Retromer Contributes to Immunity-Associated Cell Death in Arabidopsis

Membrane trafficking is required during plant immune responses, but its contribution to the hypersensitive response (HR), a form of programmed cell death (PCD) associated with effector-triggered immunity, is not well understood. HR is induced by nucleotide binding-leucine-rich repeat (NB-LRR) immune receptors and can involve vacuole-mediated processes, including autophagy. We previously isolated lazarus (laz) suppressors of autoimmunity-triggered PCD in the Arabidopsis thaliana mutant accelerated cell death11 (acd11) and demonstrated that the cell death phenotype is due to ectopic activation of the LAZ5 NB-LRR. We report here that laz4 is mutated in one of three VACUOLAR PROTEIN SORTING35 (VPS35) genes. We verify that LAZ4/VPS35B is part of the retromer complex, which functions in endosomal protein sorting and vacuolar trafficking. We show that VPS35B acts in an endosomal trafficking pathway and plays a role in LAZ5-dependent acd11 cell death. Furthermore, we find that VPS35 homologs contribute to certain forms of NB-LRR protein-mediated autoimmunity as well as pathogen-triggered HR. Finally, we demonstrate that retromer deficiency causes defects in late endocytic/lytic compartments and impairs autophagy-associated vacuolar processes. Our findings indicate important roles of retromer-mediated trafficking during the HR; these may include endosomal sorting of immune components and targeting of vacuolar cargo.     

The Rab GTPase RabG3b Positively Regulates Autophagy and Immunity-Associated Hypersensitive Cell Death in Arabidopsis

