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Plant Physiology Preview. Published on December 1, 2006, as DOI:10.1104/pp.106.090878 Running head: BI-1 associated with ion homeostasis 5 Correspondence; Dr. Maki Kawai-Yamada Institute of Molecular and Cellular Biosciences The University of Tokyo 10 1-1-1 Yayoi, Bunkyo-ku, Tokyo 113-0032, Japan Tel & Fax: +81-3-5841-8466 E-mail: [email protected] 15 Research area: Cell Biology 1 Downloaded from on June 18, 2017 - Published by www.plantphysiol.org Copyright © 2006 American Society of Plant Biologists. All rights reserved. Copyright 2006 by the American Society of Plant Biologists Title: Cell death suppressor, Arabidopsis BI-1, is associated with calmodulin-binding and ion homeostasis 20 Yuri Ihara-Ohori1, Minoru Nagano1, Shoshi Muto2, Hirofumi Uchimiya1, Kawai-Yamada1, 4 * 25 1 Institute of Molecular and Cellular Biosciences, The University of Tokyo, 1-1-1 Yayoi, Bunkyo-ku, Tokyo 113-0032, Japan (Y.I-O., H.U., M.K-Y) 2 Nagoya University Bioscience Center, Nagoya University, Chikusa, Nagoya 464-8601, Japan (S.M.) 30 3 Iwate Biotechnology Research Center, Kitakami, Iwate 024-0003, Japan (H.U) 4 Japan Science and Technology Agency (JST), CREST, 4-1-8 Honcho, Kawaguchi, Saitama 332-0012, Japan (M.K-Y) This paper is dedicated to the memory of the late Prof. Muto. 35 2 Downloaded from on June 18, 2017 - Published by www.plantphysiol.org Copyright © 2006 American Society of Plant Biologists. All rights reserved. 3 and Maki Financial source: This work was supported by a Grant-in-Aid for Scientific Research on Priority Arias (Grant No. 40 17051006) from the Ministry of Education, Culture, Sports, Science and Technology of Japan, a grant from the Ministry of Agriculture, Forestry, and Fisheries of Japan, and from CREST, JST (to M.K-Y). 45 Corresponding author Dr. Maki Kawai-Yamada Institute of Molecular and Cellular Biosciences 50 The University of Tokyo, 1-1-1 Yayoi, Bunkyo-ku, Tokyo 113-0032, Japan Tel & Fax: +81-3-5841-8466 E-mail: [email protected] 55 3 Downloaded from on June 18, 2017 - Published by www.plantphysiol.org Copyright © 2006 American Society of Plant Biologists. All rights reserved. ABSTRACT Cell death suppressor Bax inhibitor-1 (BI-1), an endoplasmic reticulum (ER) membrane protein, exists in a wide range of organisms. The split-ubiquitin system, overlay assay and the bimolecular fluorescence complementation (BiFC) analysis demonstrated that Arabidopsis 60 BI-1 (AtBI-1) interacted with calmodulin (CaM) in yeast and in plant cells. Furthermore, AtBI-1 failed to rescue yeast mutants lacking Ca2+-ATPase (Pmr1 or Spf1) from Bax-induced cell death. Pmr1 and Spf1, p-type ATPases localized at inner membrane, are believed to be involved in transmembrane movement of calcium ion in yeast. Thus, the presence of intact Ca2+-ATPases was essential for AtBI-1-mediated cell death suppression in yeast. To 65 investigate the effect of AtBI-1 on calcium homeostasis, we evaluated sensitivity against cyclopiazonic acid (CPA), an inhibitor of SERCA-type Ca2+ ATPases, in AtBI-1 overexpressing or knock-down transgenic Arabidopsis plants. These plants demonstrated altered CPA or ion stress sensitivities. Furthermore, AtBI-1 overexpressing cells demonstrated attenuated rise in cytosolic calcium following CPA- or H2O2- treatment, suggesting that AtBI-1 70 affects ion homeostasis in plant cell death regulation. 4 Downloaded from on June 18, 2017 - Published by www.plantphysiol.org Copyright © 2006 American Society of Plant Biologists. All rights reserved. INTRODUCTION In higher plants, programmed cell death (PCD) plays a vital role in proper biogenesis and morphogenesis, similar to apoptosis in animal cells where some biotic or abiotic stimuli trigger 75 the death pathway resulting in mitochondrial dysfunction, generation of reactive oxygen species (ROS) and activation of specific proteases. In apoptosis, Bax, a proapoptotic member of the Bcl-2 family proteins, is activated by certain apoptotic stimuli, and then translocates into the mitochondrial membrane, causing mitochondrial dysfunction (Wei et al., 2001). Some features of plant PCD, including hypersensitive reaction (HR), resemble the apoptotic process. 80 Thus in plant PCD: (i) caspase-like protease activity is observed during tobacco-mosaic virus (TMV)-induced HR (Chichkova et al., 2004), (ii) vacuolar processing enzyme (VPE) has caspase-1 activity and mediates TMV-induced HR in tobacco (Hatsugai et al., 2004; Hara-Nishimura et al., 2005). In addition, mammalian Bax is capable of inducing cell death in yeast (Zha et al., 1996) and also plant cells (Lacomme and Cruz, 1999). Such evidences suggest 85 the existence of a common mechanism for animal and plant cell death pathways. In animal cells, intracellular calcium level plays an important role in death pathways triggered by apoptotic stimuli. Several studies suggested that the amount of calcium ion stored in ER determines the sensitivity of the cells to apoptotic stress (Pinton et al., 2001; Scorrano et al., 2003). It was also suggested that translocation of calcium ions from the ER to the 90 mitochondrion may be required to induce cell death by some apoptotic signals; alteration of calcium level in ER could signal apoptotic cell death (Scorrano et al, 2003). On the other hand, over-expression of Bcl-2 reduces ER calcium level (Foyouzi-Youssefi et al., 2000), suggesting that the effect of anti-apoptotic proteins on the apoptosis may be mediated by regulation of calcium flux. 95 Bax inhibitor-1 (BI-1) was first identified as a suppressor of Bax-induced cell death on screening of human cDNA library in yeast cells (Xu and Reed, 1998). Although no homolog of 5 Downloaded from on June 18, 2017 - Published by www.plantphysiol.org Copyright © 2006 American Society of Plant Biologists. All