The Arabidopsis Endosomal Sorting Complex Required for Transport III Regulates Internal Vesicle Formation of the Prevacuolar Compartment and Is Required for Plant Development

We have established an efficient transient expression system with several vacuolar reporters to study the roles of endosomal sorting complex required for transport (ESCRT)-III subunits in regulating the formation of intraluminal vesicles of prevacuolar compartments (PVCs)/multivesicular bodies (MVBs) in plant cells. By measuring the distributions of reporters on/within the membrane of PVC/MVB or tonoplast, we have identified dominant negative mutants of ESCRT-III subunits that affect membrane protein degradation from both secretory and endocytic pathways. In addition, induced expression of these mutants resulted in reduction in luminal vesicles of PVC/MVB, along with increased detection of membrane-attaching vesicles inside the PVC/MVB. Transgenic Arabidopsis (Arabidopsis thaliana) plants with induced expression of ESCRT-III dominant negative mutants also displayed severe cotyledon developmental defects with reduced cell size, loss of the central vacuole, and abnormal chloroplast development in mesophyll cells, pointing out an essential role of the ESCRT-III complex in postembryonic development in plants. Finally, membrane dissociation of ESCRT-III components is important for their biological functions and is regulated by direct interaction among Vacuolar Protein Sorting-Associated Protein20-1 (VPS20.1), Sucrose Nonfermenting7-1, VPS2.1, and the adenosine triphosphatase VPS4/SUPPRESSOR OF K⁺ TRANSPORT GROWTH DEFECT1.Endomembrane trafficking in plant cells is complicated such that secretory, endocytic, and recycling pathways are usually integrated with each other at the post-Golgi compartments, among which, the trans-Golgi network (TGN) and prevacuolar compartment (PVC)/multivesicular body (MVB) are best studied (Tse et al., 2004; Lam et al., 2007a, 2007b; Müller et al., 2007; Foresti and Denecke, 2008; Hwang, 2008; Otegui and Spitzer, 2008; Robinson et al., 2008; Richter et al., 2009; Ding et al., 2012; Gao et al., 2014). Following the endocytic trafficking of a lipophilic dye, FM4-64, the TGN and PVC/MVB are sequentially labeled and thus are defined as the early and late endosome, respectively, in plant cells (Lam et al., 2007a; Chow et al., 2008). While the TGN is a tubular vesicular-like structure that may include several different microdomains and fit its biological function as a sorting station (Chow et al., 2008; Kang et al., 2011), the PVC/MVB is 200 to 500 nm in size with multiple luminal vesicles of approximately 40 nm (Tse et al., 2004). Membrane cargoes destined for degradation are sequestered into these tiny luminal vesicles and delivered to the lumen of the lytic vacuole (LV) via direct fusion between the PVC/MVB and the LV (Spitzer et al., 2009; Viotti et al., 2010; Cai et al., 2012). Therefore, the PVC/MVB functions between the TGN and LV as an intermediate organelle and decides the fate of membrane cargoes in the LV.In yeast (Saccharomyces cerevisiae), carboxypeptidase S (CPS) is synthesized as a type II integral membrane protein and sorted from the Golgi to the lumen of the vacuole (Spormann et al., 1992). Genetic analyses on the trafficking of CPS have led to the identification of approximately 17 class E genes (Piper et al., 1995; Babst et al., 1997, 2002a, 2002b; Odorizzi et al., 1998; Katzmann et al., 2001) that constitute the core endosomal sorting complex required for transport (ESCRT) machinery. The evolutionarily conserved ESCRT complex consists of several functionally different subcomplexes, ESCRT-0, ESCRT-I, ESCRT-II, and ESCRT-III and the ESCRT-III-associated/Vacuolar Protein Sorting4 (VPS4) complex. Together, they form a complex protein-protein interaction network that coordinates sorting of cargoes and inward budding of the membrane on the MVB (Hurley and Hanson, 2010; Henne et al., 2011). Cargo proteins carrying ubiquitin signals are thought to be passed from one ESCRT subcomplex to the next, starting with their recognition by ESCRT-0 (Bilodeau et al., 2002, 2003; Hislop and von Zastrow, 2011; Le Bras et al., 2011; Shields and Piper, 2011; Urbé, 2011). ESCRT-0 recruits the ESCRT-I complex, a heterotetramer of VPS23, VPS28, VPS37, and MVB12, from the cytosol to the endosomal membrane (Katzmann et al., 2001, 2003). The C terminus of VPS28 interacts with the N terminus of VPS36, a member of the ESCRT-II complex (Kostelansky et al., 2006; Teo et al., 2006). Then, cargoes passed from ESCRT-I and ESCRT-II are concentrated in certain membrane domains of the endosome by ESCRT-III, which includes four coiled-coil proteins and is sufficient to induce the membrane invagination (Babst et al., 2002b; Saksena et al., 2009; Wollert et al., 2009). Finally, the ESCRT components are disassociated from the membrane by the adenosine triphosphatase (ATPase) associated with diverse cellular activities (AAA) VPS4/SUPPRESSOR OF K+ TRANSPORT GROWTH DEFECT1 (SKD1) before releasing the internal vesicles (Babst et al., 1997, 1998).Putative homologs of ESCRT-I–ESCRT-III and ESCRT-III-associated components have been identified in plants, except for ESCRT-0, which is only present in Opisthokonta (Winter and Hauser, 2006; Leung et al., 2008; Schellmann and Pimpl, 2009). To date, only a few plant ESCRT components have been studied in detail. The Arabidopsis (Arabidopsis thaliana) AAA ATPase SKD1 localized to the PVC/MVB and showed ATPase activity that was regulated by Lysosomal Trafficking Regulator-Interacting Protein5, a plant homolog of Vps Twenty Associated1 Protein (Haas et al., 2007). Expression of the dominant negative form of SKD1 caused an increase in the size of the MVB and a reduction in the number of internal vesicles (Haas et al., 2007). This protein also contributes to the maintenance of the central vacuole and might be associated with cell cycle regulation, as leaf trichomes expressing its dominant negative mutant form lost the central vacuole and frequently contained multiple nuclei (Shahriari et al., 2010). Double null mutants of CHARGED MULTIVESICULAR BODY PROTEIN, chmp1achmp1b, displayed severe growth defects and were seedling lethal. This may be due to the mislocalization of plasma membrane (PM) proteins, including those involved in auxin transport such as PINFORMED1, PINFORMED2, and AUXIN-RESISTANT1, from the vacuolar degradation pathway to the tonoplast of the LV (Spitzer et al., 2009).Plant ESCRT components usually contain several homologs, with the possibility of functional redundancy. Single mutants of individual ESCRT components may not result in an obvious phenotype, whereas knockout of all homologs of an ESCRT component by generating double or triple mutants may be lethal to the plant. As a first step to carry out systematic analysis on each ESCRT complex in plant cells, here, we established an efficient analysis system to monitor the localization changes of four vacuolar reporters that accumulate either in the lumen (LRR84A-GFP, EMP12-GFP, and aleurain-GFP) or on the tonoplast (GFP-VIT1) of the LV and identified several ESCRT-III dominant negative mutants. We reported that ESCRT-III subunits were involved in the release of PVC/MVB’s internal vesicles from the limiting membrane and were required for membrane protein degradation from secretory and endocytic pathways. In addition, transgenic Arabidopsis plants with induced expression of ESCRT-III dominant negative mutants showed severe cotyledon developmental defects. We also showed that membrane dissociation of ESCRT-III subunits was regulated by direct interaction with SKD1.     