A central component of the plant defense response to pathogens is the hypersensitive response (HR), a form of programmed cell death (PCD). Rapid and localized induction of HR PCD ensures that pathogen invasion is prevented. Autophagy has been implicated in the regulation of HR cell death, but the functional relationship between autophagy and HR PCD and the regulation of these processes during the plant immune response remain controversial. Here, we show that a small GTP-binding protein, RabG3b, plays a positive role in autophagy and promotes HR cell death in response to avirulent bacterial pathogens in Arabidopsis (Arabidopsis thaliana). Transgenic plants overexpressing a constitutively active RabG3b (RabG3bCA) displayed accelerated, unrestricted HR PCD within 1 d of infection, in contrast to the autophagy-defective atg5-1 mutant, which gradually developed chlorotic cell death through uninfected sites over several days. Microscopic analyses showed the accumulation of autophagic structures during HR cell death in RabG3bCA cells. Our results suggest that RabG3b contributes to HR cell death via the activation of autophagy, which plays a positive role in plant immunity-triggered HR PCD.In response to the constant attack by microbial pathogens, plants have developed defense mechanisms to protect themselves against harmful diseases caused by various pathogens. Plants primarily rely on two layers of innate immunity to cope with microbial pathogens (Jones and Dangl, 2006). The first layer of plant immunity, which is triggered by pathogen-associated molecular patterns (PAMPs) such as bacterial flagellin, lipopolysaccharides, and fungal chitin, is designated PAMP-triggered immunity (PTI; Boller and He, 2009). Because pathogens have evolved to overcome PTI, plants have developed a second layer of immunity, referred to as effector-triggered immunity (ETI; Dodds and Rathjen, 2010). ETI depends on specific interactions between plant Resistance proteins and pathogen effectors and is often associated with a form of programmed cell death (PCD) termed the hypersensitive response (HR), which inhibits pathogen growth (Coll et al., 2011).Plants use PCD to regulate developmental and defense responses. In addition to pathogen attack, many abiotic stress factors such as heat and ozone exposure elicit PCD in plants (Hayward and Dinesh-Kumar, 2011). PCD also occurs during various developmental processes, including endosperm development, tracheary element (TE) differentiation, female gametophyte differentiation, leaf abscission, and senescence (Kuriyama and Fukuda, 2002; Gunawardena, 2008). Recently, plant PCD has been classified into two types, “autolytic” PCD and “nonautolytic” PCD, on the basis of the presence or absence of rapid cytoplasm clearance after tonoplast rupture, respectively (van Doorn et al., 2011). Autolytic PCD, which mainly occurs during plant development, falls under “autophagic” PCD in animals because it is associated with the accumulation of autophagy-related structures in the cytoplasm. Some forms of HR PCD classified as nonautolytic PCD in plants are accompanied by increased vacuolization, indicating the progress of autophagy, and therefore can be placed under autophagic PCD (Hara-Nishimura et al., 2005; Hatsugai et al., 2009).Autophagy is an intracellular process in which double membrane-bound autophagosomes enclose cytoplasmic components and damaged or toxic materials and target them to the vacuole or lysosome for degradation (Chung, 2011). In plants, autophagy plays important roles in the responses to nutrient starvation, senescence, and abiotic and biotic stresses (Liu et al., 2005; Xiong et al., 2005, 2007; Bassham, 2007; Hofius et al., 2009). Accumulating evidence indicates that autophagy regulates immune responses in both animals and plants. Autophagy is essential for the direct elimination of pathogens in mammalian systems (Levine et al., 2011). Invading bacteria and viruses are targeted to autophagosomes and then delivered to the lysosome for degradation in a process called xenophagy (Levine, 2005). In addition to its function in directly killing pathogens, xenophagic degradation can provide microbial antigens for major histocompatibility complex class II presentation to the innate and adaptive immune systems (Levine, 2005; Schmid and Münz, 2007). Furthermore, the human surface receptor CD46 was shown to directly induce autophagy through physical interaction with the autophagic machinery (Joubert et al., 2009). The role of autophagy in plant basal immunity to virulent pathogens has been determined (Patel and Dinesh-Kumar, 2008; Hofius et al., 2009; Lai et al., 2011; Lenz et al., 2011). Arabidopsis (Arabidopsis thaliana) plants defective in AUTOPHAGY-RELATED (ATG) genes exhibited enhanced susceptibility to the necrotrophic fungal pathogens Botrytis cinerea and Alternaria brassicicola, suggesting that the massive breakdown of cytoplasmic materials provides nutrients for the growth of necrotrophic pathogens or that fungal toxin-induced necrotic cell death is enhanced in atg mutants (Lai et al., 2011; Lenz et al., 2011). However, studies on the responses to the biotrophic pathogen Pseudomonas syringae pv tomato DC3000 (Pst DC3000) have yielded contradictory results. Whereas earlier studies reported that bacterial numbers significantly increased in ATG6-antisense (AS) and atg mutant plants (Patel and Dinesh-Kumar, 2008; Hofius et al., 2009), a recent study indicated that atg mutants exhibit increased resistance to Pst DC3000 (Lenz et al., 2011). Although these discrepancies remain to be resolved, salicylic acid (SA) levels and SA-dependent gene expression were both elevated in atg mutants, suggesting that autophagy may negatively regulate SA-associated plant immunity (Yoshimoto et al., 2009; Lenz et al., 2011). These findings indicate that the role of autophagy in plant immunity depends on the lifestyle of the invading pathogens (Lenz et al., 2011).Autophagy plays an important role in the regulation of HR PCD in plant innate immunity (Hayward and Dinesh-Kumar, 2011). Tobacco (Nicotiana tabacum) plants silenced for ATG6/Beclin1 and other ATG genes such as phosphatidylinositol 3-kinase (PI3K)/vacuolar protein sorting34 (VPS34), ATG3, and ATG7 underwent unrestricted HR PCD upon pathogen infection (Liu et al., 2005). ATG6-AS and atg5 mutant Arabidopsis plants also displayed unlimited HR PCD upon infection with the avirulent bacterium Pst DC3000 (AvrRpm1; Patel and Dinesh-Kumar, 2008; Yoshimoto et al., 2009). These studies suggest that autophagy is a “prosurvival” or “antideath” mechanism that negatively regulates HR PCD (Liu and Bassham, 2012). By contrast, a “prodeath” role has been suggested for autophagy in HR PCD regulation (Hofius et al., 2009). Pst DC3000 (AvrRps4)-induced and, to a lesser extent, Pst DC3000 (AvrRpm1)-induced HR PCD was suppressed in atg mutants, suggesting that autophagy plays a positive role and that autophagic cell death is involved in RPS4- and RPM1-mediated HR cell death.We previously showed that the small GTP-binding protein RabG3b, isolated from secretome analysis in Arabidopsis (Oh et al., 2005), functions as a component of autophagy and positively regulates TE differentiation via the activation of autophagic cell death (Kwon et al., 2010a, 2010b). Overexpression of a constitutively active RabG3b (RabG3bCA) in plants significantly increased autophagy during PCD associated with TE differentiation, thereby enhancing TE formation and xylem development. Transgenic poplar (Populus alba × Populus tremula var glandulosa) overexpressing Arabidopsis RabG3bCA was further generated, and these exhibited significant stimulation of xylem development together with autophagic activation, suggesting that RabG3b is a positive regulator of autophagy and xylem development in Populus spp. as well as Arabidopsis (Kwon et al., 2011). We also reported that RabG3b is involved in cell death associated with the fungal pathogen A. brassicicola and infection with the fungal toxin fumonisin B1 (FB1) as well as leaf senescence (Kwon et al., 2009). Here, we extend our work to determine the role of RabG3b and autophagy in immunity-associated HR PCD. We found that RabG3bCA transgenic plants accumulated a large number of autophagic structures and displayed accelerated, expanded cell death against a number of PCD inducers, such as FB1 and the bacterial pathogens Pst DC3000 (AvrRpm1) and Pst DC3000 (AvrRpt2). Our results suggest that RabG3b plays a positive role in immunity-associated HR PCD via the activation of autophagic cell death.     