rights reserved. the Bcl-2 family proteins have been identified in plants and yeast, BI-1 is widely conserved in organisms including Caenorhabditis elegans and Xenopus laevis (Hückelhoven 2004). Overexpression of Arabidopsis BI-1 (AtBI-1) suppresses Bax-induced cell death in 100 Arabidopsis and yeast (Kawai et al., 1999; Sanchez et al., 2000; Kawai-Yamada et al., 2001; Kawai-Yamada et al., 2004). Bax expression in plant cells causes ROS generation, organelle disruption and ion leakage from cells (Baek et al., 2004; Yoshinaga et al., 2005). AtBI-1 prevents ion leakage but not ROS generation when overexpressed together with Bax in Arabidopsis (Kawai-Yamada et al., 2004). In addition, H2O2-, SA-, elicitor-, heat- and 105 cold-induced cell death were suppressed in plant cells overexpressing AtBI-1 (Matsumura et al., 2003; Chae et al., 2003; Kawai-Yamada et al., 2004). Moreover, tobacco BY-2 cells became sensitive to sucrose starvation after overexpression of antisense BI-1 (Bolduc and Brisson, 2002, Bolduc et al., 2003). It was recently reported that cells from BI-1-deficient mice showed hypersensitivity toward agents that induce endoplasmic reticulum (ER) stress, such as 110 tunicamycin or thapsigargin (Chae et al., 2004). However, the mechanism of BI-1-mediated suppression of cell death is still unclear. The barley Mlo protein, a plant-specific plasma membrane protein, is known as a modulator of cellular defense and cell death (Piffanelli et al., 2002). Recently, it was shown that overexpression of barley BI-1 in mlo5 resistant cultivar restored Mlo function in 115 penetration by Blumeria graminis (Hückelhoven et al., 2003), suggesting that AtBI-1 and Mlo may possess similar functions in cellular defense and cell death modulation. Moreover, it was demonstrated that the barley Mlo protein binds to calmodulin (HvCaM3) and the interaction is related to the control of its function (Kim et al., 2002). Calmodulins facilitate Ca2+ -dependent responses through binding to their target proteins and modulate their activities. We were 120 inspired by these facts to study the interaction of BI-1 and calmodulin. Here we show that 6 Downloaded from on June 18, 2017 - Published by www.plantphysiol.org Copyright © 2006 American Society of Plant Biologists. All rights reserved. AtBI-1 can also interact with calmodulin and the cell death suppression activities of AtBI-1 in plant cells are mediated, at least in part, by modulation of ion homeostasis. Results 125 AtBI-1 interacts with calmodulin Overexpression of barley BI-1 in resistant mlo5 barley plant results in almost completely reconstitution of susceptibility to penetration by Blumeria graminis (Hückelhoven et al., 2003), suggesting that BI-1 and Mlo, CaM -binding protein, possess similar functions in plant defense 130 system. Thus, we tried to evaluate the interaction between CaM and BI-1 proteins. The plasmid possessing barley calmodulin 3 protein (HvCaM3) was kindly provided by Dr. Ralph Panstruga (Max-Planck Institute). The yeast split-ubiquitin system demonstrated that AtBI-1 interacted with HvCaM3 (Figure 1). As reported previously, AtBI-29, 30 and 32 are C-terminal mutants of AtBI-1 (Kawai-Yamada et al., 2004). Although the AtBI-29 and 32 mutants 135 maintained inhibitory function toward Bax-induced cell death in yeast, the AtBI-30 lacked the C-terminal coiled-coil structure and such function (Kawai-Yamada et al 2004) (Figure 1A). As shown in Figure 1B, AtBI-29 and 32 maintained the interaction with HvCaM3, while AtBI-30 did not. These results suggest the possibility that such interaction may be necessary for the suppressive action of AtBI-1 on Bax-induced cell death. 140 To further investigate the interaction between AtBI-1 and Arabidopsis calmodulin, in vitro overlay assay was performed. HvCaM3 is almost identical to Arabidopsis CaM7 (AtCaM7; Zielinski, 2002) with only one amino acid substitution (A11 →S 11). S- and His- tagged AtCaM7 expressed in Escherichia coli was purified by Ni-NTA resin. MBP-tagged C-terminal 14 amino acids of AtBI-1 (BI-C) or β-galactosidase (control; gal) purified by 145 amylose resin were used for the overlay assay. As shown Figure 2, purified BI-C and gal 7 Downloaded from on June 18, 2017 - Published by www.plantphysiol.org Copyright © 2006 American Society of Plant Biologists. All rights reserved. proteins were immunoblotted with anti-MBP antibody. The membrane was re-probed with recombinant AtCaM7 protein in the presence of 1 mM CaCl2 or 5 mM ethylene glycol bis (beta-aminoethyl ether)-N,N,N',N'-tetraacetic acid (EGTA). The AtCaM7 bound to the BI-C, although this protein did not bind to the gal protein (control). EGTA inhibited such binding, 150 confirming the importance of calcium in the calmodulin-mediated binding. To verify AtBI-1/CaM binding in planta, BiFC assay was performed in Agrobacterium-infiltrated tobacco (Nicotiana benthamiana) leaves. As previously reported, the GFP-tagged AtBI-1 protein (AtBI-GFP) localized to the perinuclear region, which is an indicative of ER localization, in tobacco epidermal cells (Figure 3F). When the AtBI-1-fused to 155 the N-terminal YFP fragment and AtCaM7-fused with C-terminal YFP were coexpressed in tobacco leaves, a strong BiFC signal was detected in the epidermal cells (Figure 3A, C, and E), confirming the interaction of AtBI-1 and AtCaM7 in planta. Control experiments in which pSPYNE-AtBI-1 and un-fused pSPYCE were coexpressed, did not show any fluorescence (Figure 3B and D). 