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J. Biol. Chem., Vol. 283, Issue 2, 774-783, January 11, 2008

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Metacaspase-8 Modulates Programmed Cell Death Induced by Ultraviolet Light and H₂O₂ in Arabidopsis^*

Rui He¹, Georgina E. Drury², Vitalie I. Rotari, Anna Gordon, Martin Willer, Tabasum Farzaneh, Ernst J. Woltering, and Patrick Gallois³

From the Faculty of Life Sciences, University of Manchester, 3.614 Stopford Building, Oxford Road, Manchester M13 9PT, United Kingdom and the Agrotechnology and Food Sciences Group, Wageningen University and Research Centre, 6700 AA Wageningen, The Netherlands

Received for publication, May 21, 2007 , and in revised form, November 12, 2007.

	ABSTRACT

TOP ABSTRACT INTRODUCTION EXPERIMENTAL PROCEDURES RESULTS DISCUSSION REFERENCES

 
Programmed cell death (PCD) is a genetically controlled cell death that is regulated during development and activated in response to environmental stresses or pathogen infection. The degree of conservation of PCD across kingdoms and phylum is not yet clear; however, whereas caspases are proteases that act as key components of animal apoptosis, plants have no orthologous caspase sequences in their genomes. The discovery of plant and fungi metacaspases as proteases most closely related to animal caspases led to the hypothesis that metacaspases are the functional homologues of animal caspases in these organisms. Arabidopsis thaliana has nine metacaspase genes, and so far it is unknown which members of the family if any are involved in the regulation of PCD. We show here that metacaspase-8 (AtMC8) is a member of the gene family strongly up-regulated by oxidative stresses caused by UVC, H₂O₂, or methyl viologen. This up-regulation was dependent of RCD1, a mediator of the oxidative stress response. Recombinant metacaspase-8 cleaved after arginine, had a pH optimum of 8, and complemented the H₂O₂ no-death phenotype of a yeast metacaspase knock-out. Overexpressing AtMC8 up-regulated PCD induced by UVC or H₂O₂, and knocking out AtMC8 reduced cell death triggered by UVC and H₂O₂ in protoplasts. Knock-out seeds and seedlings had an increased tolerance to the herbicide methyl viologen. We suggest that metacaspase-8 is part of an evolutionary conserved PCD pathway activated by oxidative stress.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION EXPERIMENTAL PROCEDURES RESULTS DISCUSSION REFERENCES

 
In some instances, programmed cell death (PCD)⁴ in plants is comparable with animal apoptosis at the cellular level. However, sequencing the Arabidopsis genome revealed that very few of the animal PCD regulators are conserved in plants. This suggests a greater divergence of the PCD pathways across kingdoms than thought. Initial reports seemed to provide indirect evidence supporting the existence of caspase orthologues in plants, with several caspase-like activities detected in plant extracts and inhibitor studies that show them to be required for PCD (for review, see Ref. 1). Although several research groups reported the absence of orthologous caspase sequences in plant genomes, a more in depth analysis revealed a greater diversity of caspase-related proteases than previously suspected (2). In particular, two families of predicted proteases were identified that are more closely related to animal caspases than to other proteases: the paracaspases and metacaspases. Paracaspases and caspases appear animal specific, whereas metacaspases are present in other eukaryotes, including plants. Plant metacaspases are subdivided in type I and type II on the basis of their structure; type I have an N-terminal prodomain that is not present in type II. A role for metacaspases in plant PCD was proposed (3) for four reasons; 1) a common origin with caspases, 2) the absence of closer caspase homologues in plants, 3) the proliferation of the genes coding for metacaspases in plant genomes mirrors the pattern of the proliferation and specialization of caspases in animal genomes, and 4) the fusion of type I plant metacaspases with a zinc-finger domain also present in LSD1, a regulator of the hypersensitive response in plants (4). Early observations suggested that metacaspases could be responsible for caspase-like activities detected in plants (5, 6); however, three reports have now demonstrated that metacaspases are unable to cleave caspase substrates. So far, all four recombinant Arabidopsis metacaspases tested have arginine as the preferred P1 amino acid in the cleavage site instead of caspase aspartic acid (7). A recombinant metacaspase from pine showed the same preferred cleavage site with Arg in P1 (8). These activities are not inhibited by caspase inhibitors.

Although metacaspases do not have caspase-like activities, there is strong support for a role in PCD. The yeast metacaspase (YCA1) knock-out survives in the presence of H₂O₂ (5), and the down-regulation of a metacaspase suppresses PCD in the suspensor cells of Picea abies embryogenic culture (9). Another report using Arabidopsis detected small but statistically significant changes in metacaspase KOs; KOs of Arabidopsis type II metacaspases had a reduced cell death, whereas KOs of type I metacaspases had an increased cell death when challenged by botrytis (10). A study of botrytis infection in tomato further supported the idea that type II metacaspases may mediate cell death in response to necrotic pathogens, as pathogen exposure led to type II metacaspase up-regulation (11). In contrast, there is no support for a metacaspase role in PCD using a range of stresses in Trypanosoma brucei (12) where metacaspases may function in cell proliferation and mitochondria biogenesis (13). A study using metacaspase KO strains in Aspergillus fumigatus found metacaspases required for phosphatidylserine exposure, a cellular marker of PCD but not for other markers such as activation of caspase-like activities and loss of viability (14). Finally, it has been reported that Arabidopsis plants overproducing selected members of the metacaspase gene family had no obvious cell death-related phenotype (15). Taken together, evidence is conflicting but certainly suggestive that some metacaspases may play a role in PCD, and some may not.

