, Dainobu T, Ebine K, Takeuchi M, Sato K, Ueda T, Nakano A (2007) VPS9a, the common activator for two distinct types of Rab5 GTPases, is essential for the development of Arabidopsis thaliana. Plant Cell 19: 3504–3515 Gomez L, Chrispeels MJ (1993) Tonoplast and soluble vacuolar proteins are targeted by different mechanisms. Plant Cell 5: 1113–1124 Haas TJ, Sliwinski MK, Martinez DE, Preuss M, Ebine K, Ueda T, Nielsen E, Odorizzi G, Otegui MS (2007) The Arabidopsis AAA ATPase SKD1 is involved in multivesicular endosome function and interacts with its positive regulator LYST-INTERACTING PROTEIN5. Plant Cell 19: 1295–1312 Hanton SL, Renna L, Bortolotti LE, Chatre L, Stefano G, Brandizzi F (2005) Diacidic motifs influence the export of transmembrane proteins from the endoplasmic reticulum in plant cells. Plant Cell 17: 3081–3093 Happel N, Honing S, Neuhaus JM, Paris N, Robinson DG, Holstein SE (2004) Arabidopsis mu A-adaptin interacts with the tyrosine motif of the vacuolar sorting receptor VSR-PS1. Plant J 37: 678–693[CrossRef][Web of Science][Medline] Hara-Nishimura II, Shimada T, Hatano K, Takeuchi Y, Nishimura M (1998) Transport of storage proteins to protein storage vacuoles is mediated by large precursor-accumulating vesicles. Plant Cell 10: 825–836 Hinz G, Colanesi S, Hillmer S, Rogers JC, Robinson DG (2007) Localization of vacuolar transport receptors and cargo proteins in the Golgi apparatus of developing Arabidopsis embryos. Traffic 8: 1452–1464[CrossRef][Web of Science][Medline] Hofte H, Chrispeels MJ (1992) Protein sorting to the vacuolar membrane. Plant Cell 4: 995–1004 Hoh B, Hinz G, Jeong BK, Robinson DG (1995) Protein storage vacuoles form de novo during pea cotyledon development. J Cell Sci 108: 299–310[Abstract] Hunter PR, Craddock CP, Di Benedetto S, Roberts LM, Frigerio L (2007) Fluorescent reporter proteins for the tonoplast and the vacuolar lumen identify a single vacuolar compartment in Arabidopsis cells. Plant Physiol 145: 1371–1382 Jaillais Y, Santambrogio M, Rozier F, Fobis-Loisy I, Miege C, Gaude T (2007) The retromer protein VPS29 links cell polarity and organ initiation in plants. Cell 130: 1057–1070[CrossRef][Web of Science][Medline] Jolliffe NA, Brown JC, Neumann U, Vicre M, Bachi A, Hawes C, Ceriotti A, Roberts LM, Frigerio L (2004) Transport of ricin and 2S albumin precursors to the storage vacuoles of Ricinus communis endosperm involves the Golgi and VSR-like receptors. Plant J 39: 821–833[CrossRef][Web of Science][Medline] Jones S, Litt RJ, Richardson CJ, Segev N (1995) Requirement of nucleotide exchange factor for Ypt1 GTPase mediated protein transport. J Cell Biol 130: 1051–1061 Kalde M, Nuhse TS, Findlay K, Peck SC (2007) The syntaxin SYP132 contributes to plant resistance against bacteria and secretion of pathogenesis-related protein 1. Proc Natl Acad Sci USA 104: 11850–11855 Kamena F, Spang A (2004) Tip20p prohibits back-fusion of COPII vesicles with the endoplasmic reticulum. Science 304: 286–289 Kirsch T, Saalbach G, Raikhel NV, Beevers L (1996) Interaction of a potential vacuolar targeting receptor with amino- and carboxyl-terminal targeting determinants. Plant Physiol 111: 469–474[Abstract] Kotzer AM, Brandizzi F, Neumann U, Paris N, Moore I, Hawes C (2004) AtRabF2b (Ara7) acts on the vacuolar trafficking pathway in tobacco leaf epidermal cells. J Cell Sci 117: 6377–6389 Kraynack BA, Chan A, Rosenthal E, Essid M, Umansky B, Waters MG, Schmitt HD (2005) Dsl1p, Tip20p, and the novel Dsl3(Sec39) protein are required for the stability of the Q/t-SNARE complex at the endoplasmic reticulum in yeast. Mol Biol Cell 16: 3963–3977 Lam SK, Siu CL, Hillmer S, Jang S, An G, Robinson DG, Jiang L (2007a) Rice SCAMP1 defines clathrin-coated, trans-Golgi-located tubular-vesicular structures as an early endosome in tobacco BY-2 cells. Plant Cell 19: 296–319 Lam SK, Tse YC, Robinson DG, Jiang L (2007b) Tracking down the elusive early endosome. Trends Plant Sci 12: 497–505[CrossRef][Medline] Langhans M, Marcote MJ, Pimpl P, Virgili-Lopez G, Robinson DG, Aniento F (2008) In vivo trafficking and localization of p24 proteins in plant cells. Traffic 9: 770–785[CrossRef][Web of Science][Medline] Leshem Y, Melamed-Book N, Cagnac O, Ronen G, Nishri Y, Solomon M, Cohen G, Levine A (2006) Suppression of Arabidopsis vesicle-SNARE expression inhibited fusion of H2O2-containing vesicles with tonoplast and increased salt tolerance. Proc Natl Acad Sci USA 103: 18008–18013 Leucci MR, Di Sansebastiano GP, Gigante M, Dalessandro G, Piro G (2007) Secretion marker proteins and cell-wall polysaccharides move through different secretory pathways. Planta 225: 1001–1017[CrossRef][Web of Science][Medline] Li L, Shimada T, Takahashi H, Ueda H, Fukao Y, Kondo M, Nishimura M, Hara-Nishimura I (2006) MAIGO2 is involved in exit of seed storage proteins from the endoplasmic reticulum in Arabidopsis thaliana. Plant Cell 18: 3535–3547 Manfield IW, Jen CH, Pinney JW, Michalopoulos I, Bradford JR, Gilmartin PM, Westhead DR (2006) Arabidopsis Co-expression Tool (ACT): web server tools for microarray-based gene expression analysis. Nucleic Acids Res (Web Server issue) 34: W504–W509 Marty F (1999) Plant vacuoles. Plant Cell 11: 587–600 Matsuoka K, Bassham DC, Raikhel NV, Nakamura K (1995) Different sensitivity to wortmannin of two vacuolar sorting signals indicates the presence of distinct sorting machineries in tobacco cells. J Cell Biol 130: 1307–1318 Mouratou B, Biou V, Joubert A, Cohen J, Shields DJ, Geldner N, Jurgens G, Melancon P, Cherfils J (2005) The domain architecture of large guanine nucleotide exchange factors for the small GTP-binding protein Arf. BMC Genomics 6: 20[CrossRef][Medline] Nebenfuhr A, Staehelin LA (2001) Mobile factories: Golgi dynamics in plant cells. Trends Plant Sci 6: 160–167[CrossRef][Web of Science][Medline] Newell-Litwa K, Seong E, Burmeister M, Faundez V (2007) Neuronal and non-neuronal functions of the AP-3 sorting machinery. J Cell Sci 120: 531–541 Nielsen E, Cheung AY, Ueda T (2008) The regulatory RAB and ARF GTPases for vesicular trafficking. Plant Physiol 147: 1516–1526 Niihama M, Uemura T, Saito C, Nakano A, Sato MH, Tasaka M, Morita MT (2005) Conversion of functional specificity in Qb-SNARE VTI1 homologues of Arabidopsis. Curr Biol 15: 555–560[CrossRef][Web of Science][Medline] Olbrich A, Hillmer S, Hinz G, Oliviusson P, Robinson DG (2007) Newly formed vacuoles in root meristems of barley and pea seedlings have characteristics of both protein storage and lytic vacuoles. Plant Physiol 145: 1383–1394 Otegui MS, Herder R, Schulze J, Jung R, Staehelin LA (2006) The proteolytic processing of seed storage proteins in Arabidopsis embryo cells starts in the multivesicular bodies. Plant Cell 18: 2567–2581 Paris N, Stanley CM, Jones RL, Rogers JC (1996) Plant cells contain two functionally distinct vacuolar compartments. Cell 85: 563–572[CrossRef][Web of Science][Medline] Park JH, Oufattole M, Rogers JC (2007) Golgi-mediated vacuolar sorting in plant cells: RMR proteins are sorting receptors for the protein aggregation/membrane internalization pathway. Plant Sci 172: 728–745 Park M, Kim SJ, Vitale A, Hwang I (2004) Identification of the protein storage vacuole and protein targeting to the vacuole in leaf cells of three plant species. Plant Physiol 134: 625–639 Park M, Lee D, Lee GJ, Hwang I (2005) AtRMR1 functions as a cargo receptor for protein trafficking to the protein storage vacuole. J Cell Biol 170: 757–767 Phillipson BA, Pimpl P, daSilva LL, Crofts AJ, Taylor JP, Movafeghi A, Robinson DG, Denecke J (2001) Secretory bulk flow of soluble proteins is efficient and COPII dependent. Plant Cell 13: 2005–2020 Pimpl P, Hanton SL, Taylor JP, Pinto-daSilva LL, Denecke J (2003) The GTPase ARF1p controls the