Spore Density Determines Infection Strategy by the Plant Pathogenic Fungus Plectosphaerella cucumerina

Necrotrophic and biotrophic pathogens are resisted by different plant defenses. While necrotrophic pathogens are sensitive to jasmonic acid (JA)-dependent resistance, biotrophic pathogens are resisted by salicylic acid (SA)- and reactive oxygen species (ROS)-dependent resistance. Although many pathogens switch from biotrophy to necrotrophy during infection, little is known about the signals triggering this transition. This study is based on the observation that the early colonization pattern and symptom development by the ascomycete pathogen Plectosphaerella cucumerina (P. cucumerina) vary between inoculation methods. Using the Arabidopsis (Arabidopsis thaliana) defense response as a proxy for infection strategy, we examined whether P. cucumerina alternates between hemibiotrophic and necrotrophic lifestyles, depending on initial spore density and distribution on the leaf surface. Untargeted metabolome analysis revealed profound differences in metabolic defense signatures upon different inoculation methods. Quantification of JA and SA, marker gene expression, and cell death confirmed that infection from high spore densities activates JA-dependent defenses with excessive cell death, while infection from low spore densities induces SA-dependent defenses with lower levels of cell death. Phenotyping of Arabidopsis mutants in JA, SA, and ROS signaling confirmed that P. cucumerina is differentially resisted by JA- and SA/ROS-dependent defenses, depending on initial spore density and distribution on the leaf. Furthermore, in situ staining for early callose deposition at the infection sites revealed that necrotrophy by P. cucumerina is associated with elevated host defense. We conclude that P. cucumerina adapts to early-acting plant defenses by switching from a hemibiotrophic to a necrotrophic infection program, thereby gaining an advantage of immunity-related cell death in the host.Plant pathogens are often classified as necrotrophic or biotrophic, depending on their infection strategy (Glazebrook, 2005; Nishimura and Dangl, 2010). Necrotrophic pathogens kill living host cells and use the decayed plant tissue as a substrate to colonize the plant, whereas biotrophic pathogens parasitize living plant cells by employing effector molecules that suppress the host immune system (Pel and Pieterse, 2013). Despite this binary classification, the majority of pathogenic microbes employ a hemibiotrophic infection strategy, which is characterized by an initial biotrophic phase followed by a necrotrophic infection strategy at later stages of infection (Perfect and Green, 2001). The pathogenic fungi Magnaporthe grisea, Sclerotinia sclerotiorum, and Mycosphaerella graminicola, the oomycete Phytophthora infestans, and the bacterial pathogen Pseudomonas syringae are examples of hemibiotrophic plant pathogens (Perfect and Green, 2001; Koeck et al., 2011; van Kan et al., 2014; Kabbage et al., 2015).Despite considerable progress in our understanding of plant resistance to necrotrophic and biotrophic pathogens (Glazebrook, 2005; Mengiste, 2012; Lai and Mengiste, 2013), recent debate highlights the dynamic and complex interplay between plant-pathogenic microbes and their hosts, which is raising concerns about the use of infection strategies as a static tool to classify plant pathogens. For instance, the fungal genus Botrytis is often labeled as an archetypal necrotroph, even though there is evidence that it can behave as an endophytic fungus with a biotrophic lifestyle (van Kan et al., 2014). The rice blast fungus Magnaporthe oryzae, which is often classified as a hemibiotrophic leaf pathogen (Perfect and Green, 2001; Koeck et al., 2011), can adopt a purely biotrophic lifestyle when infecting root tissues (Marcel et al., 2010). It remains unclear which signals are responsible for the switch from biotrophy to necrotrophy and whether these signals rely solely on the physiological state of the pathogen, or whether host-derived signals play a role as well (Kabbage et al., 2015).The plant hormones salicylic acid (SA) and jasmonic acid (JA) play a central role in the activation of plant defenses (Glazebrook, 2005; Pieterse et al., 2009, 2012). The first evidence that biotrophic and necrotrophic pathogens are resisted by different immune responses came from Thomma et al. (1998), who demonstrated that Arabidopsis (Arabidopsis thaliana) genotypes impaired in SA signaling show enhanced susceptibility to the biotrophic pathogen Hyaloperonospora arabidopsidis (formerly known as Peronospora parastitica), while JA-insensitive genotypes were more susceptible to the necrotrophic fungus Alternaria brassicicola. In subsequent years, the differential effectiveness of SA- and JA-dependent defense mechanisms has been confirmed in different plant-pathogen interactions, while additional plant hormones, such as ethylene, abscisic acid (ABA), auxins, and cytokinins, have emerged as regulators of SA- and JA-dependent defenses (Bari and Jones, 2009; Cao et al., 2011; Pieterse et al., 2012). Moreover, SA- and JA-dependent defense pathways have been shown to act antagonistically on each other, which allows plants to prioritize an appropriate defense response to attack by biotrophic pathogens, necrotrophic pathogens, or herbivores (Koornneef and Pieterse, 