Previously alluded to, the proliferation of metacaspase genes in plants may reflect some form of specialization. Arabidopsis thaliana has nine metacaspase genes, and it can be expected that some members of the family are involved in the regulation of PCD, and some may be involved in other processes. As an illustration of that, two type-I metacaspases (At5g64240 and At1g02170) are up-regulated in Arabidopsis plants 24 h post-infiltration with bacterial pathogens, whereas type II metacaspases are not significantly affected (7). In addition, metacaspases can have different pH optima, suggesting various subcellular localizations (16), and display different substrate affinities (7). It is, therefore, important to analyze the function of each member of this gene family in Arabidopsis. In addition, different PCD pathways activated in plants may be either metacaspase-dependent or metacaspase-independent. This hypothesis is exemplified in yeast, where the single yeast metacaspase (YCA1) mediates PCD induced by H₂O₂ or acetic acid (5), by viruses (17), and by hyperosmotic stress (18), but in contrast, it is not required for PCD during mating (19), triggered by ammonia (20), or induced by Bax expression (21). We show here that Arabidopsis metacaspase-8, a type II metacaspase, is up-regulated by the oxidative stress caused by UVC and leading to PCD, and this up-regulation is RCD1-dependent. We have genetic evidence that metacaspase 8 is part of a PCD pathway induced by UVC, H₂O₂, or methyl viologen. This report contributes to our understanding of the organization of the metacaspase family in Arabidopsis and the origin of eukaryotic PCD.

	EXPERIMENTAL PROCEDURES

TOP ABSTRACT INTRODUCTION EXPERIMENTAL PROCEDURES RESULTS DISCUSSION REFERENCES

 
Plant Growth Conditions—Three A. thaliana ecotypes, Columbia (Col-0), Wassilewskija (WS), and Landsberg erecta (Ler) were used. Transgenic overexpressing metacaspase-8 were constructed in a Col-0 background. The AtMC8-1 (FLAG322_G10) line in a WS background was supplied by FLAGDB (FLAGDB, Institut National de la Recherche Agronomique, France), and AtMC8-2 (JII Gene Trap line GT_3_12679) in a Ler background was purchased from NASC. Salk_047489 Salk_047493 and Salk_063109 were purchased from NASC. The rcd1-1 mutant was provided by Dr. R. Ahlfors (University of Helsinki). Plants were grown at 22–23 °C in long day (16/8 h) or short day (8/16 h) photoperiod in Perceval growth cabinets. In vitro seedlings were grown in a Sanyo cabinet under continuous light at 22 °C.

Plasmids—An AtMC8 ORF was obtained using RT-PCR and RNA from UV-treated seedlings using primers with Lic adaptors GAC GAC GAC AAG ATG GCG AAG AAA GCA CTT TTG and GAG GAG AAG CCC GGT CCG TAG CAT ATA AAT GGT TTA TCA AC. The full ORF was cloned into the pET-30 Ek/LIC vector (Novagen), which added a His tag at both termini and an S ·tag at the N terminus to give pLIC-AtMC8. A point-mutated form, pLIC -AtMC8^C140A, was generated using the QuikChange mutagenesis protocol (Stratagene). The AtMC8 ORF was excised from pLIC-AtMC8 with the His and S tags using XbaI and SalI and ligated into pDH51 (22) using XboI and SalI to add a cauliflower mosaic virus 35 S promoter and terminator. The resulting plasmid was then restricted with PVU II to excise the AtMC8 coding sequence flanked with the cauliflower mosaic virus 35 S promoter and terminator. This fragment was ligated into the T-DNA vector pZP111b (23) linearized using SmaI and dephosphorylated to give pZP111-AtMC8. pZP111-AtMC8^C140A was generated the same way using pLIC-AtMC8^C140A as a starting point. The wild type and the point-mutated AtMC8 ORF were cloned into the yeast vector pYES2 (Invitrogen) using XbaI and SacI to give pYES-AtMC8 and pYES-AtMC8^C140A.

Expression in Escherichia coli—pLIC-AtMC8 and pLIC-AtMC8^C140A were transformed into BL21(DE3) competent cells (Invitrogen). Kanamycin-resistant colonies were grown to an absorbance of 0.5 and induced with 1 mM isopropyl 1-thio-β-D-galactopyranoside, 2%ethanol for 48 h at 22 °C. Proteins were extracted in ice-cold 500 mM NaCl, 50 mM K₂PO₄ pH7.4, 3mM dithiothreitol, 10%(w/v) glycerol, 1%(w/v) CHAPS, 5 µl·ml^–1 aprotinin with a ratio of 200 µl/5 absorbance units. Cells were broken using a sonicator (Vibra Cell^TM, JECONS Sonics & Materials Inc.) with five short bursts of 10 s followed by intervals of 30 s on ice. A supernatant was obtained by centrifugation at 4 °C for 30 min at 16,000 rpm using a refrigerated microcentrifuge (Eppendorf). For purification, cell lysis was performed using a French press at 900 p.s.i. Cell debris were pelleted by ultracentrifugation at 4 °C, 25,000 x g for 1 h. His-tag purification was obtained using Talon magnetic beads (Dynabeads, Qiagen).

Yeast Complementation—The yeast deletion strain yca1 (Y02453; yca1::kanMX4) in YOR197W and the wild type strain BY4741 (MATa his31 leu20 met150 ura30) were supplied by Euroscaf. pYES2 (Invitrogen) and pYES-AtMC8 were introduced in Y02453 and BY4741. The survival assay was carried out essentially as published (5). In short, yeast cultures were grown overnight with glucose or galactose, diluted to the same density, and then treated or not with 1.2 mM H₂O₂ (Sigma) for 24 h. Cells were counted using a Thoma double cell "Clearsight" chamber and 1000 cells plated on solid yeast extract/peptone/dextrose medium for each replicate. The survival rate was calculated using the number of colonies formed after 2 days at 30 °C.