160 Involvement of calcium pump in BI-1 function An increase in cytosolic Ca2+ has been implicated in the signal transduction pathway that mediates apoptosis (Pinton et al., 2001). It is possible that members of Bcl-2 family affect the apoptotic process by modulating ion fluxes in the cell (Lam et al., 1994). Based on the above 165 background, we then investigated the role of proteins involved in calcium transport on the inhibitory function of AtBI-1 against Bax-induced cell death in yeast. As shown in Table 1, we employed several mutants deficient in calcium homeostasis-related proteins. Mid1, Yvc1 and Cch1 are Ca2+-channels located in ER and plasma membrane (PM), vacuole, and PM, respectively (Bertl and Slayman 1990; Locke et al., 2000; Yoshimura et al., 2004). Spf1, Pmc1 170 and Pmr1 are Ca2+-ATPases localized in endomembranes (Cunningham and Fink 1994; Antebi 8 Downloaded from on June 18, 2017 - Published by www.plantphysiol.org Copyright © 2006 American Society of Plant Biologists. All rights reserved. and Fink 1992; Cronin et al., 2002). Vcx1 is a vacuolar H+/Ca2+ antipoter, and Ccc1 localized on vacuole is involved in iron, manganese and Ca2+-homeostasis in yeast (Cunninghan and Fink 1994; Lapinskas et al., 1996). To evaluate the anti-apoptotic function of AtBI-1, wild type (WT) yeast line and mutants possessing Yep51-Bax plasmid were transformed with 175 pYX112-AtBI, which were then subjected to spot assay. The growth curve of these yeast strains expressing AtBI-1 were almost same, and sensitivities of these yeast strains against Bax-induced cell death were also similar (data not shown). As shown in Figure 4A and B, WT and most mutants expressing both Bax and AtBI-1 grew on galactose containing medium. However, ∆pmr1 and ∆spf1 cells failed to grow by the expression of Bax even when AtBI-1 180 was overexpressed. RT-PCR demonstrated that deficiency in Pmr1 and Spf1 did not affect the AtBI-1 expression (Figure 4C). Furthermore, microscopic analysis using green fluorescent protein (GFP)-tagged AtBI-1 protein confirmed the perinuclear localization of AtBI-1 in ∆pmr1 and ∆spf1 cells as well as in WT cells (Figure 4D). We demonstrated previously that AtBI-GFP fusion protein has cell death suppressing activity similar to AtBI-1 (Kawai-Yamada 185 et al., 2001). Pmr1 is a Ca2+-ATPase with sequence similarity to animal SERCA (sarco/endoplasmic reticulum Ca2+-ATPase) and is located in the membranes of Golgi body (Antebi and Fink, 1992). It is suggested that Pmr1 is involved in the regulation of calcium concentration in ER (Strayle et al., 1999). On the other hand, Spf1 is a homologue of SERCA localized at ER. Both Ca2+-ATPases are believed to be involved in transmembrane movement 190 of ions, calcium and manganese (Rudolph et al., 1989; Cronin et al., 2002). Other mutants deficient in calcium transport in plasma membrane and vacuole did not influence the anti-apoptotic function of AtBI-1 (Figure 4A). 9 Downloaded from on June 18, 2017 - Published by www.plantphysiol.org Copyright © 2006 American Society of Plant Biologists. All rights reserved. Enhanced resistance of AtBI-1 overexpressing plants to CPA 195 Pmr1 and Spf1 are members of SERCA family and plant homologs have also been identified (Geisler et al., 2000). To understand the relationship between intracellular calcium homeostasis and BI-1 in plant cells, we evaluated the effect of cyclopiazonic acid (CPA), a specific inhibitor of SERCA, using transgenic Arabidopsis plants with AtBI-1 overexpression or knock-down (Figure 5A). RT-PCR analysis demonstrated that AtBI-1 was overexpressed in 200 OX lines (OX1 and OX2) and reduced in knock-down lines (KD1 and KD2) (Figure 5B). To evaluate the CPA sensitivity, each plant line was grown on the 0.5 x MS-medium with or without 5 µM CPA. Although these transgenic plants showed no obvious phenotype under general growing conditions, a slight growth retardation were observed in control and KD lines on CPA-containing medium (data not shown). To examine the effect of CPA on leaves, we 205 measured chlorophyll contents using 3-5th leaves of 3 week-old plants (Figure 5C). Although the chlorophyll contents measured in untreated plants were similar in all lines, KD and control lines (WT and GFP) demonstrated reduced chlorophyll contents on the CPA containing medium. In contrast, OX lines showed elevated chlorophyll contents with unknown mechanism, suggesting that overexpression of AtBI-1 overcame the effect of SERCA 210 inhibition by CPA. We also investigated the effects of thapsigargin (TG), which is also a well-known SERCA inhibitor in animals. However, no obvious phenotype was evident in TGtreated plants (20 µM) (data not shown). In fact, ECA1, an Arabidopsis homologue of SERCA, is CPA-sensitive but TG-insensitive (Liang and Sze, 1998). To gain more insight into the function of AtBI-1, we investigated ion stress sensitivities 215 of AtBI-1 transgenic plants. It is reported that Arabidopsis ECA1, an ER-localized SERCA-type Ca2+-pump, plays a role in both Ca2+ and Mn2+ homeostasis, and is required to support plant growth under conditions of Ca2+ deficiency or Mn2+ toxicity (Wu et al., 2002). To evaluate the ion stress sensitivity in plants with altered AtBI-1 expression, AtBI-1 transgenic 10 Downloaded from on June 18, 2017 - Published by www.plantphysiol.org Copyright © 2006 American Society of Plant Biologists. All rights reserved. plants were grown on Ca2+-deficient or Mn2+-rich (0.5 mM) plate. When plants were grown on 220 such plates for 3 weeks, KD lines showed severe growth defect and less chlorophyll contents (Figure 6). In contrast, OX plants had elevated chlorophyll contents and less growth retardation on both ion stress conditions, suggesting AtBI-1 affects ion homeostasis in plant cells. Measurement of [Ca2+]cyt in AtBI-1 overexpressing plant cells 225 Alterations in cytosolic Ca2+ ([Ca2+]cyt) have been implicated in apoptosis control mechanisms. The anti-apoptotic protein Bcl2 reduces Ca2+ efflux through the ER membrane (Lam et al., 1994). A rapid increase in [Ca2+]cyt is a common response to pathogen challenge in plant cells (Blume