2008; Pieterse et al., 2009; Verhage et al., 2010).In addition to plant hormones, reactive oxygen species (ROS) play an important regulatory role in plant defenses (Torres et al., 2006; Lehmann et al., 2015). Within minutes after the perception of pathogen-associated molecular patterns, NADPH oxidases and apoplastic peroxidases generate early ROS bursts (Torres et al., 2002; Daudi et al., 2012; O’Brien et al., 2012), which activate downstream defense signaling cascades (Apel and Hirt, 2004; Torres et al., 2006; Miller et al., 2009; Mittler et al., 2011; Lehmann et al., 2015). ROS play an important regulatory role in the deposition of callose (Luna et al., 2011; Pastor et al., 2013) and can also stimulate SA-dependent defenses (Chaouch et al., 2010; Yun and Chen, 2011; Wang et al., 2014; Mammarella et al., 2015). However, the spread of SA-induced apoptosis during hyperstimulation of the plant immune system is contained by the ROS-generating NADPH oxidase RBOHD (Torres et al., 2005), presumably to allow for the sufficient generation of SA-dependent defense signals from living cells that are adjacent to apoptotic cells. Nitric oxide (NO) plays an additional role in the regulation of SA/ROS-dependent defense (Trapet et al., 2015). This gaseous molecule can stimulate ROS production and cell death in the absence of SA while preventing excessive ROS production at high cellular SA levels via S-nitrosylation of RBOHD (Yun et al., 2011). Recently, it was shown that pathogen-induced accumulation of NO and ROS promotes the production of azelaic acid, a lipid derivative that primes distal plants for SA-dependent defenses (Wang et al., 2014). Hence, NO, ROS, and SA are intertwined in a complex regulatory network to mount local and systemic resistance against biotrophic pathogens. Interestingly, pathogens with a necrotrophic lifestyle can benefit from ROS/SA-dependent defenses and associated cell death (Govrin and Levine, 2000). For instance, Kabbage et al. (2013) demonstrated that S. sclerotiorum utilizes oxalic acid to repress oxidative defense signaling during initial biotrophic colonization, but it stimulates apoptosis at later stages to advance necrotrophic colonization. Moreover, SA-induced repression of JA-dependent resistance not only benefits necrotrophic pathogens but also hemibiotrophic pathogens after having switched from biotrophy to necrotrophy (Glazebrook, 2005; Pieterse et al., 2009, 2012).Plectosphaerella cucumerina ((P. cucumerina, anamorph Plectosporum tabacinum) anamorph Plectosporum tabacinum) is a filamentous ascomycete fungus that can survive saprophytically in soil by decomposing plant material (Palm et al., 1995). The fungus can cause sudden death and blight disease in a variety of crops (Chen et al., 1999; Harrington et al., 2000). Because P. cucumerina can infect Arabidopsis leaves, the P. cucumerina-Arabidopsis interaction has emerged as a popular model system in which to study plant defense reactions to necrotrophic fungi (Berrocal-Lobo et al., 2002; Ton and Mauch-Mani, 2004; Carlucci et al., 2012; Ramos et al., 2013). Various studies have shown that Arabidopsis deploys a wide range of inducible defense strategies against P. cucumerina, including JA-, SA-, ABA-, and auxin-dependent defenses, glucosinolates (Tierens et al., 2001; Sánchez-Vallet et al., 2010; Gamir et al., 2014; Pastor et al., 2014), callose deposition (García-Andrade et al., 2011; Gamir et al., 2012, 2014; Sánchez-Vallet et al., 2012), and ROS (Tierens et al., 2002; Sánchez-Vallet et al., 2010; Barna et al., 2012; Gamir et al., 2012, 2014; Pastor et al., 2014). Recent metabolomics studies have revealed large-scale metabolic changes in P. cucumerina-infected Arabidopsis, presumably to mobilize chemical defenses (Sánchez-Vallet et al., 2010; Gamir et al., 2014; Pastor et al., 2014). Furthermore, various chemical agents have been reported to induce resistance against P. cucumerina. These chemicals include β-amino-butyric acid, which primes callose deposition and SA-dependent defenses, benzothiadiazole (BTH or Bion; Görlach et al., 1996; Ton and Mauch-Mani, 2004), which activates SA-related defenses (Lawton et al., 1996; Ton and Mauch-Mani, 2004; Gamir et al., 2014; Luna et al., 2014), JA (Ton and Mauch-Mani, 2004), and ABA, which primes ROS and callose deposition (Ton and Mauch-Mani, 2004; Pastor et al., 2013). However, among all these studies, there is increasing controversy about the exact signaling pathways and defense responses contributing to plant resistance against P. cucumerina. While it is clear that JA and ethylene contribute to basal resistance against the fungus, the exact roles of SA, ABA, and ROS in P. cucumerina resistance vary between studies (Thomma et al., 1998; Ton and Mauch-Mani, 2004; Sánchez-Vallet et al., 2012; Gamir et al., 2014).This study is based on the observation that the disease phenotype during P. cucumerina infection differs according to the inoculation method used. We provide evidence that the fungus follows a hemibiotrophic infection strategy when infecting from relatively low spore densities on the leaf surface. By contrast, when challenged by localized host defense to relatively high spore densities, the fungus switches to a necrotrophic infection program. Our study has uncovered a novel strategy by which plant-pathogenic fungi can take advantage of the early immune response in the host plant.     