Plant Transformation—pZP111-AtMC8 and pZP111-AtMC8^C140A were transformed into competent Agrobacterium tumefaciens GV3101 using electroporation. Agrobacterium strains were grown with appropriate antibiotics (20 mg·liter^–1 gentamycin, 50 mg·liter^–1 kanamycin, and 200 mg·liter^–1 rifampicin) and used to transform Arabidopsis Col0 by the floral dip method (24) in 10 mM MgCl_2, 300 µl·liter^–1 Silwet L-77 with 30 s of vacuum infiltration. Transformed seeds were collected and selected on 50 mg.liter^–1 kanamycin and 1% Bactoagar.

RT-PCR—Total RNA was extracted from 3-week-old seedlings grown in vitro using Invisorb Spin Plant RNA mini kit (Invitek, Gmbh) according to the manufacturer's instructions and then treated with RQ1 RNase-free DNase (Promega) for 60 min. The treated RNA was used to perform cDNA synthesis using Reverse-iT^TM First Strand Synthesis Kit (ABgene) following the protocol supplied with the kit. The resulting cDNA samples were used as templates for PCR reactions with Bioline Taq. To amplify the full-length ORF the following primers were used: MC8-ATG, 5'-TGG CGA AGA AAG CAC TTT TGA-3'; MC8-GGT, GGT CGT TGA CTA TAC CCC CGT. For expression studies the following primers were used: AtMC1-At1g02170, CTC CTC CGC AAC CTT CCT and CAT CAA CTT CAT CAC CGT TGT; AtMC2-At5g64240, TCT GGT CAT GGA TCT CAG CA and CTG TGT TCT TCC CCG TGA AC; AtMC3-At4g25110, TGG ACC ACA GGA CTT CAG GT and AAG CGC CTA AGA TGA GCA AA; AtMC4-At1g79310, TGA TTG ACA CCG ACG AAT CT and CTT CCG ATT CCA CAA AAA GC; AtMC5-At1g79340, GCT TGC TGA TCT CGT CGA A and GCT GCG CAA GAA CTT CCT AA; AtMC6-At1g79330, CGA AGG GCA TTG TTG AAT CT and GCT TCT TCC ACA GCT TCA CG; AtMC7-At1g79320, AGA TCT CGT TGA ACC GGC TA and TCC AAT GGC AGA GAT CTG TTT; AtMC8-At1g16420; GGA TAA TCT CAT CGC ATC AGG and GCT GCT TCA TAT GGC TTT CC; AtMC9-At5g04200, GTG TTC ACG GGG AAG AAC and GCG GAT GCA TCA GAG CTT; AtDAD1, GGA TGC TCA GGA TCT ATT TCG and GTG AAA CCT CTA TCC GAG GAA GTT G; Actin2, GTT AGC AAC TGG GAT GAT ATG G and CAG CAC CAA TCG TGA TGA CTT GCC C.

Q-PCR—cDNA was synthesized as described in the RT-PCR method and used as templates in Q-PCR reactions using Taqman Master mix (Eurogentec) according to the manufacturer's instruction and an ABI 7000. For 18S detection, the primers 18 S-29F (5'-GGT CTG TGA TGC CCT TAG ATG TT-3'), 18 S-102R (5'-GGC AAG GTG TGA ACT CGT TGA-3') and probe 18 S-58T (5'-CGC ACG CGC GCT ACA CTG ATG T-3') were used. For Actin2 detection, the primers ACT2-123F (5'-GAG AGA TTC AGA TGC CCA GAA GTC-3'), ACT2-190R (5'-TGG ATT CCA GCA GCT TCC A-3'), and probe ACT2-148T (5'-TCC CAC AAA CGA GGG CTG CAA CA-3') were used. For AtMC8 detection, the primers AtMC8-50F (5'-TGG AGT TAC GTG GCT GTG TCA-3'), AtMC8-124R (5'-TGT TGG CGA ACC CGT AAA G-3'), and probe AtMC8-79T (5'-CAC CGG ATG CAG AAA TGC CTA ATC GA-3') were used. A standard curve using dilutions of Arabidopsis genomic DNA was used to calculate the absolute number of cDNA copies in each sample.

H₂O₂ Measurement—The Amplex Red Hydrogen Peroxide/Peroxidase Assay kit (Invitrogen) was used to measure H₂O₂ production in 10⁵ protoplasts. After a treatment with 50 kJ·m^–2, the samples were kept in the light for 30 min before harvesting, and the Amplex Red reagent (10-acetyl-3,7-dihydrophenoxazine) was used according to the manufacturer's instruction.

Protease Assay—Standard 2x assay buffer was 20 mM HEPES, pH 7.4, 4 mM EDTA, 0.04% NaN₃, 50 mM CaCl₂, 6 mM dithiothreitol; the pH range was obtained using 100 mM sodium acetate for pH 4–5, 50 mM MES for pH 5.5–6.5, and 100 mM Tris-HCl for pH 7–9. Protein extracts were carried out in distilled water and 3 mM dithiothreitol. For plant extract the FW/buffer ratio was 1 g/2 ml. For yeast total protein was extracted from yeast cell pellets by adding glass beads and shaking with a Ribolyser. Protease activities were determined by incubation of 48 µl of plant extract (or 20 µl of yeast extract, 10 µl of E. coli extract, or 2 µl of purified AtMC8 made up to 48 µl with sterile distilled water), 50 µl of 2x assay buffer at different pH, and 50 µM t-butoxycarbonyl-GRR-aminomethylcoumarin (AMC) and benzyloxycarbonyl-FR-AMC (substrate for papain; Bachem Ltd). Ac-DEVD-AMC (substrate for caspase-3, -6, -7, -8, and -10; MP Biomedicals), Ac-VEID-AMC (substrate for caspase-6), Ac-YVAD-AMC (substrate for caspase-1), Ac-IETD-AMC (substrate for caspase-6 and -8, Granzyme B), and benzyloxycarbonyl-AAN-AMC (substrate for legumain) (Bachem) were used at 50 µM final. The release of AMC was measured every 2 min at 30 °C with a Microtiter Plate Fluorometer (Labsystems, DYNEX Technologies) using an excitation wavelength of 360 nm and an emission wavelength of 460 nm. Data time points were analyzed by the Fluoroskan Ascent software, and activities were expressed in fluorescence units/min/mg or µg of total protein. Protein concentration was measured using the Bradford reagent (Bio-Rad).