et al., 2000) and oxidative stress (Rentel and Knight 2004). We therefore explored the effects of BI-1 overexpression on Ca2+ homeostasis. To investigate the role of AtBI-1 on the 230 calcium flux in plant cells, transgenic tobacco BY-2 cells were examined using calcium-sensitive luminescent protein aequorin. In our previous work, BY-2 cells overexpressing AtBI-1 showed resistance to H2O2 or SA- induced cell death (Kawai-Yamada et al., 2004). The vectors, pBIG-AtBI-MBP (BI) and pBIG-MBP (VC) were introduced into tobacco BY-2 cells expressing proaequorin protein (Takahashi et al., 1997). The transformed 235 cells were treated with H2O2 or CPA, and their viability were measured. It is known that H2O2 and CPA induces rapid [Ca2+]cyt elevation and cell death (Berridge 1993; Akaishi et al., 2004). Although CPA- or H2O2- treatment caused massive cell death in the control BY-2 cell line (VC), AtBI-1 overexpressed line (BI) repressed such effect (Figure 7A). Using the same cell lines, we monitored [Ca2+]cyt after H2O2 or CPA treatment. As shown in Figure 7B and C, rapid 240 elevation in [Ca2+]cy appeared as a peak at 1-2 min after H2O2 or CPA treatment. The luminescence traces showed individual properties between CPA and H2O2 treatments. The duration and peak time were similar between cells expressing vector control and AtBI-1 (data not shown). Treatment of AtBI-1-expressing cells with H2O2 resulted in slight decrease of 11 Downloaded from on June 18, 2017 - Published by www.plantphysiol.org Copyright © 2006 American Society of Plant Biologists. All rights reserved. [Ca2+]cyt at peak point compared with the control cells. The CPA-released calcium 245 concentration in AtBI-1-overexpressing cells was reduced to 75 - 80% of the control at peak point. The resting value of [Ca2+]cyt before treatment was around 100 nM in all transformed strains (data not shown). Discussion 250 BI-1 interacts with calmodulin A rapid elevation in [Ca2+]cyt is a common response of organisms against various external stresses. Evidences from previous studies suggest that such Ca2+ fluxes trigger various cellular responses such as microtubule depolymerization, defense gene activation, and cell death 255 (Lecourieux et al., 2002). Using the yeast split-ubiquitin system, we demonstrated the interaction of AtBI-1 with calmodulin protein. Furthermore, mutants of AtBI-1 lacking function of cell death inhibition lost the ability to interact with calmodulin, suggesting that interaction with calmodulin is essential in yeast for suppressing cell death by AtBI-1. Furthermore, overlay assay indicated that C-terminal 14 amino acids of AtBI-1 interacted with 260 AtCaM7 protein. Our previous study demonstrated that the C-terminal 14 aa deleted mutant protein failed to inhibit plant cell death caused by H2O2 or salicylic acid (Kawai-Yamada et al., 2004), suggesting the C-terminal region is essential for the inhibition of cell death by AtBI-1. Recent studies have demonstrated close interactions between calmodulin and several enzymes involved in oxidative cell death responses. For instance, the calmodulin interacts with 265 and activates some plant catalases (Yang and Poovaiah 2002) and NAD kinase, which generates NAD(P)H for NAD(P)H oxidase (Turner et al, 2004). In addition, the barley Mlo protein, a plant-specific modulator of cellular defense and cell death, also binds to calmodulin and the interaction was related to the control of pathogen defense (Kim et al., 2002). In the 12 Downloaded from on June 18, 2017 - Published by www.plantphysiol.org Copyright © 2006 American Society of Plant Biologists. All rights reserved. present study, we showed that AtBI-1 also interacted with calmodulin, suggesting that 270 calmodulin may be one of key factors that regulate cell death or survival. The biochemical function of CaM-binding BI-1 remains to be elucidated. Anti-cell death function of AtBI-1 is associated with calcium flux Several investigators point to a direct role of calcium in controlling life and death of plant cells 275 as well as mammalian cells (Sanders et al., 2002). The present study indicated that AtBI-1 did not suppress Bax-induced cell death in yeast mutants lacking Pmr1 and Spf1. The two proteins are homologues of animal SERCA pumps localized at Golgi and ER, respectively (Antebi et al., 1992; Cronin et al., 2002), and are known to be involved in ER calcium homeostasis (Strayle et al., 1999; Vashist et al., 2002). The inability of AtBI-1 to suppress cell death in ∆pmr1 and 280 ∆spf1 suggests that an accurate calcium flux at Golgi or ER may be needed to the cell death inhibitory function of AtBI-1 in yeast. Mutants deficient in other calcium transporters located at the area, such as plasma membrane or vacuole, did not influence the anti-apoptotic function of AtBI-1, supporting the conclusion that the cell death suppression by AtBI-1 involves ER or Golgi calcium translocations. 285 To investigate the effect of AtBI-1 on calcium response to plant cell death stimuli, we measured changes in [Ca2+]cyt in response to H2O2 and CPA using proaequorin protein-expressing tobacco BY-2 cells. The finding that H2O2- treatment on tobacco plants induced a transient increase in [Ca2+]cyt was previously reported (Price et al., 1994). In the present study, a rise in [Ca2+]cyt was found at 1-2 min after H2O2 or CPA treatment, similar to 290 the result described by Price et al (1994). In contrast, Lecourieux et al (2002) showed biphasic elevation caused by cryptogein of Phytophthora cryptogea and H2O2 in Nicotiana plumbaginifolia cells. The [Ca2+]cyt elevation caused by various treatments might be different 13 Downloaded from on June 18, 2017 - Published by www.plantphysiol.org Copyright © 2006 American Society of Plant Biologists. All rights reserved. in the magnitude, duration and frequency, leading to diverse cellular responses such as adaptation to various stresses and cell death (Lecourieux et al., 2002). 