Your search keyword '"Hiroki Osawa"' showing total 16 results

1. The rapid accumulation of aluminum is ubiquitous in both the evergreen and deciduous leaves of Theaceae and Ternstroemiaceae plants over a wide pH range in acidic soils

Author

Takeshi Tange, Shinsuke Ikeda, and Hiroki Osawa

Subjects

biology, fungi, food and beverages, Soil Science, Plant physiology, Plant Science, Evergreen, biology.organism_classification, Deciduous, Phylogenetics, Soil pH, Botany, Hyperaccumulator, Theaceae, Woody plant

Abstract

Background and aims Aluminum (Al) accumulator plants are occasionally found in certain genera or families of woody plant species that are broadly dispersed in the angiosperm phylogeny. However, spatial and seasonal patterns in Al accumulation within the closely related species of each group remain poorly understood.

Published

2012

2. A cell-type-specific defect in border cell formation in the Acacia mangium root cap developing an extraordinary sheath of sloughed-off cells

Author

Izuki Endo, Hiroki Osawa, and Takeshi Tange

Subjects

biology, Lateral root, Acacia, Cell Growth Process, Cell Growth Processes, Original Articles, Plant Science, biology.organism_classification, Cell Physiological Phenomena, Cell biology, Plant Root Cap, Acacia mangium, Border cells, Botany, Fluorescence microscope, Soybeans, Elongation, Root cap

Abstract

BACKGROUND AND AIMS: Root caps release border cells, which play central roles in microbe interaction and root protection against soil stresses. However, the number and connectivity of border cells differ widely among plant species. Better understanding of key border-cell phenotype across species will help define the total function of border cells and associated genes. METHODS: The spatio-temporal detachment of border cells in the leguminous tree Acacia mangium was investigated by using light and fluorescent microscopy with fluorescein diacetate, and their number and structural connectivity compared with that in soybean (Glycine max). KEY RESULTS: Border-like cells with a sheet structure peeled bilaterally from the lateral root cap of A. mangium. Hydroponic root elongation partially facilitated acropetal peeling of border-like cells, which accumulate as a sheath that covers the 0- to 4-mm tip within 1 week. Although root elongation under friction caused basipetal peeling, lateral root caps were minimally trimmed as compared with hydroponic roots. In the meantime, A. mangium columella caps simultaneously released single border cells with a number similar to those in soybean. CONCLUSIONS: These results suggest that cell type-specific inhibitory factors induce a distinct defective phenotype in single border-cell formation in A. mangium lateral root caps.

Published

2011

3. Transient Proliferation of Proanthocyanidin-Accumulating Cells on the Epidermal Apex Contributes to Highly Aluminum-Resistant Root Elongation in Camphor Tree

Author

Takeshi Tange, Hiroki Osawa, Yuki Matsushima, Izuki Endo, and Yukari Hara

Subjects

biology, Epidermis (botany), Cell division, Physiology, Cell, Lateral root, Plant physiology, Cinnamomum camphora, Plant Science, biology.organism_classification, Camphor, chemistry.chemical_compound, medicine.anatomical_structure, chemistry, Botany, Genetics, medicine, Biophysics, Elongation

Abstract

Aluminum (Al) is a harmful element that rapidly inhibits the elongation of plant roots in acidic soils. The release of organic anions explains Al resistance in annual crops, but the mechanisms that are responsible for superior Al resistance in some woody plants remain unclear. We examined cell properties at the surface layer of the root apex in the camphor tree (Cinnamomum camphora) to understand its high Al resistance mechanism. Exposure to 500 μm Al for 8 d, more than 20-fold higher concentration and longer duration than what soybean (Glycine max) can tolerate, only reduced root elongation in the camphor tree to 64% of the control despite the slight induction of citrate release. In addition, Al content in the root apices was maintained at low levels. Histochemical profiling revealed that proanthocyanidin (PA)-accumulating cells were present at the adjacent outer layer of epidermis cells at the root apex, having distinctive zones for cell division and the early phase of cell expansion. Then the PA cells were gradually detached off the root, leaving thin debris behind, and the root surface was replaced with the elongating epidermis cells at the 3- to 4-mm region behind the tip. Al did not affect the proliferation of PA cells or epidermis cells, except for the delay in the start of expansion and the accelerated detachment of the former. In soybean roots, the innermost lateral root cap cells were absent in both PA accumulation and active cell division and failed to protect the epidermal cell expansion at 25 μm Al. These results suggest that transient proliferation and detachment of PA cells may facilitate the expansion of epidermis cells away from Al during root elongation in camphor tree.