Immunodetection—Antibodies used comprised a rabbit polyclonal raised against purified recombinant AtMC8 (by Eurogentec). Acrylamide gels were cast and run using a Bio-Rad mini gel apparatus. Western analysis was carried out according to Sambrook et al. (25) using Hybond P (Amersham Biosciences). For signal detection ECL (Pierce) and Eastman Kodak Co. Biomax film were used.

Ion Leakage—Seedlings were grown in soil under short days for 4 weeks and watered 24 h before the experiment to avoid ion leakage variation linked to variation in water status. 1100 µl of sterile distilled water was added in each well of a 24-well culture plate (Techno Plastic Products). 3-mm diameter discs were punched out from leaves, and 3 discs were floated in each well. At 0.5 h, the conductivity of the water in each well was measured using 100 µl and an HORIBA Twin Cond conductivity meter B-173 (HORIBA Ltd, Kyoto, Japan). Stress treatment were carried by applying UVC radiation using a CL-1000 UV cross-linker (UVP Ltd) or the addition of H₂O₂ (Sigma) to the discs to reach the doses required, and the discs were left in continuous light at 22 °C for 16 h. The conductivity of the liquid in each well was measured again, and the difference before and after treatment was calculated to represent the amount of cell death of each sample. Three wells were used for each treatment.

Protoplasts and Evans Blue—Seedlings grown in vitro for 3–4 weeks were incubated with leaf digestion medium (4.41 g·liter^–1 Murashige and Skoog (MS) medium including Gamborg B5 vitamins (Duchefa), 0.4 M sucrose, 0.96% cellulase R-10, and 0.64% macerozyme (Yakult Pharmaceutical), pH 5.8) in the dark for 16 h at room temperature. Buoyant protoplasts were harvested by centrifugation for 5 min at 600 rpm and washed 2–3 times in 12 ml of W5 medium (154 mM NaCl, 5 mM KCl, 5 mM glucose, and 125 mM CaCl₂, pH 5.6–5.8). The pellet was then resuspended in protoplast culture medium (4.41 g·liter^–1 MS medium including Gamborg B5 vitamins, 0.4 M sucrose, 0.4 M mannitol, and 0.5 g·liter^–1 MES, pH 5.8) at a density of 1 x 10⁶ protoplasts per ml. For each replicate, 1 ml of protoplasts was used per well of a 6-well culture plate (Techno Plastic Products). Stress treatments were carried by applying UV radiation using a CL-1000 UV cross-linker (UVP Ltd) or exogenous application of H₂O₂ (Sigma) to wells in triplicate, and the protoplasts were left in continuous light for 4 h at 22°C. The dye Evans blue (Sigma) was added to protoplast suspension to the final concentration of 0.05%. After 5 min of room temperature incubation, an aliquot of the stained protoplasts was mounted on a slide. Pictures of at least four randomly selected fields of view (150–250 cells/field) were taken within 10 min. The ratio of number of Evans blue-stained cells over total cell number was calculated. All the microscopic work was carried using a Leica microscope connected to a digital SPOT camera.

Germination on Methyl Viologen—Seeds were sterilized for 10 min in 70% ethanol and sown on MS media with Gamborg B5 vitamins (Duchefa), 0.5g/liter MES, pH 5.8, 0.7% phytagel (Sigma). Plates were supplemented with 0, 0.25, or 25 µM methyl viologen (Sigma). Seeds were incubated for 3 days at 8 °C and then germinated at 22 °C in continuous light. Germination was scored using a stereomicroscope. Digital pictures were taken with a Nikon D100. Each treatment was carried out in triplicate with at least 100 seeds.