295 Recently, Kadota et al (2005) demonstrated that the Ca2+ -permeable channel NtTPC1A/B located at plasma membrane plays a role in H2O2-induced rise in [Ca2+]cyt in tobacco BY-2 cells. Inhibition of SERCA by CPA treatment also leads to a rise in [Ca2+]cyt (Berridge 1993). Because of leak of Ca2+ through an unidentified channel, inhibition of Ca2+-pump by CPA induces an efflux of Ca2+ from the ER into the cytosol, producing an increase in cytosolic free 300 Ca2+ concentration (Zuppini et al., 2004; Sivaguru et al., 2005). In this study, CPA- and H2O2-induced calcium elevation was reduced by AtBI-1-overexpression in tobacco cells. This result is in agreement with those of previous studies demonstrating that human BI-1 overexpression led to decreased ER- releasable calcium concentration in human fibrosarcoma cells as well as Bcl-2 overexpression in various animal cells (Chae et al., 2004, 305 Foyouzi-Youssefi et al., 2000). As mentioned above, inhibition of SERCA pump causes the passive release of calcium from the ER and an increase in cytosolic calcium, which induces cell death (Zhou et al., 1998). However, overexpression of SERCA can also result in induction of cell death (Ma et al., 1999). These results indicate that accurate management of intracellular calcium homeostasis is necessary for cell living/death regulation. We found that Arabidopsis 310 plants with overexpression or knocked-down of AtBI-1 demonstrated altered CPA or ion stress tolerance, as reported in ECA1 transgenic plants (Wu et al., 2002), suggesting that AtBI-1 also plays a role in regulation of calcium homeostasis. Whether AtBI-1 acts solely in modulating ER-related [Ca2+]cyt flux or also regulates other steps remains to be determined. Ca2+-pumps are widely distributed on membranes, including the plasma membrane, 315 vacuole, Golgi, and ER. The role of Ca2+ in cellular signaling pathway is well recognized in mammalian cells, whereas the regulation of Ca2+ homeostasis in plant is still poorly understood. CPA and TG are well known inhibitors of the SERCA causing an increase in [Ca2+]cyt 14 Downloaded from on June 18, 2017 - Published by www.plantphysiol.org Copyright © 2006 American Society of Plant Biologists. All rights reserved. (Wuytack et al., 2003). In our experimental system, TG treatment did not cause effective Ca2+ efflux to the cytosol for unknown reason. The conflicts of such experimental results need to be 320 solved by isolation of target pumps. Sze et al (2000) classified plant Ca2+-pumps in two different classes based on similarity to animal proteins; type IIA, homologous to the SERCA class of Ca2+-ATPase located in ER, and type IIB, homologous to the plasma membrane (PM)-type Ca2+-ATPase (PMCA). Interestingly, Arabidopsis type IIA Ca2+-ATPase ECA1 can complement the yeast mutant defective in both 325 Golgi and vacuole Ca2+-pumps (pmr1 and pmc1, cnb1) (Liang et al., 1997; Sze et al., 2000). Furthermore, the ECA1 is inhibited by CPA but not by TG (Liang and Sze 1998). In contrast, the ACA2 of Arabidopsis encodes type IIB Ca2+-pump is unaffected by both CPA and TG (Hwang et al., 2000). A pump showing mixed characteristics of both ECA and ACA pumps was also identified in maize (Subbaiah and Sachs, 2000). 330 There is no experimental evidence for the regulation of plant type IIA Ca2+ pump activity. The most closely related ER-type calcium pump in animal, SERCA, is highly regulated by phosphorylation (East 2000). Since the plant type IIA pump is not directly regulated by calmodulin (Liang and Sze, 1998), AtBI-1 may act as the mediator between calmodulin signaling and Ca2+ pumps. Or, It is possible to speculate that the AtBI-1 may recruits/ or 335 remove calmodulin to/from the pump. Our data suggesting the involvement of Ca2+ -ATPases localized at ER or Golgi for BI-1 function in yeast system are in good agreement with this model. To elucidate the real function of AtBI-1 in plant cells, further analysis in AtBI-1/AtCaM bindings, calcium flux measurement and target pumps in Arabidopsis are needed. 340 It is demonstrated that the overexpression of BI-1 overcomes various stress-induced defects. For example, H2O2-, SA-, elicitor-, heat- and cold-induced cell death were suppressed in plant cells overexpressing AtBI-1 (Matsumura et al., 2003; Chae et al., 2003; 15 Downloaded from on June 18, 2017 - Published by www.plantphysiol.org Copyright © 2006 American Society of Plant Biologists. All rights reserved. Kawai-Yamada et al., 2004). The expression of plant BI-1 genes is rapidly up-regulated during wounding, pathogen attack (Sanchez et al., 2000) and senescence (Coupe et al., 2004), but 345 down-regulated by elicitor treatment (Matsumura et al., 2003). These results suggest the involvement of BI-1 in stress response and HR in plants. Furthermore, AtBI-1 overexpressing and knock-down plants grew normally under general growth conditions. This suggests that AtBI-1 is not essential for normal development and growth in Arabidopsis. Recently, two Arabidopsis mutants with a T-DNA insertion in the AtBI-1 gene (atbi1-11 and atbi1-2) were 350 characterized by Watanabe and Lam (2006). Both mutants also showed no obvious phenotype under general growth conditions. However, these mutants exhibited accelerated cell death upon exposure to fungal toxin fumonisin B1. The BI-1 deficient mice also showed normal growth, however increased susceptibility to ER-damage and oxidative stresses was reported (Chae et al., 2004). In conclusion, the BI-1 is presumably not required for physiological regulation of 355 developmental plant PCD. Rather, BI-1 possesses evolutionarily conserved functions that allow it to provide tolerance against