Published

2010

4. Effects of evening and nighttime leaf wetting on stomatal behavior of Cryptomeria japonica growing in dry soil

Author

Hiroki Osawa, Katsuhiko Yanaga, Masaya Masumori, and Takeshi Tange

Subjects

Evening, biology, Physiology, fungi, food and beverages, Cryptomeria, Plant physiology, Plant Science, biology.organism_classification, Photosynthesis, Japonica, Agronomy, Dry soil, Environmental science, Wetting, Transpiration

Abstract

To examine the hypothesis that stomatal behavior of plants in dry soil is influenced by a slow recovery from daytime water deficit, we studied the effect of repeated wetting of leaves during evening and night in Cryptomeria japonica seedlings grown in dry soil. After 7 and 10 days of leaf wetting treatment the midday leaf water potential decreased and the transpiration rate increased, respectively. Therefore, we suggest that rapid recovery from daytime water deficit could weaken the water conserving stomatal behavior that adapts to drought conditions in the roots.

Published

2009

5. Malate enhances recovery from aluminum-caused inhibition of root elongation in wheat

Author

Hiroki Osawa, Satoshi Kikui, Takayuki Sasaki, Yoko Yamamoto, and Hideaki Matsumoto

Subjects

Root growth, Plant growth, Al content, Soil Science, Plant physiology, chemistry.chemical_element, Plant Science, Biology, Calcium, chemistry, Aluminium, Botany, Chelation, Elongation

Abstract

Toxic aluminum (Al) ion is a major constraint to plant growth in acid soils. Aluminum tolerance in wheat (Triticum aestivum L.) is strongly related to the Al-triggered efflux of malate from root apices. A role of the secreted malate has been postulated to be in chelating Al and thus excluding it from root apices (malate hypothesis), but the actual process has yet to be fully elucidated. We measured Al content and root growth during and after Al exposure using seedlings of near-isogenic lines [ET8 (Al tolerant) and ES8 (Al sensitive)] differing in the capacity to induce Al-triggered malate efflux. Aluminum doses that caused 50% root growth inhibition during 24-h exposure to Al in calcium (Ca) solution (0.5 mM CaCl2, pH 4.5) were 50 µM in ET8 and 5 µM in ES8. Under such conditions, the amount of Al accumulated in root apices was approximately 2-fold higher in ET8 than ES8. Al-treated seedlings were then transferred to the Al-free Ca solution for 24 h. Compared to control roots (no Al pretreatment), root regrowth of Al-treated roots was about 100% in ET8 and about 25% in ES8. The impaired regrowth in ES8 was observed even after 24-h exposure to 2.5 µM Al which had caused only 20% root growth inhibition. The addition of malate (100 µM) during exposure to 50 µM Al in ES8 enhanced root growth 1.6 times and regrowth in Al-free solution 7 times, resulting in similar root growth and regrowth as in ET8. Short-term Al treatments of ES8 for up to 5 h indicated that the Al-caused inhibition of root regrowth started after 1-h exposure to Al. The stimulating effect of malate on root regrowth was observed when malate was present during Al exposure, but not when roots previously exposed to Al were rinsed with malate, although Al accumulation in root apices was similar under these malate treatments. We conclude that the malate secreted from root apices under Al exposure is essential for the apices to commence regrowth in Al-free medium, the trait that is not related to the exclusion of Al from the apices.