The Endoplasmic Reticulum Is a Reservoir for WAVE/SCAR Regulatory Complex Signaling in the Arabidopsis Leaf

During plant cell morphogenesis, signal transduction and cytoskeletal dynamics interact to locally organize the cytoplasm and define the geometry of cell expansion. The WAVE/SCAR (for WASP family verprolin homologous/suppressor of cyclic AMP receptor) regulatory complex (W/SRC) is an evolutionarily conserved heteromeric protein complex. Within the plant kingdom W/SRC is a broadly used effector that converts Rho-of-Plants (ROP)/Rac small GTPase signals into Actin-Related Protein2/3 and actin-dependent growth responses. Although the components and biochemistry of the W/SRC pathway are well understood, a basic understanding of how cells partition W/SRC into active and inactive pools is lacking. In this paper, we report that the endoplasmic reticulum (ER) is an important organelle for W/SRC regulation. We determined that a large intracellular pool of the core W/SRC subunit NAP1, like the known positive regulator of W/SRC, the DOCK family guanine nucleotide-exchange factor SPIKE1 (SPK1), localizes to the surface of the ER. The ER-associated NAP1 is inactive because it displays little colocalization with the actin network, and ER localization requires neither activating signals from SPK1 nor a physical association with its W/SRC-binding partner, SRA1. Our results indicate that in Arabidopsis (Arabidopsis thaliana) leaf pavement cells and trichomes, the ER is a reservoir for W/SRC signaling and may have a key role in the early steps of W/SRC assembly and/or activation.The W/SRC (for WASP family verprolin homologous/suppressor of cAMP receptor regulatory complex) and Actin-Related Protein (ARP)2/3 complex are part of an evolutionarily conserved Rho-of-Plants (ROP)/Rac small GTPase signal transduction cascade that controls actin-dependent morphogenesis in a wide variety of tissues and developmental contexts (Smith and Oppenheimer, 2005; Szymanski, 2005; Yalovsky et al., 2008). Many of the components and regulatory relationships among the complexes were discovered based on the stage-specific cell-swelling and -twisting phenotypes of the distorted class of Arabidopsis (Arabidopsis thaliana) trichome mutants (Szymanski et al., 1999; Zhang et al., 2005, 2008; Djakovic et al., 2006; Le et al., 2006; Uhrig et al., 2007). However, in both maize (Zea mays) and Arabidopsis, W/SRC and/or ARP2/3 are required for normal pavement cell morphogenesis (Frank and Smith, 2002; Mathur et al., 2003b; Brembu et al., 2004). Compared with other Arabidopsis pavement cell mutants, the shape defects of the distorted group are relatively mild. However, the distorted mutants and spike1 (spk1) differ from most other morphology mutants in that they display gaps in the shoot epidermis, most frequently at the interface of pavement cells and stomata (Qiu et al., 2002; Le et al., 2003; Li et al., 2003; Mathur et al., 2003b; Zhang et al., 2005; Djakovic et al., 2006). The cell gaps may reflect either uncoordinated growth between neighboring cells or defective cortical actin-dependent secretion of polysaccharides and/or proteins that promote cell-cell adhesion (Smith and Oppenheimer, 2005; Hussey et al., 2006; Leucci et al., 2007).In tip-growing cells, there is a strict requirement for actin to organize the trafficking and secretion activities of the cell to restrict growth to the apex. In Arabidopsis, the W/SRC-ARP2/3 pathway is not an essential tip growth component, because null alleles of both W/SRC and ARP2/3 subunits do not cause noticeable pollen tube or root hair phenotypes (Le et al., 2003; Djakovic et al., 2006). However, reverse genetic analysis of the W/SRC subunit BRK1 and ARP2/3 in the tip-growing protonemal cells of Physcomitrella patens revealed the obvious importance of this pathway (Harries et al., 2005; Perroud and Quatrano, 2008). Along similar lines, in two different legume species, W/SRC subunits are required for a normal root nodulation response to symbiotic bacteria (Yokota et al., 2009; Miyahara et al., 2010), indicating a conditional importance for this pathway in root hair growth. These genetic studies centered on the W/SRC and ARP2/3 pathways, in addition to those that involve a broader collection of actin-based morphology mutants (Smith and Oppenheimer, 2005; Blanchoin et al., 2010), are defining important cytoskeletal proteins and new interactions with the endomembrane system during morphogenesis. However, it is not completely clear how unstable actin filaments and actin bundle networks dictate the growth patterns of cells (Staiger et al., 2009).The difficulty of understanding the functions of specific actin arrays can be explained, in part, by the fact that plant cells that employ a diffuse growth mechanism have highly unstable cortical actin filaments and large actin bundles that do not have a geometry that obviously relates to the direction of growth or a specific subcellular activity (Blanchoin et al., 2010). This is in contrast to the cortical endocytic actin patches in yeast (Saccharomyces cerevisiae; Evangelista et al., 2002; Kaksonen et al., 2003) and cortical meshworks in the lamellipodia of crawling cells (Pollard and Borisy, 2003) that reveal subcellular locations where actin works to locally control membrane dynamics. In thick-walled plant cells, the magnitude of the forces that accompany turgor-driven cell expansion exceed those that could be generated by actin polymerization by orders of magnitude (Szymanski and Cosgrove, 2009). Localized cell wall loosening or the assembly of an anisotropic cell wall generates asymmetric yielding responses to turgor-induced stress (Baskin, 2005; Cosgrove, 2005). Therefore, the actin-based control of cell boundary dynamics is indirect, and the actin cytoskeleton influences cell shape change, in part, by actin and/or myosin-dependent trafficking of hormone transporters (Geldner et al., 2001) and organelles (Prokhnevsky et al., 2008), including those that control the localized delivery of protein complexes and polysaccharides that pattern the cell wall (Leucci et al., 2007; Gutierrez et al., 2009). In this scheme for actin-based growth control, the actin network dynamically rearranges at spatial scales that span from approximately 1- to 10-µm subcellular domains that may locally