	RESULTS

TOP ABSTRACT INTRODUCTION EXPERIMENTAL PROCEDURES RESULTS DISCUSSION REFERENCES

 
AtMC8 Expression Is Induced by Oxidative Stress and Correlates with Cell Death—We have previously shown that a UVC treatment can induce PCD in Arabidopsis (26). Using RT-PCR and gene-specific primers, we analyzed the transcription during UVC-induced PCD of the nine metacaspases (AtMC1–9) that are present in the Arabidopsis genome. Three-week-old seedlings were treated with 50 kJ/m² and kept in the light. Total RNA was extracted 30 or 120 min after treatment. We found that the AtMC-8 transcript (At1g16420) was the only metacaspase strongly up-regulated, with a peak 30 min after UVC treatment (Fig. 1A). We found no transcript for AtMC6 and AtMC7. AtMC1, -2, -3, and -5 were present and down-regulated by the UV treatment. AtMC-4 was expressed at a low level and slightly up-regulated with higher expression at 2 h. AtMC9 was slightly up-regulated. The expression of AtMC8 was then analyzed using Taqman Q-PCR. Q-PCR results (Fig. 1B) showed that a lethal UV dose of 50 kJ/m² is required to induce the expression of AtMC8 80-fold using 18 S as a reference gene. Using ACTIN2 as a reference gene instead of 18S resulted in a calculated induction of 120-fold (data not shown) because UVC down-regulates ACTIN2. A sublethal dose of 1 kJ/m² was ineffective, and a 10 kJ/m² resulted in a 10-fold induction, indicating that expression of the AtMC8 transcript is proportional to the level of stress. To investigate whether AtMC8 induction could be linked either to the induction of PCD or linked to the general stress caused by the UV treatment, we analyzed its expression level under heat and light stresses thought to be associated with a UV treatment (Fig. 1B). Light stress (1000 µmol/m²/s), and heat shock (42 °C, 2 h) did not induce the expression of AtMC8. Finally, we have shown that UV-induced PCD is light-dependent (27), and our experiments showed that light was required after UVC treatment to induce AtMC8 expression, suggesting a correlation between the expression of AtMC8 and the induction of PCD. A light requirement suggested a link with oxidative stress. H₂O₂ production was measured using 10⁵ protoplasts treated with 50 kJ·m^–2 UVC and was found to be 8.5 µM, 30 min after treatment. Untreated protoplasts only generated 0.4 µM H₂O₂.H₂O₂ was found to induce AtMC-8 expression 23-fold, 5 h after seedlings were transferred on MS media supplemented with 30 mM (Fig. 1C). To further investigate a link with oxidative stress and cell death, we analyzed the effect of methyl viologen, an herbicide that induces an apoptotic-like PCD (28) and causes the production of superoxide in the chloroplast, which is converted into H₂O₂. Methyl viologen (MV) was found to induce AtMC8 expression 64-fold, 5 h after seedlings were transferred on MS media supplemented with 25 µM (Fig. 1C). This concentration caused bleaching and cell death of seedlings (not shown). To establish whether the oxidative stress inducing AtMC8 expression originated from the chloroplast, we analyzed the transcript level of AtMC8 in the mutant rcd1-1. RCD1 is proposed to regulate specific stress-responsive genes, and rcd1 is insensitive to ROS produced by the chloroplast (29). A 50-kJ UVC treatment was found to cause an actual 5-fold decrease of the expression of AtMC8 in the rcd1-1 background rather than an increase (Fig. 1D), similar to the effect of UVC on ACTIN2 and members of metacaspase gene family. There was a similar reduction of expression when transferring rcd1-1 seedlings to solid media supplemented with 25 µM MV. This suggested that in the absence of an RCD1-mediated induction by oxidative stress, AtMC8 expression is subject to a general down-regulation of expression by stress. This general down-regulation is seen with some members of the metacaspase gene family (Fig. 1A), and our microarray data indicate that most protease transcripts are down-regulated after UV treatment (Affymetrix microarray data⁵). Induction of expression by H₂O₂ and MV added to a requirement for a functional RCD1 suggested that an oxidative stress generated at the chloroplast level induces AtMC8 expression. In all, these results show a correlation between AtMC8 expression, oxidative stress, and cell death. Metacaspase-8 was, therefore, selected for further studies bearing in mind that a correlation at the expression level is not proof of a definitive link between metacaspase-8 and PCD.

View larger version (37K): [in this window] [in a new window]   FIGURE 1. AtMC8 expression is up-regulated by oxidative stress. A, 3-week-old A. thaliana Col-0 seedlings were grown in vitro, treated with UV-C (50 kJ/m2), and harvested after 30 min or 2 h in the light; control plants (CL) were not treated with UV-C. cDNAs were synthesized from DNase-treated RNA samples, and RT-PCR was performed with gene-specific primers for each member of the metacaspase genes family in A. thaliana (AtMC-1–9) and AtDAD1 as a reference gene. B, total RNA was extracted from Col-0 seedlings grown in vitro for 3 weeks. cDNAs were synthesized from DNase-treated RNA samples and analyzed using Taqman Q-PCR. Transcript levels are given as AtMC8/18S copy number ratio using the untreated sample + light (CL) as a value of 1. Various treatments were: untreated and kept in light (CL) or in the dark (CD); 1-h light stress and kept in the light (LL) or in the dark for 1 h (LD); seedlings irradiated with 1 kJ·m–2, 10 kJ·m–2, or 50 kJ·m–2 UV-C and kept in the light (1KL, 10KL, and 50KL) or kept in the dark for 1 h (1KD, 10KD, and 50KD); seedlings heat-shocked at 42 °C 2 h and kept in the light (42L) or in the dark for 1 h (42D). C, 3-week-old Col-0 seedlings grown in vitro on solid MS medium were transferred on MS medium supplemented with 30 mM H2O2 or 25µM MV for 5 h. cDNAs were synthesized from DNase-treated RNA samples and analyzed using Taqman Q-PCR. Error bars indicate ±S.D. of three replicates. D, 3-week-old seedlings of the mutant rcd1-1 grown in vitro on solid MS medium were untreated (CL), treated with 50 kJ/m2 UVC (50KL), and left in the light for 1 h or transferred on MS medium supplemented with 25 µM MV for 5 h. cDNAs were synthesized from DNase-treated RNA samples and analyzed using Taqman Q-PCR. Error bars indicate ±S.D. of three replicates.