Published

2006

6. Citrate-release-mediated aluminum resistance is coupled to the inducible expression of mitochondrial citrate synthase gene in Paraserianthes falcataria

Author

Katsumi Kojima and Hiroki Osawa

Subjects

Physiology, Molecular Sequence Data, Drug Resistance, chemistry.chemical_element, Citrate (si)-Synthase, Plant Science, Cycloheximide, Calcium, Mitochondrial Proteins, chemistry.chemical_compound, Falcataria, Gene Expression Regulation, Plant, Gene expression, Citrate synthase, Amino Acid Sequence, Citrates, Protein Synthesis Inhibitors, Leucaena leucocephala, Sequence Homology, Amino Acid, biology, Fabaceae, Blotting, Northern, biology.organism_classification, Molecular biology, Isocitrate Dehydrogenase, De novo synthesis, chemistry, biology.protein, Elongation, Aluminum

Abstract

Aluminum (Al) resistance in some leguminous plants is achieved by enhanced citrate release from roots. Enhancement requires several hours for complete activation and is postulated to involve Al-responsive genes or components. We examined the mechanism of Al-induced citrate release by studying the relationship between citrate release and expression of the mitochondrial citrate synthase (mCS) gene in three leguminous trees. Root elongation in Leucaena leucocephala (Lam.) de Wit was arrested within 24 h by 30 microM Al, whereas root elongation in Paraserianthes falcataria (L.) Neilson and Acacia mangium Willd. was inhibited < 50% by a 48-h treatment with 100 microM Al in calcium chloride solution. Roots of P. falcataria and A. mangium maintained enhanced release and accumulation of citrate for at least 28 days in response to Al treatment. Aluminum increased the accumulation of mCS transcripts in P. falcataria roots, but not in L. leucocephala roots, and thus up-regulation decreased following removal of Al. Lanthanum did not alter the expression level of mCS. Aluminum increased mCS activity concomitantly with enhanced mCS gene expression in P. falcataria, whereas it did not affect mCS activity in L. leucocephala. Aluminum content in root apices of P. falcataria was increased by cycloheximide, supporting the idea that de novo synthesis of proteins is a prerequisite for Al resistance. Our findings suggest that Al-inducible expression of mCS coupled with enhanced citrate release mediates Al resistance in P. falcataria.

Published

2006

7. Aluminum-Induced Gene Expression and Protein Localization of a Cell Wall-Associated Receptor Kinase in Arabidopsis

Author

Bunichi Ezaki, Hiroki Osawa, Dieter Volkmann, Hideaki Matsumoto, Hongyun Tong, František Baluška, Mayandi Sivaguru, and Zheng-Hui He

Subjects

Physiology, Cell, Arabidopsis, Plant Science, Root hair, Plant Roots, Cell wall, Cell Wall, Gene Expression Regulation, Plant, Transcription (biology), Gene expression, Genetics, medicine, Wall-Associated Kinase, biology, Arabidopsis Proteins, Membrane Proteins, Plants, Genetically Modified, biology.organism_classification, Protein subcellular localization prediction, Cell biology, medicine.anatomical_structure, Biochemistry, Enzyme Induction, biology.protein, Protein Kinases, Aluminum, Research Article

Abstract

Here, we report the aluminum (Al)-induced organ-specific expression of a WAK1 (cell wall-associated receptor kinase 1) gene and cell type-specific localization of WAK proteins in Arabidopsis. WAK1-specific reverse transcriptase-polymerase chain reaction analysis revealed an Al-induced WAK1 gene expression in roots. Short- and long-term analysis of gene expression in root fractions showed a typical “on” and “off” pattern with a first peak at 3 h of Al exposure followed by a sharp decline at 6 h and a complete disappearance after 9 h of Al exposure, suggesting the WAK1 is a further representative of Al-induced early genes. In shoots, upon root Al exposure, an increased but stable WAK1 expression was observed. Using confocal microscopy, we visualized Al-induced closure of leaf stomata, consistent with previous suggestions that the Al stress primarily experienced in roots associated with the transfer of root-shoot signals. Elevated levels of WAK protein in root cells were observed through western blots after 6 h of Al exposure, indicating a lag time between the Al-induced WAK transcription and translation. WAK proteins are localized abundantly to peripheries of cortex cells within the elongation zone of the root apex. In these root cells, disintegration of cortical microtubules was observed after Al treatment but not after the Al analog lanthanum treatments. Tip-growing control root hairs, stem stomata, and leaf stomatal pores are characterized with high amounts of WAKs, suggesting WAKs are accumulating at plasma membrane domains, which suffer from mechanical stress and lack dense arrays of supporting cortical microtubules. Further, transgenic plants overexpressing WAK1 showed an enhanced Al tolerance in terms of root growth when compared with the wild-type plants, making the WAK1 one of the important candidates for plant defense against Al toxicity.