stress-mediated cell death. Materials and methods Yeast split-ubiquitin two hybrid system 360 Protein interaction with AtBI-1 was analyzed using yeast split-ubiquitin system (Stagljar et al., 1998; Kim et al., 2002). Plasmid vector (HvCaM3) and yeast cells were kindly provided by Dr. Ralph Panstruga and Dr. IE Somssich (Max-Planck Institute). The C-terminal mutants of AtBI-1 were constructed using PCR, as described previously (Kawai-Yamada et al., 2004). The coding region of AtBI-1 and the C-terminal mutants (AtBI-29, 30, and 32) were cloned 365 into pMet-Cub-Ura3 vector to construct the bait plasmids. Yeast cells (JD53 strain) were transformed with different combinations of bait (AtBI-1 and the mutants) and prey constructs, and the His+Trp+Ura+ transformants were streaked on the minimum medium containing 16 Downloaded from on June 18, 2017 - Published by www.plantphysiol.org Copyright © 2006 American Society of Plant Biologists. All rights reserved. 5-fluoroorotic acid (5-FOA; 0.1%) and were incubated at 30°C for 4 days. Replacement of Ile-13 of wild type Nubi by alanine (NuA) decreases the affinity to Cubi (Stagljar et al., 1998; 370 Kim et al., 2002). The low Cub-affinity NuA prey variant served as a negative control. Plant materials The transgenic plants expressing AtBI-1 and GFP (Arabidopsis thaliana ecotype Col-0) were described previously in Kawai-Yamada et al (2001, 2004). To generate knock-down plants, 375 RNAi plasmid, pK7GWIWG2(II)-AtBI, was constructed. Briefly, the 3’-terminal fragment of AtBI-1 cDNA (+291/+744; translation initiation is +1) was introduced into the RNAi plasmid, pK7GWIWG2(II) (Karimi et al., 2002) by the Gateway system. The resulting plasmid was transferred to Agrobacterium tumefaciens strain EHA105 (Hood et al., 1993) using the freeze thaw method (An et al., 1998). Transformation of Arabidopsis plants was carried out by the 380 floral dip method (Bechtold and Pelletier 1998). Obtained plants were grown at 23°C under continuous light conditions (60 µmol/m2/s). Calmodulin overlay assay We used an overlay assay to examine the ability of C-terminal region of AtBI-1 to bind with 385 Arabidopsis calmodulin 7 (AtCaM7) protein in vitro. The AtCaM7 cDNA was inserted into pET32+ vector (Novagen, Madison, WI) to obtain His- and S-tagged AtCaM7 protein. The resultant vector pET32-AtCaM7 was transformed into Escherichia coli BL21 strain and, the recombinant His- and S-tagged CaM7 protein was purified according to the manufacture’s instruction (Invitrogen). 390 The 14-amino acid C-terminal of AtBI-1 was ligated into pMAL vector (NEB, Beverly, MA) to express MBP-tagged protein. The resultant vector was transformed into E. coli BL21 strain and MBP-tagged BI-C protein was purified according to the instructions provided by the 17 Downloaded from on June 18, 2017 - Published by www.plantphysiol.org Copyright © 2006 American Society of Plant Biologists. All rights reserved. manufacturer (NEB, Beverly, MA). The empty pMAL vector possessing in-frame β-galactosidase was used as a control (MAL-Gal). The purified BI-C and MAL-Gal proteins 395 were applied to SDS-PAGE, then blotted onto polyvinylidene difluoride (PVDF) membranes. The membranes were immunoblotted with anti-MBP antibody (NEB) or overlay assayed with recombinant AtCaM7 protein in the presence of 1 mM CaCl2 or 5 mM EGTA as described by Kim et al (2002). To detect CaM7 binding, HRP conjugated-S-protein (Novagen) and ECL kit (Amersham Biosciences, Little Chalfont, UK) were used because CaM7 protein was expressed 400 as S-tagged protein. BiFC analysis Plasmids for BiFC analysis were kindly provided from Dr. Klaus Harter (Univ. Köln, Germany) and Dr. Hironori Kaminaka (Univ. Tottori, Japan) (Walter et al., 2004). 405 PCR-amplified coding regions of AtBI-1 and AtCaM7 were introduced into the XbaI/BamHI site. The resultant plasmid, pSPYNE-AtBI-1 was fused with N-terminal (1-155 aa) region of YEP, and pSPYCE-AtCaM7 was fused with C-terminal (156-239 aa) part of YFP. BiFC was performed in 6-week-old Nicotiana benthamiana plants after Agrobacterium-mediated transient transformation according to Walter et al (2004). For analysis of BiFC signal, a 410 fluorescence microscope (DMRD; Leica, Germany) was applied. For the control experiment, pBin-AtBI-GFP (Kawai et al., 2001) was infiltrated to tobacco leaves and GFP fluorescence was examined. Yeast strain and cell death suppression assay 415 Saccharomyces cerevisiae disruption mutants were purchased from Euroscarf (Frankfurt, Germany). Plasmids used here were described previously (Kawai et al., 1999; Kawai-Yamada et al., 2001). Yeast disruption mutants and wild-type (BY4741) cells were transformed with 18 Downloaded from on June 18, 2017 - Published by www.plantphysiol.org Copyright © 2006 American Society of Plant Biologists. All rights reserved. galactose-inducible Yep51 vector harboring Bax (Yep51-Bax), and pYX112 vector harboring AtBI-1 (pYX112-AtBI-1). After culture of transformants in liquid medium containing 420 glucose for 1 day, the A600 of each culture was adjusted to 0.1 and serially diluted to 0.0001. Each dilution (5 µl) was spotted on SD medium containing glucose or galactose and was incubated at 30°C for 2 days (glucose) or 4 days (galactose). Cytological analysis 425 GFP-tagged AtBI-1 (pYX112-AtBI-GFP) was transformed into yeast cells (Kawai-Yamada et al., 2001). GFP fluorescence was examined with a fluorescence microscope (DMRD; Leica, Germany). For measurement of cell viability, tobacco BY-2 cells were treated with the indicated reagents for 16 hours and stained with 0.03% Evans blue. The numbers of stained (dead) and unstained (live) cells were counted under microscopy. 