Recombinant AtMC8 Cleaves Substrates with R in p1 and Is More Active at pH 7.5–8.5—An AtMC8 cDNA was obtained using RT-PCR and RNA from UV-treated seedlings. AtMC8, a type II metacaspase, is a cysteine protease with a predicted size of 42.5 kDa. Previous studies have shown there is a clear conservation of the cysteine-histidine dyad in the catalytic center for cysteine proteases (2). To establish whether activity was required for the function of AtMC8 in cell death, the cysteine residue in position 140 was mutated to create a nonfunctional allele. AtMC8 and AtMC8^C140A were cloned in the expression vector PET-30, which enables detection and purification of the recombinant protein using a His tag or an S tag. Western analysis confirmed that the protein was expressed upon induction using isopropyl 1-thio-β-D-galactopyranoside (Fig. 2A). Immunodetection using an antibody against AtMC8 confirmed the production of a 50-kDa protein corresponding to the full-length-tagged metacaspase. The soluble protein fraction and the His-purified enzyme presented evidence of activation by cleavage, generating a p20-like subunit at 29 kDa as described for other metacaspases (7, 8, 16). Enzymatic assays on E. coli extracts and purified recombinant protein confirmed that AtMC8 has no activity against the caspase substrates DEVD, YVAD, IETD, or VEID (Fig. 2B). Of the substrates tested, AtMC8 was able to cleave the papain substrates FR and GRR (Fig. 2B). This activity was abolished with the mutation of the predicted catalytic cysteine in the recombinant AtMC8^C140A. The optimum pH was determined to be between 7.5 and 8.5 with no activity below pH 6 (Fig. 2C). AtMC8 expressed in yeast using the yeast expression vector pYES2 showed the same substrate specificity as the recombinant AtMC8 produced in E. coli (data not shown).

View larger version (21K): [in this window] [in a new window]   FIGURE 2. Recombinant AtMC8 shows GRR and FR cleavage activity. A, expression of AtMC8 in E. coli. A lysate from non-induced E. coli was prepared as a control (lane 1). A crude cell lysate was prepared from the induced culture (lane 2) and the C- and N-His tag were used to purify AtMC8 using TalonTM beads (lane 3). Samples were immunoblotted and analyzed using a polyclonal antibody raised against AtMC8. Full-length tagged AtMC8 has an approximate molecular mass of 50 kDa (arrow a). The 29-kDa band (arrow b) is thought to be the p20-like subunit resulting from activation by autoprocessing. B, recombinant AtMC8 and the null allele AtMC8C140A were incubated at pH 8 at 30 °C with 10 µM benzyloxycarbonyl-FR-AMC (FR) or t-butoxycarbonyl-GRR-AMC (GRR), 50 µM caspase substrates Ac-DEVD-AMC (DEVD), Ac-YVAD-AMC (YVAD), Ac-VEID-AMC (VEID), and Ac-IETD-AMC (IETD), legumain substrate benzyloxycarbonyl-AAN-AMC (AAN), calpain substrate Suc-LLVY-AMC (LLVY). Note the change of scale in the inset. Protease activity is given as fluorescence unit/min/µg or mg of total protein. Error bars represent the S.D. of three replicates. FU, fluorescence units. C, proteolytic activity of AtMC8 against 50 µM t-butoxycarbonyl-GRR-AMC at different pH values. Relative activity is expressed as the percentage of the optimal activity. The error bar is the S.D. of triplicates.

View larger version (33K): [in this window] [in a new window]   FIGURE 3. Expression of AtMC8 complements the reduced cell death phenotype of yeast metacaspase knock-out cells. A, detection of AtMC8 in yeast protein extracts. AtMC8 expression was induced in yeast yca1 knockout Y02453 (KO) by shifting from glucose (–) to galactose (+). pYES is the empty expression vector. Protease extracts were immunoblotted using an antibody against AtMC8. KO+pYES is Y02453 + empty pYES2; KO+AtMC8 is Y02453+ pYES2-AtMC8. B, complementation. After 24 h of growth in SCD medium, yeast cultures were transferred to a galactose-containing medium for an overnight induction period and then treated with 1.2 mM H2O2 for 24 h. The survival was expressed as the number of colonies grown of 1000 cells plated on YPD plates. WT+pYES is wild type + empty pYES2; KO+pYES is Y02453 + empty pYES2; KO+AtMC8 is Y02453 + pYES2-AtMC8. Error bars indicate ±S.D. of triplicates.

To confirm those results with a different experimental system, protoplasts were prepared from homozygous lines overexpressing AtMC8 or AtMC8^C140A. PCD was then induced by applying H₂O₂. Measurements using Evans blue were conducted after 4 h incubation under continuous light. A dose of 100 µM H₂O₂ did not induce cell death in wild type Col-0; by contrast, in lines overexpressing AtMC8, there was a 2-fold increase in cell death, going from 8 to 15%. Overexpressing the inactive metacaspase, AtMC8^C140A, did not increase protoplast cell death when treated with 100 µM H₂O₂ (Fig. 4E). The effect of overexpression was also studied using UV, and protoplasts were prepared from transgenic plants. A dose of 5 kJ/m² was used in this experiment, causing no cell death increase in protoplasts prepared from wild type Col-0 seedlings. Similar to PCD induction by H₂O₂, cell death increased 2-fold with protoplasts from over-expressers, and protoplasts overexpressing AtMC8^C140A showed a cell death close to that of wild type protoplasts (Fig. 4F). Therefore, overexpressing AtMC8 increased the sensitivity of Arabidopsis to the two PCD inducers used in these experiments. Overall, the increased ion leakage or cell death correlated with the increase at the enzymatic level, albeit an attenuation of this correlation in protoplasts. In experiments with increasing H₂O₂ or UV doses, the increased death in the Ox lines became less obvious as the difference with wild type is reduced (data not shown). Therefore, overexpressing AtMC8 caused an increased sensitivity at the low dose end of the spectrum.