Published

2003

8. Aluminium triggers malate-independent potassium release via ion channels from the root apex in wheat

Author

Hideaki Matsumoto and Hiroki Osawa

Subjects

Potassium Channels, Intracellular pH, Potassium, Malates, chemistry.chemical_element, Plant Science, Biology, Plant Roots, chemistry.chemical_compound, Lanthanum, Genetics, medicine, Ytterbium, Cells, Cultured, Triticum, Tetraethylammonium, Niflumic acid, food and beverages, Biochemistry, chemistry, Biophysics, Liberation, Malic acid, Efflux, Copper, Intracellular, Aluminum, medicine.drug

Abstract

The regulatory mechanisms for the aluminium (Al)-induced efflux of K(+) and malate from the root apex of Al-resistant wheat ( Triticum aestivum L. cv. Atlas) were characterized. Treatment with 20 mM tetraethylammonium (TEA) chloride, a K(+)-channel inhibitor, blocked the Al-induced K(+) efflux by 65%, but blocked the Al-induced malate efflux only slightly. Lanthanum (La(3+)) or ytterbium (Yb(3+)) strongly inhibited the K(+) efflux, but slightly increased malate efflux. These lanthanides applied together with Al did not affect the Al-induced malate efflux, but reduced the Al-induced K(+) efflux by 57% for La(3+) and by 35% for Yb(3+). By contrast, pretreatment with 50 microM niflumic acid, an anion-channel inhibitor, strongly suppressed the Al-induced malate efflux, but did not affect the Al-induced K(+) efflux. The efflux of K(+) uncoupled with that of malate resulted in the alkalization of intracellular pH in the root apex, suggesting that the release of K(+) coupled with malate plays an important role in stabilizing intracellular pH. Copper (Cu(2+)) induced the release of K(+) via a TEA-insensitive pathway without the release of malate in both Al-resistant and Al-sensitive (cultivar Scout) wheat. Simultaneous application of Al and Cu(2+) to the root apices resulted in TEA-sensitive K(+) efflux in Atlas but not in Scout, suggesting that Al competes with Cu(2+) for K(+) efflux. Taken together, these results suggest that Al-induced K(+) efflux is mediated by both TEA- and lanthanide-sensitive K(+) channels, although this induction is not a prerequisite for the induction of the release of malate.

Published

2002

9. ScOPT1 and AtOPT4 function as proton-coupled oligopeptide transporters with broad but distinct substrate specificities

Author

Gary Stacey, Walter Gassmann, and Hiroki Osawa

Subjects

Saccharomyces cerevisiae Proteins, Monosaccharide Transport Proteins, Saccharomyces cerevisiae, Xenopus, Oligopeptide transport, Biochemistry, Substrate Specificity, Xenopus laevis, Animals, Molecular Biology, chemistry.chemical_classification, Oligopeptide, Tetrapeptide, biology, Symporters, Arabidopsis Proteins, Cell Biology, biology.organism_classification, Amino acid, chemistry, Gene Expression Regulation, Glutathione transport, Oocytes, Phytochelatin, Protons, Oligopeptides, Research Article