sequence-specific vacuolar sorting route to the lytic vacuole. Plant Cell 15: 1242–1256 Pimpl P, Taylor JP, Snowden C, Hillmer S, Robinson DG, Denecke J (2006) Golgi-mediated vacuolar sorting of the endoplasmic reticulum chaperone BiP may play an active role in quality control within the secretory pathway. Plant Cell 18: 198–211 Richardson CJ, Jones S, Litt RJ, Segev N (1998) GTP hydrolysis is not important for Ypt1 GTPase function in vesicular transport. Mol Cell Biol 18: 827–838 Richter S, Geldner N, Schrader J, Wolters H, Stierhof YD, Rios G, Koncz C, Robinson DG, Jurgens G (2007) Functional diversification of closely related ARF-GEFs in protein secretion and recycling. Nature 448: 488–492[CrossRef][Web of Science][Medline] Rojas-Pierce M, Titapiwatanakun B, Sohn EJ, Fang F, Larive CK, Blakeslee J, Cheng Y, Cutler SR, Peer WA, Murphy AS, et al (2007) Arabidopsis P-glycoprotein19 participates in the inhibition of gravitropism by gravacin. Chem Biol 14: 1366–1376[CrossRef][Web of Science][Medline] Rojo E, Gillmor CS, Kovaleva V, Somerville CR, Raikhel NV (2001) VACUOLELESS1 is an essential gene required for vacuole formation and morphogenesis in Arabidopsis. Dev Cell 1: 303–310[CrossRef][Web of Science][Medline] Rutherford S, Moore I (2002) The Arabidopsis Rab GTPase family: another enigma variation. Curr Opin Plant Biol 5: 518–528[CrossRef][Web of Science][Medline] Saint-Jore-Dupas C, Nebenfuhr A, Boulaflous A, Follet-Gueye ML, Plasson C, Hawes C, Driouich A, Faye L, Gomord V (2006) Plant N-glycan processing enzymes employ different targeting mechanisms for their spatial arrangement along the secretory pathway. Plant Cell 18: 3182–3200 Saito C, Ueda T, Abe H, Wada Y, Kuroiwa T, Hisada A, Furuya M, Nakano A (2002) A complex and mobile structure forms a distinct subregion within the continuous vacuolar membrane in young cotyledons of Arabidopsis. Plant J 29: 245–255[CrossRef][Web of Science][Medline] Sanderfoot A (2007) Increases in the number of SNARE genes parallels the rise of multicellularity among the green plants. Plant Physiol 144: 6–17 Sanderfoot AA, Ahmed SU, Marty-Mazars D, Rapoport I, Kirchhausen T, Marty F, Raikhel NV (1998) A putative vacuolar cargo receptor partially colocalizes with AtPEP12p on a prevacuolar compartment in Arabidopsis roots. Proc Natl Acad Sci USA 95: 9920–9925 Sanderfoot AA, Pilgrim M, Adam L, Raikhel NV (2001) Disruption of individual members of Arabidopsis syntaxin gene families indicates each has essential functions. Plant Cell 13: 659–666 Sanmartin M, Ordonez A, Sohn EJ, Robert S, Sanchez-Serrano JJ, Surpin MA, Raikhel NV, Rojo E (2007) Divergent functions of VTI12 and VTI11 in trafficking to storage and lytic vacuoles in Arabidopsis. Proc Natl Acad Sci USA 104: 3645–3650 Shimada T, Fuji K, Tamura K, Kondo M, Nishimura M, Hara-Nishimura I (2003) Vacuolar sorting receptor for seed storage proteins in Arabidopsis thaliana. Proc Natl Acad Sci USA 100: 16095–16100 Shimada T, Koumoto Y, Li L, Yamazaki M, Kondo M, Nishimura M, Hara-Nishimura I (2006) AtVPS29, a putative component of a retromer complex, is required for the efficient sorting of seed storage proteins. Plant Cell Physiol 47: 1187–1194 Sohn EJ, Rojas-Pierce M, Pan S, Carter C, Serrano-Mislata A, Madueno F, Rojo E, Surpin M, Raikhel NV (2007) The shoot meristem identity gene TFL1 is involved in flower development and trafficking to the protein storage vacuole. Proc Natl Acad Sci USA 104: 18801–18806 Stefanovic S, Hegde RS (2007) Identification of a targeting factor for posttranslational membrane protein insertion into the ER. Cell 128: 1147–1159[CrossRef][Medline] Surpin M, Zheng H, Morita MT, Saito C, Avila E, Blakeslee JJ, Bandyopadhyay A, Kovaleva V, Carter D, Murphy A, et al (2003) The VTI family of SNARE proteins is necessary for plant viability and mediates different protein transport pathways. Plant Cell 15: 2885–2899 Tamura