View larger version (33K): [in this window] [in a new window]   FIGURE 4. Increased ion leakage and protoplasts cell death in lines overexpressing AtMC8. Three lines overexpressing AtMC8 (Ox5, Ox7, Ox12) and two lines overexpressing AtMC8C140A (C140A5, C140A8) were selected. Col-0 is the genetic background of the over-expressers. A, level of AtMC8 transcript in over-expressers. Total RNA was extracted from leaves. cDNA synthesized from DNase-treated RNA was used to carry out Taqman Q-PCR analysis using 18 S transcript as the internal reference. Expression of AtMC8 in Col-0 is around 1% of 18 S. Error bars indicate ±S.D. of the mean of three replicates. B, Phe-Arg-ase activity in over-expresser plants. Seedlings grown in vitro for 3 weeks were treated with 50 kJ·m–2 UVC and incubated in the light for 1 h, and total soluble proteins were extracted. Protein extracts were incubated in the presence of 10 µM Ac-FR-AMC substrate at 30 °C for 30 min. The activity is expressed as fluorescence units/min/µg of protein; error bars indicate ±S.D. of the mean of three replicates. C and D, 3-mm-diameter leaf discs were punched from 4-week-old plants floated on sterile distilled water. Water conductivity was measured before treatment and 16 h after treatment with 20 mM H2O2 (C) or 5 kJ·m–2 UV (D). E and F, protoplasts isolated from 3–4-week-old seedlings grown in vitro were treated with the sublethal doses of 100 µM H2O2 (E) or 5 kJ·m–2 UV (F). Protoplasts death was scored using Evans blue uptake. For each replicate at least 200 protoplasts were examined. Error bars represent ±S.D. of three replicates.

There was no obvious morphological phenotype during development of the KO lines compared with their wild type. The wild type and KO lines were then exposed to UV or H₂O₂ in leaf discs or protoplasts. The two different wild type ecotypes, WS and Ler, were shown to have different thresholds of cell death induction, Ler being less sensitive than WS, and doses applied were adjusted accordingly. Experiments using leaf discs and H₂O₂ indicated that knocking out AtMC8 had little effect on cell death measured using ion leakage as a marker. Only the mutation in the Ler background showed a significant reduction of ion leakage when challenged with UV (Fig. 5, B and C). By contrast, protoplast experiments were very clear. In both KO lines and using either H₂O₂ or UV, knocking the gene in a Ler or WS background resulted in a reduction of cell death by 30–40% (Fig. 5, D and E).

View larger version (27K): [in this window] [in a new window]   FIGURE 5. Ion leakage and protoplasts cell death in two AtMC8 KO lines. A, localization of the selected T-DNA insertions in the AtMC8 gene. Closed boxes represent exons. The positions of the ATG, stop codon, and the two AtMC8-1 and AtMC8-2 T-DNA insertions are indicated. The conserved histidine 86 and cysteine 140 of the catalytic site are highlighted. B and C, 3-mm-diameter leaf discs were punched off our week-old plants and floated on sterile distilled water. Water conductivity was measured before treatment and 16 h after H2O2 (B) or UV(C) treatment. D and E, protoplasts isolated from 3-weeks-old in vitro grown seedlings were treated with H2O2 (D) or UV(E). AtMC8-1 and AtMC8-2 are KO lines in AtMC8; WS, genetic background of AtMC8-1; Ler, genetic background of AtMC8-2. Protoplasts cell death was scored using Evans blue uptake. To make ecotypes comparable, the untreated values have been subtracted from the treated values. For each replicate at least 200 protoplasts were examined. Error bars represent ±S.D. of three replicates.

View larger version (33K): [in this window] [in a new window]   FIGURE 6. AtMC8 KO lines have reduced sensitivity to methyl viologen. Sterile seeds were plated in vitro on solid MS media supplemented with 0, 0.25, or 25 µM methyl viologen and placed to germinate in continuous light, 22 °C. A, germination was scored at 6 days; error bars represent S.D. of triplicates. B, seedlings of wild types and knock-out lines, photographed at day 9, representative of the 100 seeds plated for each genotype. White scales represent 5 mm.

	DISCUSSION

TOP ABSTRACT INTRODUCTION EXPERIMENTAL PROCEDURES RESULTS DISCUSSION REFERENCES

There is a striking expression pattern of AtMC8 during PCD induced by UV, which our results show correlated with a PCD phenotype. This correlation is reinforced by the fact that H₂O₂ and MV induce cell death and AtMC8 expression This gene is the only one in the metacaspase family that is induced strongly by our UV treatment; the transcript is present at very low levels in seedlings, and it is induced as soon as 30 min after a UV treatment leading to PCD. This induction of expression precedes an increase in caspase-3 like activity peaking at 1 h (our data). AtMC8 induction is dependent of a functional RCD1, and this dependence places AtMC8 in an oxidative stress pathway activated by ROS produced in chloroplast, possibly after damage by UV radiation. This is consistent with methyl viologen, generating and H₂O₂ in chloroplasts that in turn induce AtMC8 expression. Genetically, AtMC8 could be downstream of RCD1 as RCD1 has been shown to interact with transcription factors (35) that may in turn interact with the AtMC8 promoter. Another possibility is that the rcd1-2 mutant has been reported to up-regulate reactive oxygen species scavenging enzymes (36), and this may explain indirectly why AtMC8 is not induced in the rcd1-1 background by UVC or MV. Interestingly, rcd1-1, although ozone-sensitive, is resistant to MV (29), reinforcing the idea that RCD1 and AtMC8 are in the same pathway. Crucially, AtMC8 induction is dependent of the seedlings being kept in the light after the UV treatment, as is cell death. This expression pattern suggests that AtMC8 is involved in the process of a light-dependent PCD induced here by UV. Light dependence has been shown in several examples of cell death such as developmental cell death in Monstera (37), fumonisin (38), singlet oxygen cell death (39), and hypersensitive response (40). Little is yet known as to how light dependence is integrated in plant PCD molecular cascades, but we suggest here that AtMC8 is part of it.