Role of Aminoalcoholphosphotransferases 1 and 2 in Phospholipid Homeostasis in Arabidopsis

Aminoalcoholphosphotransferase (AAPT) catalyzes the synthesis of phosphatidylcholine (PC) and phosphotidylethanolamine (PE), which are the most prevalent membrane phospholipids in all eukaryotic cells. Here, we show that suppression of AAPTs results in extensive membrane phospholipid remodeling in Arabidopsis thaliana. Double knockout (KO) mutants that are hemizygous for either aapt1 or aapt2 display impaired pollen and seed development, leading to embryotic lethality of the double KO plants, whereas aapt1 or aapt2 single KO plants show no overt phenotypic alterations. The growth rate and seed yield of AAPT RNA interference (RNAi) plants are greatly reduced. Lipid profiling shows decreased total galactolipid and phospholipid content in aapt1-containing mutants, including aapt1, aapt1/aapt1 aapt2/AAPT2, aapt1/AAPT1 aapt2/aapt2, and AAPT RNAi plants. The level of PC in leaves was unchanged, whereas that of PE was reduced in all AAPT-deficient plants, except aapt2 KO. However, the acyl species of PC was altered, with increased levels of C34 species and decreased C36 species. Conversely, the levels of PE and phosphatidylinositol were decreased in C34 species. In seeds, all AAPT-deficient plants, including aapt2 KO, displayed a decrease in PE. The data show that AAPT1 and AAPT2 are essential to plant vegetative growth and reproduction and have overlapping functions but that AAPT1 contributes more than AAPT2 to PC production in vegetative tissues. The opposite changes in molecular species between PC and PE and unchanged PC level indicate the existence of additional pathways that maintain homeostatic levels of PC, which are crucial for the survival and proper development of plants.     

Novel Plant Immune-Priming Compounds Identified via High-Throughput Chemical Screening Target Salicylic Acid Glucosyltransferases in Arabidopsis

Plant activators are compounds, such as analogs of the defense hormone salicylic acid (SA), that protect plants from pathogens by activating the plant immune system. Although some plant activators have been widely used in agriculture, the molecular mechanisms of immune induction are largely unknown. Using a newly established high-throughput screening procedure that screens for compounds that specifically potentiate pathogen-activated cell death in Arabidopsis thaliana cultured suspension cells, we identified five compounds that prime the immune response. These compounds enhanced disease resistance against pathogenic Pseudomonas bacteria in Arabidopsis plants. Pretreatments increased the accumulation of endogenous SA, but reduced its metabolite, SA-O-β-d-glucoside. Inducing compounds inhibited two SA glucosyltransferases (SAGTs) in vitro. Double knockout plants that lack both SAGTs consistently exhibited enhanced disease resistance. Our results demonstrate that manipulation of the active free SA pool via SA-inactivating enzymes can be a useful strategy for fortifying plant disease resistance and may identify useful crop protectants.     

Identification and Characterization of an Epi-Allele of FIE1 Reveals a Regulatory Linkage between Two Epigenetic Marks in Rice

DNA methylation and histone H3 Lys 9 dimethylation (H3K9me2) are important epigenetic repression marks for silencing transposons in heterochromatin and for regulating gene expression. However, the mechanistic relationship to other repressive marks, such as histone H3 Lys 27 trimethylation (H3K27me3) is unclear. FERTILIZATION-INDEPENDENT ENDOSPERM1 (FIE1) encodes an Esc-like core component of the Polycomb repressive complex 2, which is involved in H3K27me3-mediated gene repression. Here, we identify a gain-of-function epi-allele (Epi-df) of rice (Oryza sativa) FIE1; this allele causes a dwarf stature and various floral defects that are inherited in a dominant fashion. We found that Epi-df has no changes in nucleotide sequence but is hypomethylated in the 5′ region of FIE1 and has reduced H3K9me2 and increased H3K4me3. In Epi-df, FIE1 was ectopically expressed and its imprinting was disrupted. FIE1 interacted with rice Enhancer of Zeste homologs, consistent with its role in H3K27me3 repression. Ectopic expression of FIE1 in Epi-df resulted in alteration of H3K27me3 levels in hundreds of genes. In summary, this work identifies an epi-allele involved in H3K27me3-mediated gene repression that itself is highly regulated by DNA methylation and histone H3K9me2, thereby shedding light on the link between DNA methylation and histone methylation, the two important epigenetic marks regulating rice development.     