position organelles (Cleary, 1995; Gibbon et al., 1999; Szymanski et al., 1999) to the more than 100-µm actin bundle networks that operate at the spatial scales of entire cells (Gutierrez et al., 2009; Dyachok et al., 2011). It is clear from the work of several laboratories that the W/SRC and ARP2/3 protein complexes are required to organize cortical actin and actin bundle networks in trichomes (Szymanski et al., 1999; Le et al., 2003; Deeks et al., 2004; Zhang et al., 2005) and cylindrical epidermal cells (Mathur et al., 2003b; Dyachok et al., 2008, 2011). A key challenge now is to understand how plant cells deploy these approximately 10- to 20-nm heteromeric protein complexes to influence the patterns of growth at cellular scales.The genetic and biochemical control of ARP2/3 is complicated, but this is a tractable problem in plants, because the pathway is relatively simple compared with most other species in which it has been characterized. For example, in organisms ranging from yeast to humans, there are multiple types of ARP2/3 activators, protein complexes, and pathways that activate ARP2/3 (Welch and Mullins, 2002; Derivery and Gautreau, 2010). However, the maize and Arabidopsis genomes encode only WAVE/SCAR homologous proteins that can potently activate ARP2/3 (Frank et al., 2004; Basu et al., 2005). Detailed genetic and biochemical analyses of the WAVE/SCAR gene family in Arabidopsis demonstrated that the plant activators function interchangeably within the context of the W/SRC and define the lone pathway for ARP2/3 activation (Zhang et al., 2008). Bioinformatic analyses are consistent with a prominent role for W/SRC in the angiosperms, because in general, WASH complex subunits, which are structurally similar to WAVE/SCAR proteins, are largely absent from the higher plant genomes, while WAVE/SCAR genes are highly conserved (Kollmar et al., 2012).The components and regulatory schemes of the W/SRC-ARP2/3 pathway in Arabidopsis and P. patens are conserved compared with vertebrate species that employ these same protein complexes (Szymanski, 2005). For example, mutant complementation tests indicate that human W/SRC and ARP2/3 complex subunits can substitute for the Arabidopsis proteins (Mathur et al., 2003b). Furthermore, biochemical assays of Arabidopsis W/SRC (Basu et al., 2004; El-Assal et al., 2004; Frank et al., 2004; Le et al., 2006; Uhrig et al., 2007) and ARP2/3 assembly (Kotchoni et al., 2009) have shown that the binary interactions among W/SRC subunits and ARP2/3 complex assembly mechanisms are indistinguishable from those that have been observed for human W/SRC (Gautreau et al., 2004) and yeast ARP2/3 (Winter et al., 1999). After an initial period of controversy concerning the biochemical control of W/SRC, it is now apparent that vertebrate W/SRC (Derivery et al., 2009; Ismail et al., 2009), like the ARP2/3 complex (Machesky et al., 1999), is intrinsically inactive and requires positive regulation by Rac and other factors to fully activate ARP2/3 (Ismail et al., 2009; Lebensohn and Kirschner, 2009; Chen et al., 2010). Although overexpression of dominant negative ROP mutants causes trichome swelling and a reduced trichome branch number (Fu et al., 2002), the involvement of ROPs in trichome morphogenesis has been difficult to prove with a loss-of-function ROP allele because so many ROPs are expressed in this cell type (Marks et al., 2009). Existing reports on ROP loss-of-function mutants demonstrate the importance of pavement cell morphogenesis but do not document a trichome phenotype (Fu et al., 2005; Xu et al., 2010). A recent report describes a clever strategy to generate ROP loss-of-function lines that used the ectopic expression of ROP-specific bacterial toxins. There was a strong association between inducible expression of the toxins and the appearance of trichomes with severe trichome swelling and reduced branch number phenotypes (Singh et al., 2012). Although the exact mechanism of ROP-dependent control of W/SRC remains to be determined, the results described above in combination with the detection of direct interactions between the ROPGEF SPK1, active forms of ROP, and W/SRC subunits (Basu et al., 2004, 2008; Uhrig et al., 2007) strongly suggest that W/SRC is a ROP effector complex.The major challenge in the field now is to better understand the cellular control of W/SRC and how the complex is partitioned into active and inactive pools. In mammalian cells that crawl on a solid substrate, current models propose that a cytosolic pool of inactive WAVE/SCAR proteins and W/SRC is locally recruited and activated at specific plasma membrane surfaces in response to signals from some unknown Rac guanine nucleotide-exchange factor (GEF), protein kinase, and/or lipid kinase (Oikawa et al., 2004; Lebensohn and Kirschner, 2009; Chen et al., 2010). However, in Drosophila melanogaster neurons (Bogdan and Klämbt, 2003) and cultured human melanoma cells (Steffen et al., 2004), there are large pools of W/SRC with a perinuclear or organelle-like punctate localization that has no obvious relationship to cell shape or motility, raising uncertainty about the cellular mechanisms of W/SRC activation and the importance of different subcellular pools of the complex.In plants, cell fractionation experiments indicate that SCAR1 and ARP2/3 have an increased association with membranes compared with their animal counterparts (Dyachok et al., 2008; Kotchoni et al., 2009). In tip-growing moss protonemal cells, both the W/SRC subunit BRK1 and ARP2/3 localize to a population of unidentified organelles within the apical zone (Perroud and Quatrano, 2008). Similar live-cell imaging experiments in Arabidopsis reported a plasma membrane localization for SCAR1 and BRK1 in a variety of shoot epidermal and root cortex, and their accumulation at young trichome branch tips and at three-way cell wall junctions may define subcellular domains for W/SRC-ARP2/3-dependent actin filament nucleation at the plasma membrane (Dyachok et al., 2008). However, to our knowledge, active W/SRC, defined here as the fraction of W/SRC that colocalizes with ARP2/3 or actin, has not been reported in plants, and the plasma membrane is not necessarily the only organelle involved in W/SRC regulation. For example, the reported accumulation of BRK1 and SCAR1 at three-way