Abstract

A group of OPTs (oligopeptide transporters) exclusively identified in plants and fungi are proposed to transport oligopeptides and derivatives of three to six amino acids in length, but their transport mechanisms and biological functions are poorly understood. We expressed the Saccharomyces cerevisiae (yeast) OPT ScOPT1 and five Arabidopsis thaliana AtOPTs in Xenopus laevis oocytes for two-electrode voltage-clamp studies. ScOPT1 produced inward currents in response to GSH or GSSG, the phytochelatin (PC) PC2 and oligopeptides including the tetrapeptide GGFL, but not KLGL. Inward currents were dependent on the external proton and substrate concentrations, with high affinity for both. This and the inward currents evoked by substrates with net negative charges showed that ScOPT1 is a proton-coupled transporter. ScOPT1 displayed highest apparent affinity for PC2, with small differences in the maximal current among substrates. Glutathione transport by any of the tested AtOPTs, including AtOPT6, was not detected in yeast growth complementation assays. With AtOPT4, initially only small KLGL-dependent currents were recorded in batches of oocytes showing high ScOPT1 expression. AtOPT4 expression was optimized by swapping the 5′-untranslated region with that of ScOPT1. AtOPT4 displayed a higher affinity for KLGL than ScOPT1 did for any peptide. AtOPT4-mediated KLGL transport was detectable at pH 5.0, but not at pH 6.0 or 7.0. Taken together, our results demonstrate that ScOPT1 and AtOPT4 are proton-coupled OPTs with broad but distinct substrate specificities and affinities.

Published

2005

10. Cytotoxic thio-malate is transported by both an aluminum-responsive malate efflux pathway in wheat and the MAE1 malate permease in Schizosaccharomyces pombe

Author

Hiroki Osawa and Hideaki Matsumoto

Subjects

Saccharomyces cerevisiae, Organic Anion Transporters, Plant Science, Microbial Sensitivity Tests, Malate dehydrogenase, Plant Roots, Substrate Specificity, chemistry.chemical_compound, Schizosaccharomyces, Genetics, Malate transport, Ion transporter, Triticum, Thiomalates, biology, Cell Death, Genetic Complementation Test, food and beverages, Biological Transport, Hydrogen-Ion Concentration, biology.organism_classification, Yeast, Biochemistry, chemistry, Schizosaccharomyces pombe, Malic acid, Efflux, Schizosaccharomyces pombe Proteins, Aluminum

Abstract

Aluminum (Al) tolerance in wheat (Triticum aestivum L.) is mainly achieved by malate efflux, which is regulated by the expression of the recently identified gene, presumably encoding an Al-activated malate efflux transporter (ALMT1). However, the transport mechanism is not fully understood, partly as a result of the rapid turnover of its substrate. We developed a tool to study malate transport in wheat by screening biological compounds using the well-characterized Schizosaccharomyces pombe malate transporter (SpMAE1). Expression of SpMAE1 in both S. pombe and Saccharomyces cerevisiae, which has no SpMAE1 homologue, caused hypersensitivity to thio-malic acid. This hypersensitivity was prominent at pH 3.5, but not pH 4.5, and was accompanied by an increase in thiol content, indicating that SpMAE1 mediates the uptake of thio-malic acid at a specific low pH. In wheat, root apices were able to accumulate thio-malic acid without growth reduction at pH values above 4.2. Pretreatment of root apices with thio-malic acid followed by Al treatment induced thio-malate efflux. Al-induced thio-malate efflux was much higher in Al-resistant cultivars/genotypes than in Al-sensitive ones, and was accompanied by a decrease in thiol-content. Thio-malate efflux in the Al-resistant cultivar was slightly activated by lanthanum or ytterbium ion. Thio-malic acid did not alleviate the Al-induced inhibition of root elongation in wheat. Taken together, our results suggest that thio-malate acts as an analogue for malate in malate transport systems in wheat and yeast, and that it may be a useful tool for the analysis of malate transport involved in Al-tolerance and of other organic ion transport processes.