430 RT-PCR Arabidopsis and yeast total RNA was extracted using RNeasy Plant Mini Prep Kit (Qiagen, Hilden, Germany), and 0.2 µg was used as a template for RT-PCR with specific primers for AtBI-1 (5’- GGAATTCATGAGCATCCT TATCACTGCATT-3’ and 435 5’-GGTACCTCAGTTTCTCCT TTTCTTCTTC-3’) and Actin8 (5’TGAGCCAGATCTTCATCGTC -3’ and 5’- TCTCTTGCTCGTAGTCGACA -3’). The conditions for direct amplification with Ready-To-Go RT-PCR Beads (Amersham Pharmacia) were 1 cycle at 42°C for 20 min and at 95°C for 5 min; 28 cycle at 95°C for 30 sec, at 58°C for 30 sec, and at 72°C for 1 min. 440 19 Downloaded from on June 18, 2017 - Published by www.plantphysiol.org Copyright © 2006 American Society of Plant Biologists. All rights reserved. Ion stress assay Ion stress treatment was performed as described in Wu et al (2002). Briefly, surface sterilized seeds were germinated on 0.8% agar plate with 0.5 x Murashige and Skoog (MS) medium with 0.5 mM MnCl2 or calcium-free medium under constant illumination (60 µmol/m2/s). To 445 measure chlorophyll contents, leaves obtained from each seedling were homogenized with 80% acetone. The supernatant, collected after centrifugation, was examined at 663 and 645 nm, and the chlorophyll contents were calculated as described in Kawai-Yamada et al (2001). Cytosolic calcium concentration 450 Tobacco BY-2 (Nicotiana tabacum L. cv bright yellow 2) suspension-culture cells expressing proaequorin in the cytosol (Takahashi et al., 1997) were used for the measurement of [Ca2+]cyt. The coding sequence of maltose-binding protein (MBP) was amplified from pMAL vector by PCR and was cloned into pBIG vector containing the 35S promoter of Cauliflower mosaic virus and nopaline synthase terminator to generate pBIG-MBP. In order to express 455 AtBI-MBP in BY-2 cells, PCR-amplified fragments of AtBI-1 was cloned into pBIG-MBP. The resultant vectors, pBIG-AtBI-MBP and pBIG-MBP (control), were used for the Agrobacterium-mediated transformation of tobacco BY-2 cells expressing proaequorin protein (Takahashi et al., 1997). The [Ca2+]cyt was measured by a method as described previously (Takahashi et al., 460 1997: Kawano et al., 1998). The transformed BY-2 cells (3-day-old) were incubated with 1 µM coelenterazine in the culture medium in darkness for 8 hours to reconstitute the calcium-sensitive luminescent protein aequorin. The cells were washed with and re-suspended in fresh medium and used after 30 min of resting incubation. H2O2 or CPA was added to the cells and [Ca2+]cyt-dependent aequorin luminescence was monitored with a 465 CHEM-GLOW Photometer (American Instrument Co., MD) equipped with a pen recorder 20 Downloaded from on June 18, 2017 - Published by www.plantphysiol.org Copyright © 2006 American Society of Plant Biologists. All rights reserved. (Rikadenki Co., Tokyo, Japan), and expressed as relative peak height of aequorin luminescence. After each experiment, all remaining aequorin was discharged with 1 M CaCl2 and 10% ethanol, and the resultant luminescence was measured to estimate the amount of remaining aequorin. [Ca2+]cyt was calculated using the calibration equation: pCa = 470 0.332588(-logk) + 5.5593 where k represents luminescence counts per second divided by total counts (Knight et al, 1996). Acknowledgements Plasmids and strains used for split-ubiquitin system were generously provided by Dr. Ralph 475 Panstruga (Max-Planck Institute, Saarbruecken, Germany) and Dr. Imre E. Somssich (Max-Planck Institute). Plasmids used for the BiFC analysis were kindly provided by Dr. Klaus Harter (Univ. Köln, Germany) and Dr. Hironori Kaminaka (Univ. Tottori, Japan). Plasmids and strains used for cell death assay in yeast were kindly provided by Dr. John C. Reed (The Burnham Institute, La Jolla, CA). We thank Ms. Y. Takahashi for her technical 480 help. This work was supported by a Grant-in-Aid for Scientific Research on Priority Arias (Grant No. 17051006) from the Ministry of Education, Culture, Sports, Science and Technology of Japan, a grant from the Ministry of Agriculture, Forestry, and Fisheries of Japan, and from CREST, JST. 21 Downloaded from on June 18, 2017 - Published by www.plantphysiol.org Copyright © 2006 American Society of Plant Biologists. All rights reserved. Figure Legends 485 Figure 1. AtBI-1 interacts with calmodulin in yeast. (A) Bait and prey vector constructs used for yeast split-ubiquitin two hybrid system. Nubi and Cubi represent the N- and the C-terminus of ubiquitin protein, respectively (Stagljar et al., 1998; Kim et al., 2002). The full-length of AtBI-1 was used as a bait protein and the 490 C-terminal 14 amino acids were replaced in mutants (AtBI-29, 32, 30) as presented. Replaced amino acids are underlined. Amino acids with positive charge are indicated in red and those with negative charge in blue. Calculated scores for coiled-coil structure and abilities for cell death suppression are indicated (Kawai-Yamada et al., 2004). pCup: pCup promoter; HvCaM3: barley calmodulin 3; tCYC: CYC1 terminator; pMet: pMet promoter; URA3: 495 reporter protein. (B) Yeast split-ubiquitin system was used to analyze the interaction between AtBIs (AtBI-1, AtBI-29, 30 and 32) and HvCaM3. Yeast cells containing different combinations of bait (AtBI-1, AtBI-29, 30 and 32) and prey (NuI-HvCaM3) constructs were tested for their growth phenotype on the minimum medium containing 5-fluoroorotic acid (5-FOA). For the negative control, yeast cells possessing NuA-HvCaM3 and AtBI-1 (BI-1 + 500 NuA) were also plated. The results show the growth of each line after 2 days (without 5-FOA) and 6 days (with 5-FOA) incubation at 30°C. Figure 2. Overlay assay reveals that Arabidopsis calmodulin protein interacts with the C-terminal region of AtBI-1. 