cell wall junctions has a punctate appearance at the cell cortex that may not simply correspond to the plasma membrane (Dyachok et al., 2008). Also, in young stage 4 trichomes, there was an uncharacterized pool of intracellular SCAR1, but not BRK1, that localized to relatively large punctate structures (Dyachok et al., 2008). The endoplasmic reticulum (ER) may also be involved in W/SRC regulation. The ER-localized DOCK family ROPGEF SPK1 (Zhang et al., 2010) physically associates with multiple W/SRC proteins (Uhrig et al., 2007; Basu et al., 2008) and, based on genetic criteria, is an upstream, positive regulator of the W/SRC-ARP2/3 pathway (Basu et al., 2008). In the leaf, one function of SPK1 is to promote normal trafficking between the ER and Golgi; however, arp2/3 mutants do not share ER-stress phenotypes with spk1 (Zhang et al., 2010), making it unclear if SPK1 and the ER are directly involved in W/SRC signaling.This paper focuses on the localization and control of the W/SRC subunit NAP1/GNARLED/NAPP/HEM1/2. Arabidopsis NAP1 directly interacts with the ROP/Rac effector subunit SRA1/PIROGI/KLUNKER/PIRP (Basu et al., 2004; El-Assal et al., 2004; Uhrig et al., 2007). Based on the equally severe syndrome of nap1 and arp2/3 null phenotypes, and double mutant analyses, the only known function of NAP1 is to positively regulate ARP2/3 (Brembu et al., 2004; Deeks et al., 2004; El-Din El-Assal et al., 2004; Li et al., 2004). The vertebrate SRA1-NAP1 dimer is important for W/SRC assembly (Gautreau et al., 2004) and forms an extended physical surface that trans-inhibits the C-terminal ARP2/3-activating domain of WAVE/SCAR (Chen et al., 2010). The plant NAP1 and SRA1 proteins share end-to-end amino acid conservation with their vertebrate homologs and may form a heterodimer with similar functions (Basu et al., 2004; El-Assal et al., 2004; Uhrig et al., 2007). We report here that Arabidopsis NAP1 is strongly associated with ER membranes. In a detailed series of localization experiments, we detect a complicated intracellular distribution of NAP1 among the ER, the nucleus, and unidentified submicrometer punctae. A large pool of ER-associated NAP1 is inactive, based on the low level of colocalization with actin.Its accumulation on the ER does not require activating signals from either SPK1 or SRA1. These data indicate that the ER is a reservoir for W/SRC signaling and suggest that early steps in the positive regulation of NAP1 and the W/SRC occur on the ER surface.     

Composition,Assembly, and Trafficking of a Wheat Xylan Synthase Complex

Xylans play an important role in plant cell wall integrity and have many industrial applications. Characterization of xylan synthase (XS) complexes responsible for the synthesis of these polymers is currently lacking. We recently purified XS activity from etiolated wheat (Triticum aestivum) seedlings. To further characterize this purified activity, we analyzed its protein composition and assembly. Proteomic analysis identified six main proteins: two glycosyltransferases (GTs) TaGT43-4 and TaGT47-13; two putative mutases (TaGT75-3 and TaGT75-4) and two non-GTs; a germin-like protein (TaGLP); and a vernalization related protein (TaVER2). Coexpression of TaGT43-4, TaGT47-13, TaGT75-3, and TaGT75-4 in Pichia pastoris confirmed that these proteins form a complex. Confocal microscopy showed that all these proteins interact in the endoplasmic reticulum (ER) but the complexes accumulate in Golgi, and TaGT43-4 acts as a scaffold protein that holds the other proteins. Furthermore, ER export of the complexes is dependent of the interaction between TaGT43-4 and TaGT47-13. Immunogold electron microscopy data support the conclusion that complex assembly occurs at specific areas of the ER before export to the Golgi. A di-Arg motif and a long sequence motif within the transmembrane domains were found conserved at the NH₂-terminal ends of TaGT43-4 and homologous proteins from diverse taxa. These conserved motifs may control the forward trafficking of the complexes and their accumulation in the Golgi. Our findings indicate that xylan synthesis in grasses may involve a new regulatory mechanism linking complex assembly with forward trafficking and provide new insights that advance our understanding of xylan biosynthesis and regulation in plants.It is believed that Golgi-localized, multiprotein complexes synthesize plant hemicellulosic polysaccharides, including xylans. Such complexes are not well characterized in plants (Zeng et al., 2010; Atmodjo et al., 2011; Chou et al., 2012), which is in sharp contrast with mammalian and yeast cells (Jungmann and Munro, 1998; McCormick et al., 2000; Giraudo et al., 2001). Xylans are the most abundant plant hemicellulosic polysaccharides on Earth and play an important role in the integrity of cell walls, which is a key factor in plant growth. Any mutations affecting xylan backbone biosynthesis seem to result in abnormal growth of plants due mostly to thinning and weakening of secondary xylem walls, described as the irregular xylem (irx) phenotype. Thus, characterizing the xylan synthase complex (XSC) would have an impact on plant improvement, as well as many industrial applications related to food, feed, and biofuel production (Yang and Wyman, 2004; Faik, 2010). Although the Arabidopsis (Arabidopsis thaliana) irx mutants have revealed the involvement of several glycosyltransferase (GT) gene families in xylan biosynthesis (Brown et al., 2007, 2009; Lee et al., 2007, 2010; Wu et al., 2009, 2010), no XSCs have been purified/isolated from Arabidopsis tissues, and we still do not know whether some of the identified Arabidopsis GTs can assemble into functional XSCs. Furthermore, if GTs do assemble into XSCs, we don’t know the mechanisms by which plant cells control their assembly and cellular trafficking. In contrast to dicots, xylan synthase activity was recently immunopurified from etiolated wheat (Triticum aestivum) microsomes (Zeng et al., 2010). This purified wheat XS activity was shown to catalyze three activities, xylan-glucuronosyltransferase (XGlcAT), xylan-xylosyltransferase (XXylT), and xylan-arabinofuranosyltranferase (XAT), which work synergistically to synthesize xylan-type polymers in vitro (Zeng et al., 2008, 2010). This work focuses on describing protein