The over-expressers showed increased cell death both in ion leakage and protoplasts experiments. This increase requires a functional catalytic site. The attenuated correlation between the increased enzymatic activity in Ox plants and protoplasts cell death suggests that additional limiting factors control cell death in protoplasts in addition to metacaspase-8 activity. Compared with the very clear and consistent phenotype obtained using over-expressers, the two independent KO data are more complex and appear to vary with the ecotype used. Germination test on MV using the KO lines showed a clear effect of the mutations with a lower sensitivity to death-inducing doses in both genetic backgrounds. Similarly, the reduction of cell death is obvious using protoplasts again in both genetic backgrounds, albeit some variation; however, the induced cell death is not totally abolished. The simplest explanation is that AtMC8 is probably not the only Arabidopsis metacaspase to be involved in the PCD process induced by UV or H₂O₂. Our RT-PCR experiments indicated that after UV treatments, up to seven metacaspases are expressed at various levels with AtMC2 and -9 being the most abundant at the transcript level. We are aware that these other members of the metacaspase family that remain constitutively expressed may also contribute to the oxidative stress PCD pathway via activation at the protein level. Unexpectedly, when using leaf discs and ion leakage, only UV and the Ler background show a small significant effect. The absence or small phenotype in leaf discs suggests that removing the cell wall in protoplasts may remove components that compensate for the loss of AtMC8 in the PCD process in leaf discs. Alternatively, metacaspase-8 may be required for loss of viability measured by Evans blue but not required for ion leakage. As a cell death marker, ion leakage may be upstream of Evans blue. This situation is reminiscent of experiments in A. fumigatus where metacaspases are required for phosphatidylserine exposure and not for loss of viability (14).

Although our data suggest a link between PCD and AtMC8, overexpressing AtMC8 in Arabidopsis is not lethal but makes plants more sensitive to UV or H₂O₂. The viability of overexpresser plants points at a control mechanism that maintains the metacaspase-8 pathway inactive in the absence of a cell death signal. Possibly, there are essential components of the PCD machinery that are downstream of AtMC8 and absent in non-induced plants. Alternatively, AtMC8 is subject to two levels of regulation, the first at the level of transcription and the second at the level of the proteolytic activity. Members of the serpin family are good candidates for regulating enzymatic activity since a serpin has been shown to inhibit AtMC9 (15). In addition, S-nitrosylation has been put forward as a possible mechanism for metacaspase activity inhibition in planta (41). This suggests that a critical level of activated metacaspase needs to be reached to trigger PCD; with overexpression, this level is reached at lower doses of the inducer. This control of enzymatic activity would possibly be lost during protein extraction. Finally, it cannot be excluded that metacaspase-8 may be involved in the signaling toward PCD rather than in the execution of it.

We show here that AtMC8 mediates cell death induced by addition of H₂O₂, and this is similar to the situation in yeast (5). This suggests that H₂O₂ activates an ancestral pathway present in both yeast and Arabidopsis. This is reinforced by the fact that when we overexpressed AtMC8 in a yeast yca1 knock-out strain, this expression was able to rescue the no-PCD phenotype in the presence of H₂O₂. It should be noted that AtMC1 (or 1b) and AtMC6 (or 2b) are also able to complement the same yeast yca1 knock-out (7).

Using expression in E. coli, we showed here that AtMC8 has an affinity for the substrates FR or GRR and is unable to cleave the caspase synthetic substrates tested. This is supported by our overexpression data in yeast and Arabidopsis. Four of the nine Arabidopsis metacaspases, AtMC1, -4, -6, and -9 have also been shown to be arginine/lysine-specific cysteine proteases and unable to cleave caspase-specific synthetic substrate, reinforcing the observation that metacaspases are not plant caspases. We found AtMC8 to be more active at pH 7 to 8.5, suggesting that AtMC8 most likely functions in the cytoplasm or organelles with neutral pH. These observations make AtMC8 clearly different from AtMC9, which has an optimum pH of 5.5 and is localized in the cell wall (15). By virtue of this difference, it seems unlikely that AtMC8 is localized in the cell wall. In addition, overexpressing or ablating AtMC8 expression affects cell death in protoplasts, cells that have been stripped of their cell wall. This phenotype in protoplasts also suggests that AtMC9 is not involved, as AtMC9 should be removed or depleted during protoplast preparation.

In summary, we have shown that in Arabidopsis metacaspase-8 mediates cell death induced by reactive oxygen species. This is an important step, but much remains to be discovered about the pathway involved and the position of AtMC8 in the cascade in relation to light and RCD1. The protein targets that are cleaved by metacaspase-8 and the molecular steps that lead to its activation at the gene or protein level remain to be identified and will help defining the pathway.

	FOOTNOTES

 
^* This work was supported in part by a Biotechnology and Biological Sciences Research Council, Swindon, United Kingdom, research grant. The costs of publication of this article were defrayed in part by the payment of page charges. This article must therefore be hereby marked "advertisement"in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

¹ Present address: College of Chinese Materia Medica, Guangzhou University of Chinese Medicine, Guangzhou, 510405, China.

² Recipient of a Biotechnology and Biological Sciences Research Council studentship.

³ To whom correspondence should be addressed. Tel.: 44-161-275-3922; Fax:44-161-275-3938; E-mail: patrick.gallois{at}manchester.ac.uk.

⁴ The abbreviations used are: PCD, programmed cell death; KO, knock out; WS, Wassilewskija; Ler, Landsberg erecta; MS, Murashige and Skoog; MV, methyl viologen; ORF, open reading frame; RT, reverse transcription; CHAPS, 3-[(3-cholamidopropyl)dimethylammonio]-1-propanesulfonic acid; Q-PCR, quantitative-PCR; AMC, aminomethylcoumarin; MES, 4-morpholineethanesulfonic acid.

⁵ V. Delorme and P. Gallois, unpublished data.

	ACKNOWLEDGMENTS

 
We thank Dr. Jonathan Clarke for help with the GT line. We thank Andrew Buck Roxane Denis and Lydia Wunderley for excellent technical help.

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TOP ABSTRACT INTRODUCTION EXPERIMENTAL PROCEDURES RESULTS DISCUSSION REFERENCES

 

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