Published

2005

11. Expression analyses of Arabidopsis oligopeptide transporters during seed germination, vegetative growth and reproduction

Author

Minviluz G. Stacey, Walter Gassmann, Gary Stacey, Hiroki Osawa, and Ami Patel

Subjects

food.ingredient, Iron, Recombinant Fusion Proteins, Arabidopsis, Biological Transport, Active, Germination, Plant Science, Flowers, medicine.disease_cause, Hypocotyl, food, Genes, Reporter, Pollen, Botany, Genetics, medicine, Radicle, Arabidopsis thaliana, Ovule, Promoter Regions, Genetic, biology, Symporters, Arabidopsis Proteins, Reproduction, food and beverages, Membrane Transport Proteins, Sequence Analysis, DNA, biology.organism_classification, Plants, Genetically Modified, Seedlings, Seeds, Pollen tube, Oligopeptides, Cotyledon

Abstract

AtOPT promoter-GUS fusions were constructed for six of the nine known, putative oligopeptide transporters (OPTs) in Arabidopsis thaliana and used to examine AtOPT expression at various stages of plant development. AtOPT1, AtOPT3, AtOPT4, AtOPT6 and AtOPT7 were expressed in the embryonic cotyledons prior to root radicle emergence. Except for AtOPT8, which gave weak expression, all AtOPTs were strongly expressed in post-germinative seedlings with strongest expression in vascular tissues of cotyledons and hypocotyls. Preferential expression of AtOPTs in vascular tissues was also observed in cotyledons, leaves, hypocotyls, roots, flowers, siliques, and seed funiculi of seedlings and adult plants. Differential tissue-specific expression was observed for specific AtOPTs. For example, AtOPT1, AtOPT3 and AtOPT8 were uniquely expressed in pollen. Only AtOPT1 was expressed in growing pollen tubes, while only AtOPT6 was observed in ovules. AtOPT8 was transiently expressed in seeds during early stages of embryogenesis. Iron limitation was found to enhance expression of AtOPT3. These data suggest distinct cellular roles for specific AtOPTs including nitrogen mobilization during germination and senescence, pollen tube growth, pollen and ovule development, seed formation and metal transport.

Published

2005

12. Evidence for the plasma membrane localization of Al-activated malate transporter (ALMT1)

Author

Hiroki Osawa, Mineo Yamaguchi, Hideaki Matsumoto, Sung Ju Ahn, Yoko Yamamoto, Mayandi Sivaguru, and Takayuki Sasaki

Subjects

Physiology, Direct evidence, Arabidopsis Proteins, Recombinant Fusion Proteins, Cell Membrane, Green Fluorescent Proteins, Drug Resistance, food and beverages, Organic Anion Transporters, Transporter, Cell Biology, Plant Science, General Medicine, Genetically modified crops, Biology, Green fluorescent protein, Membrane, Biochemistry, Gene Expression Regulation, Plant, Onions, Tobacco, Heterologous expression, Membrane fraction, Triticum, Aluminum

Abstract

Aluminum (Al)-activated malate transporter (ALMT1) was recently identified from wheat (Triticum aestivum). Heterologous expression of ALMT1 led to higher malate exudation that is associated with enhanced Al tolerance in transgenic plants. Here, we show the first direct evidence that ALMT1 is localized in the plasma membrane of Al-tolerant wheat. Phase partitioning experiments showed that this transporter was associated with the plasma membrane fraction. ALMT1 was detected in an Al-tolerant wheat line even without Al treatments. Analysis of transient expression of ALMT1::green fluorescent protein (GFP) in onion and tobacco cells further confirmed this ALMT1 localization.

Published

2005

13. Effect of K-252a and abscisic acid on the efflux of citrate from soybean roots

Author

Hiroki Osawa, Ayalew Ligaba, Mineo Yamaguchi, Hong Shen, Koichi Shibata, Xiaolong Yan, and Hideaki Matsumoto

Subjects

Physiology, Carbazoles, Plant Science, Plant Roots, Indole Alkaloids, chemistry.chemical_compound, Citrate synthase, Citrates, Enzyme Inhibitors, Protein kinase A, Abscisic acid, Protein Kinase Inhibitors, chemistry.chemical_classification, biology, Kinase, fungi, food and beverages, Kinetics, Enzyme, chemistry, Biochemistry, Verapamil, Glycine, biology.protein, Efflux, Soybeans, Organic acid, Abscisic Acid, Aluminum