Involvement of the Electrophilic Isothiocyanate Sulforaphane in Arabidopsis Local Defense Responses

Plants defend themselves against microbial pathogens through a range of highly sophisticated and integrated molecular systems. Recognition of pathogen-secreted effector proteins often triggers the hypersensitive response (HR), a complex multicellular defense reaction where programmed cell death of cells surrounding the primary site of infection is a prominent feature. Even though the HR was described almost a century ago, cell-to-cell factors acting at the local level generating the full defense reaction have remained obscure. In this study, we sought to identify diffusible molecules produced during the HR that could induce cell death in naive tissue. We found that 4-methylsulfinylbutyl isothiocyanate (sulforaphane) is released by Arabidopsis (Arabidopsis thaliana) leaf tissue undergoing the HR and that this compound induces cell death as well as primes defense in naive tissue. Two different mutants impaired in the pathogen-induced accumulation of sulforaphane displayed attenuated programmed cell death upon bacterial and oomycete effector recognition as well as decreased resistance to several isolates of the plant pathogen Hyaloperonospora arabidopsidis. Treatment with sulforaphane provided protection against a virulent H. arabidopsidis isolate. Glucosinolate breakdown products are recognized as antifeeding compounds toward insects and recently also as intracellular signaling and bacteriostatic molecules in Arabidopsis. The data presented here indicate that these compounds also trigger local defense responses in Arabidopsis tissue.Plants are constantly challenged by pathogenic microorganisms and have developed several detection and defense systems to protect themselves against the invaders. Preformed defenses include the waxy cuticle, thick cell walls, and antimicrobial compounds. After recognition of microbe-associated patterns, defense responses are induced, which include the fortification of cell walls and the production of phytoalexins (Monaghan and Zipfel, 2012). Overcoming the preformed and induced defenses of the plant hosts requires adaptation by the pathogen. Pathogenic bacteria use type III secretion to inject proteins (so-called effectors) into the host cytosol in order to overcome plant defense responses (Bent and Mackey, 2007). In turn, plants have developed systems to recognize the pathogenic effectors and mount defense. Recognition of type III effectors by plant resistance (R) proteins induces robust defense responses that frequently include the hypersensitive response (HR).The HR is a complex defense reaction characterized by the induction of programmed cell death (PCD) in the local host tissue as well as the activation of other defense responses in both local and systemic tissue (Mur et al., 2008; Shah, 2009). Oomycetes and true fungi also secrete proteinaceous effectors that can be recognized by host R proteins (Coates and Beynon, 2010; Hückelhoven and Panstruga, 2011; Feng and Zhou, 2012). The lesions formed during the HR vary in size between different host-pathogen pairs; however, a lesion induced at one or a few cells can spread to surrounding cells (Mur et al., 2008). Since pathogens inducing HR typically fail to proliferate, the first infected cell likely releases a compound that promotes PCD in surrounding cells. This is especially clear in models with oomycete and fungal pathogens, where the localization of the pathogen and the spread of cell death around the infection site can be clearly visualized (Mur et al., 2008; Coates and Beynon, 2010). Trailing necrosis is an incomplete resistance phenotype characterized by cell death that trails, but fails to contain, the filamentous growth of the pathogen. One explanation for trailing necrosis is a failure of infected cells to produce a putative mobile defense signal required to enhance defense in neighboring cells. Farther from the site of PCD, other defense pathways are activated and systemic tissue is primed for defense.The hunt for systemically acting compounds has been intense, and several candidates for this signal have been presented (Dempsey and Klessig, 2012). In contrast, even though the phenomenon of HR as a defense reaction was described almost a century ago (Stakman, 1915; Mur et al., 2008), compounds acting on the local tissue scale of the HR have attracted little attention. We set out to find substances released from cells undergoing the HR that could induce cell death in naive tissue. We report that leaf tissue of the model plant Arabidopsis (Arabidopsis thaliana) releases the reactive electrophilic compound sulforaphane after bacterial effector recognition. Mutants affected in sulforaphane production as well as other glucosinolate breakdown products showed delayed or reduced cell death after the recognition of pathogenic effectors and decreased resistance to an oomycete pathogen. Moreover, pretreatment of plants with sulforaphane enhanced resistance against a virulent oomycete isolate. Thus, we interpret this as that sulforaphane and likely similar compounds might both possess direct antimicrobial properties and, through a cytotoxic mechanism, act directly on plant cells to trigger defense responses.     