composition, assembly, and trafficking of this purified wheat XS activity.In all eukaryotes, proteins of the secretory pathway (including GTs) are synthesized in the endoplasmic reticulum (ER) and modified as they go through the Golgi cisternae. Most proteins exit the ER from ER export sites (ERESs; Hanton et al., 2009) and use a signal-based sorting mechanism that allows them to be selectively recruited into vesicles coated by coat protein II complexes (Barlowe, 2003; Beck et al., 2008). For many Golgi-resident type II membrane proteins, di-Arg motifs, such as RR, RXR, and RRR located in their cytosolic NH₂-terminal ends, have been shown to be required for their ER export (Giraudo et al., 2003; Czlapinski and Bertozzi, 2006; Schoberer et al., 2009; Tu and Banfield, 2010). Interestingly, di-Arg motifs located ∼40 amino acids from the membrane on the cytosolic side can also be used to retrieve some type II ER-resident proteins from cis-Golgi (Schutze et al., 1994; Hardt et al., 2003; Boulaflous et al., 2009). In contrast to the signal-based sorting mechanism involved in trafficking between the ER and Golgi, the steady-state localization/retention of proteins (including GTs) in the Golgi is thought to occur through vesicular cycling. Cycling is influenced by various mechanisms, including the length and composition of the transmembrane domain (TMD) of type II GTs (Bretscher and Munro, 1993; Colley, 1997; van Vliet et al., 2003; Sousa et al., 2003; Sharpe et al., 2010), and the oligomerization/aggregation of GTs (kin hypothesis), which suggests that formation of homo- or heterooligomers of GTs in the Golgi may prevent their recruitment into clathrin-coated vesicles (Machamer, 1991; Nilsson et al., 1993; Weisz et al., 1993; Cole et al., 1996). Some Golgi-resident GTs are predicted to have a cleavable NH₂-terminal secretion signal peptide (SP) and would therefore exist as soluble proteins in the Golgi lumen. To maintain their proper Golgi localization, these processed GTs are likely part of multiprotein complexes anchored to integral membrane proteins. The fact that homologs of many of the trafficking proteins from mammalian and yeast cells are found in plants indicates that trafficking machineries of the plant secretory pathway are likely conserved (d’Enfert et al., 1992; Bar-Peled and Raikhel, 1997; Batoko et al., 2000; Pimpl et al., 2000; Phillipson et al., 2001; Hawes et al., 2008).It is becoming increasingly evident that understanding the mechanisms controlling protein-protein interaction, sorting, and trafficking of polysaccharide synthases (including XSCs) will help elucidate how plants regulate cell wall synthesis and deposition during their development. To this end, we believe that the purified wheat XS activity (Zeng et al., 2010) is an excellent model for this type of study. In this work, proteomics was used to determine the protein composition of the purified XS activity. Confocal microscopy and immunogold transmission electron microscopy (TEM) were used to investigate the assembly and trafficking of the complex. Our proteomics data showed that the purified activity contains two GTs, TaGT43-4 and TaGT47-13, two putative mutases, TaGT75-3 and TaGT75-4, and two non-GT proteins: a germin-like protein (TaGLP) belonging to cupin superfamily and a protein specific to monocots annotated as wheat vernalization-related protein 2 (TaVER2). Microscopy analyses revealed that all these proteins interact in the ER, but the assembled complexes accumulate in the Golgi. Export of these complexes from the ER is controlled by the interaction between TaGT43-4 and TaGT47-13. Characterization of the wheat XSC and its trafficking furthers our understanding of xylan biosynthesis in grasses and helps elucidate how polysaccharide synthase complexes are assembled, sorted, and maintained in different compartments of the secretory pathway.     

The Role of a Potassium Transporter OsHAK5 in Potassium Acquisition and Transport from Roots to Shoots in Rice at Low Potassium Supply Levels

In plants, K transporter (KT)/high affinity K transporter (HAK)/K uptake permease (KUP) is the largest potassium (K) transporter family; however, few of the members have had their physiological functions characterized in planta. Here, we studied OsHAK5 of the KT/HAK/KUP family in rice (Oryza sativa). We determined its cellular and tissue localization and analyzed its functions in rice using both OsHAK5 knockout mutants and overexpression lines in three genetic backgrounds. A β-glucuronidase reporter driven by the OsHAK5 native promoter indicated OsHAK5 expression in various tissue organs from root to seed, abundantly in root epidermis and stele, the vascular tissues, and mesophyll cells. Net K influx rate in roots and K transport from roots to aerial parts were severely impaired by OsHAK5 knockout but increased by OsHAK5 overexpression in 0.1 and 0.3 mm K external solution. The contribution of OsHAK5 to K mobilization within the rice plant was confirmed further by the change of K concentration in the xylem sap and K distribution in the transgenic lines when K was removed completely from the external solution. Overexpression of OsHAK5 increased the K-sodium concentration ratio in the shoots and salt stress tolerance (shoot growth), while knockout of OsHAK5 decreased the K-sodium concentration ratio in the shoots, resulting in sensitivity to salt stress. Taken together, these results demonstrate that OsHAK5 plays a major role in K acquisition by roots faced with low external K and in K upward transport from roots to shoots in K-deficient rice plants.Potassium (K) is one of the three most important macronutrients and the most abundant cation in plants. As a major osmoticum in the vacuole, K drives the generation of turgor pressure, enabling cell expansion. In the vascular tissue, K is an important participant in the generation of root pressure (for review, see Wegner, 2014 [including his new hypothesis]). In the phloem, K is critical for the transport of photoassimilates from source to sink (Marschner, 1996; Deeken et al., 2002; Gajdanowicz et al., 2011). In addition, enhancing K absorption and decreasing sodium (Na) accumulation is a major strategy of glycophytes in salt stress tolerance (Maathuis and Amtmann, 1999; Munns and Tester, 2008; Shabala and Cuin, 2008).Plants