Abstract

The Al-induced release of organic acid has been suggested as an important mechanism for Al resistance in plants. In this study, the effect of K-252a and abscisic acid (ABA) on the efflux of citrate was investigated in soybean (Glycine max L.) roots. Al initiated citrate efflux from the root apices 30 min after the addition of Al. The Al-triggered efflux of citrate was sensitive to metabolic inhibitors and anion channel inhibitors. Pretreatment or treatment with K-252a, an inhibitor of protein kinase, severely inhibited the Al-induced efflux of citrate accompanying an increase in Al accumulation and intensified Al-induced root growth inhibition. Al-treatment increased the endogenous level of abscisic acid (ABA) in soybean roots in a dose- and time-dependent manner, while K-252a failed to inhibit the Al-induced increase in endogenous ABA. Exogenous application of ABA increased the activity of citrate synthase (EC 4.1.3.7) by 26.2%, and decreased Al accumulation by 32.3%, respectively. ABA-induced increases in citrate efflux and root elongation were suppressed by K-252a, while ABA could not reverse the K-252a effects. Taken together, these results suggest that ABA is probably involved in the early response, after which K-252a-sensitive protein kinases play a key step in regulating the activity of an anion channel, through which citrate is released from the apical cells of soybean roots.

Published

2004

14. Aluminum inhibits the H(+)-ATPase activity by permanently altering the plasma membrane surface potentials in squash roots

Author

Hiroki Osawa, Hideaki Matsumoto, Gap Chae Chung, Mayandi Sivaguru, and Sung Ju Ahn

Subjects

Physiology, ATPase, Plant Science, In Vitro Techniques, Models, Biological, Plant Roots, Membrane Potentials, Plant Epidermis, Cucurbita pepo, Genetics, medicine, Enzyme Inhibitors, Membrane potential, biology, Chemistry, Vesicle, Cell Membrane, Depolarization, biology.organism_classification, Adaptation, Physiological, Immunohistochemistry, Cucurbitaceae, Proton-Translocating ATPases, Mechanism of action, Biochemistry, Cytoplasm, Biophysics, biology.protein, medicine.symptom, Elongation, Aluminum, Research Article

Abstract

Although aluminum (AL) toxicity has been widely studied in monocotyledonous crop plants, the mechanism of Al impact on economically important dicotyledonous plants is poorly understood. Here, we report the spatial pattern of Al-induced root growth inhibition, which is closely associated with inhibition of H+-ATPase activity coupled with decreased surface negativity of plasma membrane (PM) vesicles isolated from apical 5-mm root segments of squash (Cucurbita pepo L. cv Tetsukabuto) plants. High-sensitivity growth measurements indicated that the central elongation zone, located 2 to 4 mm from the tip, was preferentially inhibited where high Al accumulation was found. The highest positive shifts (depolarization) in zeta potential of the isolated PM vesicles from 0- to 5-mm regions of Al-treated roots were corresponded to pronounced inhibition of H+-ATPase activity. The depolarization of PM vesicles isolated from Al-treated roots in response to added Al in vitro was less than that of control roots, suggesting, particularly in the first 5-mm root apex, a tight Al binding to PM target sites or irreversible alteration of PM properties upon Al treatment to intact plants. In line with these data, immunolocalization of H+-ATPase revealed decreases in tissue-specific H+-ATPase in the epidermal and cortex cells (2–3 mm from tip) following Al treatments. Our report provides the first circumstantial evidence for a zone-specific depolarization of PM surface potential coupled with inhibition of H+-ATPase activity. These effects may indicate a direct Al interaction with H+-ATPase from the cytoplasmic side of the PM.

Published

2001

15. Possible involvement of protein phosphorylation in aluminum-responsive malate efflux from wheat root apex

Author

Hideaki Matsumoto and Hiroki Osawa

Subjects

Anions, Physiology, Malates, Plant Science, Plant Roots, Ion Channels, chemistry.chemical_compound, Genetics, Protein phosphorylation, Enzyme Inhibitors, Phosphorylation, Protein kinase A, Protein Kinase Inhibitors, Triticum, Plant Proteins, biology, Kinase, food and beverages, Biological Transport, Phosphate, Enzyme Activation, Biochemistry, chemistry, biology.protein, Efflux, Malic acid, Protein Kinases, Organic anion, Aluminum, Research Article