The SUD1 Gene Encodes a Putative E3 Ubiquitin Ligase and Is a Positive Regulator of 3-Hydroxy-3-Methylglutaryl Coenzyme A Reductase Activity in Arabidopsis

The 3-hydroxy-3-methylglutaryl-CoA reductase (HMGR) enzyme catalyzes the major rate-limiting step of the mevalonic acid (MVA) pathway from which sterols and other isoprenoids are synthesized. In contrast with our extensive knowledge of the regulation of HMGR in yeast and animals, little is known about this process in plants. To identify regulatory components of the MVA pathway in plants, we performed a genetic screen for second-site suppressor mutations of the Arabidopsis thaliana highly drought-sensitive drought hypersensitive2 (dry2) mutant that shows decreased squalene epoxidase activity. We show that mutations in SUPPRESSOR OF DRY2 DEFECTS1 (SUD1) gene recover most developmental defects in dry2 through changes in HMGR activity. SUD1 encodes a putative E3 ubiquitin ligase that shows sequence and structural similarity to yeast Degradation of α factor (Doα10) and human TEB4, components of the endoplasmic reticulum–associated degradation C (ERAD-C) pathway. While in yeast and animals, the alternative ERAD-L/ERAD-M pathway regulates HMGR activity by controlling protein stability, SUD1 regulates HMGR activity without apparent changes in protein content. These results highlight similarities, as well as important mechanistic differences, among the components involved in HMGR regulation in plants, yeast, and animals.     

Regulation of Histone Methylation and Reprogramming of Gene Expression in the Rice Inflorescence Meristem

Rice inflorescence meristem (IM) activity is essential for panicle development and grain production. How chromatin and epigenetic mechanisms regulate IM activity remains unclear. Genome-wide analysis revealed that in addition to genes involved in the vegetative to reproductive transition, many metabolic and protein synthetic genes were activated in IM compared with shoot apical meristem and that a change in the H3K27me3/H3K4me3 ratio was an important factor for the differential expression of many genes. Thousands of genes gained or lost H3K27me3 in IM, and downregulation of the H3K27 methyltransferase gene SET DOMAIN GROUP 711 (SDG711) or mutation of the H3K4 demethylase gene JMJ703 eliminated the increase of H3K27me3 in many genes. SDG711-mediated H3K27me3 repressed several important genes involved in IM activity and many genes that are silent in the IM but activated during floral organogenesis or other developmental stages. SDG711 overexpression augmented IM activity and increased panicle size; suppression of SDG711 by RNA interference had the opposite effect. Double knockdown/knockout of SDG711 and JMJ703 further reduced panicle size. These results suggest that SDG711 and JMJ703 have agonistic functions in reprogramming the H3K27me3/H3K4me3 ratio and modulating gene expression in the IM.     

The RECG1 DNA Translocase Is a Key Factor in Recombination Surveillance,Repair, and Segregation of the Mitochondrial DNA in Arabidopsis

The mitochondria of flowering plants have considerably larger and more complex genomes than the mitochondria of animals or fungi, mostly due to recombination activities that modulate their genomic structures. These activities most probably participate in the repair of mitochondrial DNA (mtDNA) lesions by recombination-dependent processes. Rare ectopic recombination across short repeats generates new genomic configurations that contribute to mtDNA heteroplasmy, which drives rapid evolution of the sequence organization of plant mtDNAs. We found that Arabidopsis thaliana RECG1, an ortholog of the bacterial RecG translocase, is an organellar protein with multiple roles in mtDNA maintenance. RECG1 targets to mitochondria and plastids and can complement a bacterial recG mutant that shows defects in repair and replication control. Characterization of Arabidopsis recG1 mutants showed that RECG1 is required for recombination-dependent repair and for suppression of ectopic recombination in mitochondria, most likely because of its role in recovery of stalled replication forks. The analysis of alternative mitotypes present in a recG1 line and of their segregation following backcross allowed us to build a model to explain how a new stable mtDNA configuration, compatible with normal plant development, can be generated by stoichiometric shift.