K, Shimada T, Kondo M, Nishimura M, Hara-Nishimura I (2005) KATAMARI1/MURUS3 is a novel Golgi membrane protein that is required for endomembrane organization in Arabidopsis. Plant Cell 17: 1764–1776 Tamura K, Takahashi H, Kunieda T, Fuji K, Shimada T, Hara-Nishimura I (2007) Arabidopsis KAM2/GRV2 is required for proper endosome formation and functions in vacuolar sorting and determination of the embryo growth axis. Plant Cell 19: 320–332 Tamura K, Shimada T, Ono E, Tanaka Y, Nagatani A, Higashi SI, Watanabe M, Nishimura M, Hara-Nishimura I (2003) Why green fluorescent fusion proteins have not been observed in the vacuoles of higher plants. Plant J 35: 545–555[CrossRef][Web of Science][Medline] Teh OK, Moore I (2007) An ARF-GEF acting at the Golgi and in selective endocytosis in polarized plant cells. Nature 448: 493–496[CrossRef][Web of Science][Medline] Tyrrell M, Campanoni P, Sutter JU, Pratelli R, Paneque M, Sokolovski S, Blatt MR (2007) Selective targeting of plasma membrane and tonoplast traffic by inhibitory (dominant-negative) SNARE fragments. Plant J 51: 1099–1115[CrossRef][Web of Science][Medline] Ueda T, Uemura T, Sato MH, Nakano A (2004) Functional differentiation of endosomes in Arabidopsis cells. Plant J 40: 783–789[CrossRef][Web of Science][Medline] Ueda T, Yamaguchi M, Uchimiya H, Nakano A (2001) Ara6, a plant-unique novel type Rab GTPase, functions in the endocytic pathway of Arabidopsis thaliana. EMBO J 20: 4730–4741[CrossRef][Web of Science][Medline] Uemura T, Ueda T, Ohniwa RL, Nakano A, Takeyasu K, Sato MH (2004) Systematic analysis of SNARE molecules in Arabidopsis: dissection of the post-Golgi network in plant cells. Cell Struct Funct 29: 49–65[CrossRef][Web of Science][Medline] Vernoud V, Horton AC, Yang Z, Nielsen E (2003) Analysis of the small GTPase gene superfamily of Arabidopsis. Plant Physiol 131: 1191–1208 Vitale A, Hinz G (2005) Sorting of proteins to storage vacuoles: how many mechanisms? Trends Plant Sci 10: 316–323[CrossRef][Web of Science][Medline] Yamazaki M, Shimada T, Takahashi H, Tamura K, Kondo M, Nishimura M, Hara-Nishimura I (2008) Arabidopsis VPS35, a retromer component, is required for vacuolar protein sorting and involved in plant growth and leaf senescence. Plant Cell Physiol 49: 142–156 Zheng H, Kunst L, Hawes C, Moore I (2004) A GFP-based assay reveals a role for RHD3 in transport between the endoplasmic reticulum and Golgi apparatus. Plant J 37: 398–414[CrossRef][Web of Science][Medline] This article has been cited by other articles:
|
||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||
| HOME | HELP | FEEDBACK | SUBSCRIPTIONS | ARCHIVE | SEARCH | TABLE OF CONTENTS |
| ASPB Publications | PLANT PHYSIOLOGY® | THE PLANT CELL | |
|---|---|---|---|
-amylase; Aleu-GFP, first 143 amino acids from barley aleurain containing the signal peptide and the sequence-specific vacuolar sorting signal fused to GFP; ST, rat sialyl transferase; GFP-2SC, GFP with a signal peptide fused to the C-terminal propeptide from pumpkin 2S albumin; GFP-CT24, GFP with the signal peptide and the C-terminal 24 amino acids of soybean (Glycine max) (R)-conglycinin; PHT1-GFP, Arabidopsis phosphate transporter PHT1;1 fused to GFP; Inv-GFP, tobacco secreted invertase fused to GFP; PAT, phosphinothricin acetyl transferase; SynA-GFP, synthetic arabinogalactan protein fused to GFP; GFP-CTPPBL, GFP with a signal peptide fused to the C-terminal propeptide from barley lectin; BL, barley lectin; GFP-CHI, GFP with a signal peptide fused to the vacuolar sorting signal from tobacco chitinase-A.
TOP
LOSS-OF-FUNCTION MUTANTS...
DOMINANT AND SEMIDOMINANT...
-adaptin of the AP-3 adaptor complex and may therefore be involved in vacuolar cargo exit from an endosomal compartment (Newell-Litwa et al., 2007
signal for clathrin-mediated transport that is required for in vitro binding to µ-adaptin (Happel et al., 2004