Abstract

In many plants, efflux of organic anions from roots has been proposed as one of the major Al resistance mechanisms. However it remains unknown how plants regulate efflux of organic anions in response to Al. In this study, the regulatory mechanisms of Al-responsive malate efflux in wheat (Triticum aestivum) were characterized focusing on the role of protein phosphorylation. Al-resistant wheat (cv Atlas) initiated malate efflux at 5 min after addition of Al, and this response was sensitive to temperature. K-252a, a broad range inhibitor of protein kinases, effectively blocked the Al-induced malate efflux accompanied with an increased accumulation of Al and intensified Al-induced root growth inhibition. A transient activation of a 48-kD protein kinase and an irreversible repression of a 42-kD protein kinase were observed preceding the initiation of malate efflux, and these changes were canceled by K-252a. Malate efflux was accompanied with a rapid decrease in the contents of organic anions in the root apex, such as citrate, succinate, and malate but with no change in the contents of inorganic anions such as chloride, nitrate, and phosphate. These results suggest that protein phosphorylation is involved in the Al-responsive malate efflux in the wheat root apex and that the organic anion-specific channel might be a terminal target that responds to Al signaling mediated by phosphorylation.

Published

2001

16. Aluminum-induced 1--3-beta-D-glucan inhibits cell-to-cell trafficking of molecules through plasmodesmata. A new mechanism of aluminum toxicity in plants

Author

Tomoko Mori, Hideaki Matsumoto, Takanori Maeda, J. Šamaj, Toru Fujiwara, Dieter Volkmann, Mayandi Sivaguru, Zhenming Yang, František Baluška, and Hiroki Osawa

Subjects

Intracellular Fluid, Cell signaling, Physiology, Nicotiana tabacum, Fluorescent Antibody Technique, Plant Science, Plasmodesma, Cell Communication, Myosins, Plant Roots, chemistry.chemical_compound, Tobacco, Genetics, Extracellular, Calcium Signaling, Microscopy, Immunoelectron, Glucans, Triticum, Lucifer yellow, biology, Intercellular transport, Callose, Calcium-Binding Proteins, Biological Transport, biology.organism_classification, Plant cell, Plants, Toxic, Biochemistry, chemistry, Ribonucleoproteins, Biophysics, Calreticulin, Aluminum, Subcellular Fractions, Research Article

Abstract

Symplastic intercellular transport in plants is achieved by plasmodesmata (PD). These cytoplasmic channels are well known to interconnect plant cells to facilitate intercellular movement of water, nutrients, and signaling molecules including hormones. However, it is not known whether Al may affect this cell-to-cell transport process, which is a critical feature for roots as organs of nutrient/water uptake. We have microinjected the dye lucifer yellow carbohydrazide into peripheral root cells of an Al-sensitive wheat (Triticum aestivum cv Scout 66) either before or after Al treatment and followed the cell-to-cell dye-coupling through PD. Here we show that the Al-induced root growth inhibition is closely associated with the Al-induced blockage of cell-to-cell dye coupling. Immunofluorescence combined with immuno-electron microscopic techniques using monoclonal antibodies against 1→3-β-d-glucan (callose) revealed circumstantial evidence that Al-induced callose deposition at PD may responsible for this blockage of symplastic transport. Use of 2-deoxy-d-glucose, a callose synthesis inhibitor, allowed us to demonstrate that a reduction in callose particles correlated well with the improved dye-coupling and reduced root growth inhibition. While assessing the tissue specificity of this Al effect, comparable responses were obtained from the dye-coupling pattern in tobacco (Nicotiana tabacum) mesophyll cells. Analyses of the Al-induced expression of PD-associated proteins, such as calreticulin and unconventional myosin VIII, showed enhanced fluorescence and co-localizations with callose deposits. These results suggest that Al-signal mediated localized alterations to calcium homeostasis may drive callose formation and PD closure. Our data demonstrate that extracellular Al-induced callose deposition at PD could effectively block symplastic transport and communication in higher plants.

Published

2000