505 To detect the interaction between AtCaM7 and the C-terminal region of AtBI-1, an overlay assay was performed. The purified MBP tagged C-terminal 14 amino acid of AtBI-1 (BI-C) and β-galactosidase (gal) proteins were run by a gel electrophoresis, and blotted on a membrane as described in Materials and methods. CBB staining, western blotting with 22 Downloaded from on June 18, 2017 - Published by www.plantphysiol.org Copyright © 2006 American Society of Plant Biologists. All rights reserved. anti-MBP antibody were performed as control of protein loading. The overlay assay was 510 performed by a S-tagged AtCaM7 protein with 1 mM CaCl2 or 5 mM EGTA-containing solution. Figure 3. BiFC analysis of AtBI-1/AtCaM7 interaction in plant cells. (A) Schematic representation of BiFC plasmids. The coding region of AtBI-1 and AtCaM 515 genes were fused with N-terminal (YFP-N, 1-155 aa) and C-terminal (YFP-C, 156-239 aa) region of YFP, respectively. (B-E) BiFC visualization in Agrobacterium-infiltrated tobacco (Nicotiana benthamiana) leaves with pSPYNE-AtBI-1/pSPYCE (empty vector) (B and D) and pSPYNE-AtBI-1/pSPYCE-AtCaM7 (C and E). (F) Visualization of AtBI-GFP. Arrows indicate nuclei. Bars in B and C = 100 µm. Bars in D-F = 10 µm. 520 Figure 4. AtBI-1 does not suppress Bax-induced cell death in ∆pmr1 and ∆spf1. (A) Spot assay of cell death suppression activity of AtBI-1 in various yeast deletion mutants. Mutants used here are summarized in Table 1. Mutant cells transformed with plasmids containing Bax and AtBI-1 were spotted on SD medium containing glucose (Glu) or 525 galactose (Gal). The results show the growth of each line after 2-day (Glu) and 4-day (Gal) incubation at 30°C. BY4741 strain was wild-type used as a control. Red arrows indicate the lines that failed to suppress cell death even when AtBI-1 was expressed. (B) Cell death suppression activity of AtBI-1 in yeast mutants. Relative growth of yeast strains expressing AtBI-1 (Glu), or both AtBI-1 and Bax (Gal) was compared. The spots appeared in third 530 dilution (A600=0.001) of (A) were densitometricaly analyzed and expressed as relatives (Glu/Gal). Data shown are mean +S.E. of three experiments. (C) RT-PCR analysis of AtBI-1 expression in wild type (WT), ∆pmr1, and ∆spf1 yeast cells. Total RNA was prepared from cells cultured for 16h in SD-Glu medium. Ethidium bromide staining of rRNAs was served as 23 Downloaded from on June 18, 2017 - Published by www.plantphysiol.org Copyright © 2006 American Society of Plant Biologists. All rights reserved. a loading control. (D) Expression of GFP-tagged AtBI-1 protein in yeast cells. Fluorescence 535 of AtBI-GFP in wild-type cells, in ∆pmr1 cells and in ∆spf1 was observed with a fluorescence microscope. Figure 5. CPA resistance in Arabidopsis plants overexpressing AtBI-1. (A) Schematic diagrams of the vectors used for production of OX and KD transgenic lines. 540 P35S, cauliflower mosaic virus (CaMV) 35S promoter; LB, left -DNA border: RB, right T-DNA border; NosT, nopaline synthetase terminator; KanR, kanamycin resistance gene. (B) RT-PCR analysis of AtBI-1 expression in wild type (WT), overexpressing (OX), knock-down (KD) and GFP transgenic plants. Total RNA was prepared from 2 week-old seedlings. Actin8 (ACT8) was used as an internal control. Ethidium bromide staining of rRNA was served as a 545 loading control. (C) Chlorophyll contents in 3-5th leaves obtained from transgenic plants grown on 0.5 x MS-medium (Control) or 0.5 x MS-medium with CPA for 3 weeks. n=4-6. Data are mean + SE. Figure 6. Phenotypes of transgenic plants associated with ion stress conditions. 550 (A) Phenotypes of transgenic plants grown on 0.5x MS-medium with 0.5 mM MnCl2 (+Mn) or without Ca2+ (-Ca) for 3 weeks. (B) The third leaves obtained from transgenic plants gown on the 0.5x MS-medium with 0.5 mM MnCl2 or without Ca2+ for 3 weeks. (C) Chlorophyll contents in transgenic plants grown on the 0.5x MS-medium with 0.5 mM MnCl2 or without Ca2+ for 3 weeks. Data are mean + SE. n=4-6. KD, knock down; OX, overexpression. 555 Figure 7. Measurement of [Ca2+]cyt following H2O2 or CPA treatment in AtBI-1-overexpressing BY-2 cells. 24 Downloaded from on June 18, 2017 - Published by www.plantphysiol.org Copyright © 2006 American Society of Plant Biologists. All rights reserved. (A) Inhibition of H2O2 - or CPA- induced cell death by AtBI-1. Viability of BY-2 cells expressing empty vector (VC) or AtBI-MBP (BI) after 3 mM H2O2 treatment for 16 hours, or 560 after treatment with 1, 5 or 10 µM of CPA for 16 hours. Evans blue-negative (living) and -positive (dead) cells were counted under a microscope. Each bar represents the mean ± SE values of three independent experiments (n=10 - 18). (B) Typical aequorin luminescence traces of cells expressing AtBI-1 treated with 3 mM H2O2 or 10 µM CPA. Arrows indicate the time of CPA and H2O2 administration. AL, aequorin luminescence. (C) Measurement of a 565 peak [Ca2+]cyt after treatment with 3 mM H2O2 or 10 µM CPA. Each bar represents the mean ±SE values of three independent experiments. n=12-14. **, P < 0.01. *. P<0.05 25 Downloaded from on June 18, 2017 - Published by www.plantphysiol.org Copyright © 2006 American Society of Plant Biologists. All rights reserved. Table 1. Saccharomyces cerevisiae strains used in the present study. 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Downloaded from on June 18, 2017 - Published by www.plantphysiol.org Copyright © 2006 American Society of Plant Biologists. All rights reserved. Downloaded from on June 18, 2017 - Published by www.plantphysiol.org Copyright © 2006 American Society of Plant Biologists. All rights reserved. Downloaded from on June 18, 2017 - Published by www. Copyright © 2006 American Society of Plant Biologists. Al Downloaded from on June 18, 2017 - Published by www. Copyright © 2006 American Society of Plant Biologists. Al Downloaded from on June 18, 2017 - Published by www.plantphysiol.org Copyright © 2006 American Society of Plant Biologists. All rights reserved.