acquire K through K-permeable proteins at the root surface. Since available K concentration in the soil may vary by 100-fold, plants have developed multiple K uptake systems for adapting to this variability (Epstein et al., 1963; Grabov, 2007; Maathuis, 2009). In a classic K uptake experiment in barley (Hordeum vulgare), root K absorption has been described as a high-affinity and low-affinity biphasic transport process (Epstein et al., 1963). It is generally assumed that the low-affinity transport system (LATS) in the roots mediates K uptake in the millimolar range and that the activity of this system is insensitive to external K concentration (Maathuis and Sanders, 1997; Chérel et al., 2014). In contrast, the high-affinity transport system (HATS) was rapidly up-regulated when the supply of exogenous K was halted (Glass, 1976; Glass and Dunlop, 1978).The membrane transporters for K flux identified in plants are generally classified into three channels and three transporter families based on phylogenetic analysis (Mäser et al., 2001; Véry and Sentenac, 2003; Lebaudy et al., 2007; Alemán et al., 2011). For K uptake, it was predicted that, under most circumstances, K transporters function as HATS, while K-permeable channels mediate LATS (Maathuis and Sanders, 1997). However, a root-expressed K channel in Arabidopsis (Arabidopsis thaliana), Arabidopsis K Transporter1 (AKT1), mediates K absorption over a wide range of external K concentrations (Sentenac et al., 1992; Lagarde et al., 1996; Hirsch et al., 1998; Spalding et al., 1999), while evidence is accumulating that many K transporters, including members of the K transporter (KT)/high affinity K transporter (HAK)/K uptake permease (KUP) family, are low-affinity K transporters (Quintero and Blatt, 1997; Senn et al., 2001), implying that functions of plant K channels and transporters overlap at different K concentration ranges.Out of the three families of K transporters, cation proton antiporter (CPA), high affinity K/Na transporter (HKT), and KT/HAK/KUP, CPA was characterized as a K⁺(Na⁺)/H⁺ antiporter, HKT may cotransport Na and K or transport Na only (Rubio et al., 1995; Uozumi et al., 2000), while KT/HAK/KUP were predicted to be H⁺-coupled K⁺ symporters (Mäser et al., 2001; Lebaudy et al., 2007). KT/HAK/KUP were named by different researchers who first identified and cloned them (Quintero and Blatt, 1997; Santa-María et al., 1997). In plants, the KT/HAK/KUP family is the largest K transporter family, including 13 members in Arabidopsis and 27 members in the rice (Oryza sativa) genome (Rubio et al., 2000; Mäser et al., 2001; Bañuelos et al., 2002; Gupta et al., 2008). Sequence alignments show that genes of this family share relatively low homology to each other. The KT/HAK/KUP family was divided into four major clusters (Rubio et al., 2000; Gupta et al., 2008), and in cluster I and II, they were further separated into A and B groups. Genes of cluster I or II likely exist in all plants, cluster III is composed of genes from both Arabidopsis and rice, while cluster IV includes only four rice genes (Grabov, 2007; Gupta et al., 2008).The functions of KT/HAK/KUP were studied mostly in heterologous expression systems. Transporters of cluster I, such as AtHAK5, HvHAK1, OsHAK1, and OsHAK5, are localized in the plasma membrane (Kim et al., 1998; Bañuelos et al., 2002; Gierth et al., 2005) and exhibit high-affinity K uptake in the yeast Saccharomyces cerevisiae (Santa-María et al., 1997; Fu and Luan, 1998; Rubio et al., 2000) and in Escherichia coli (Horie et al., 2011). Transporters of cluster II, like AtKUP4 (TINY ROOT HAIRS1, TRH1), HvHAK2, OsHAK2, OsHAK7, and OsHAK10, could not complement the K uptake-deficient yeast (Saccharomyces cerevisiae) but were able to mediate K fluxes in a bacterial mutant; they might be tonoplast transporters (Senn et al., 2001; Bañuelos et al., 2002; Rodríguez-Navarro and Rubio, 2006). The function of transporters in clusters III and IV is even less known (Grabov, 2007).Existing data suggest that some KT/HAK/KUP transporters also may respond to salinity stress (Maathuis, 2009). The cluster I transporters of HvHAK1 mediate Na influx (Santa-María et al., 1997), while AtHAK5 expression is inhibited by Na (Rubio et al., 2000; Nieves-Cordones et al., 2010). Expression of OsHAK5 in tobacco (Nicotiana tabacum) BY2 cells enhanced the salt tolerance of these cells by accumulating more K without affecting their Na content (Horie et al., 2011).There are only scarce reports on the physiological function of KT/HAK/KUP in planta. In Arabidopsis, mutation of AtKUP2 (SHORT HYPOCOTYL3) resulted in a short hypocotyl, small leaves, and a short flowering stem (Elumalai et al., 2002), while a loss-of-function mutation of AtKUP4 (TRH1) resulted in short root hairs and a loss of gravity response in the root (Rigas et al., 2001; Desbrosses et al., 2003; Ahn et al., 2004). AtHAK5 is the only system currently known to mediate K uptake at concentrations below 0.01 mm (Rubio et al., 2010) and provides a cesium uptake pathway (Qi et al., 2008). AtHAK5 and AtAKT1 are the two major physiologically relevant molecular entities mediating K uptake into roots in the range between 0.01 and 0.05 mm (Pyo et al., 2010; Rubio et al., 2010). AtAKT1 may contribute to K uptake within the K concentrations that belong to the high-affinity system described by Epstein et al. (1963).Among all 27 members of the KT/HAK/KUP family in rice, OsHAK1, OsHAK5, OsHAK19, and OsHAK20 were grouped in cluster IB (Gupta et al., 2008). These four rice HAK members share 50.9% to 53.4% amino acid identity with AtHAK5. OsHAK1 was expressed in the whole plant, with maximum expression in roots, and was up-regulated by K deficiency; it mediated high-affinity K uptake in yeast (Bañuelos et al., 2002). In this study, we examined the tissue-specific localization and the physiological functions of OsHAK5 in response to variation in K supply and to salt stress in rice. By comparing K uptake and translocation in OsHAK5 knockout (KO) mutants and in OsHAK5-overexpressing lines with those in their respective wild-type lines supplied with different K concentrations, we found that OsHAK5 not only mediates high-affinity K acquisition but also participates in root-to-shoot K transport as well as in K-regulated salt tolerance.