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Four new tetromycin derivatives, tetromycins 1-4 and a previously known one, tetromycin B (5) were isolated from Streptomyces axinellae Pol001(T) cultivated from the Mediterranean sponge Axinella polypoides. Structures were assigned using extensive 1D and 2D NMR spectroscopy as well as HRESIMS analysis. The compounds were tested for antiparasitic activities against Leishmania major and Trypanosoma brucei, and for protease inhibition against several cysteine proteases such as falcipain, rhodesain, cathepsin L, cathepsin B, and viral proteases SARS-CoV M(pro), and PL(pro). The compounds showed antiparasitic activities against T. brucei and time-dependent inhibition of cathepsin L-like proteases with K(i) values in the low micromolar range.
Four new tetromycin derivatives, tetromycins 1–4 and a previously known one, tetromycin B (5) were isolated from Streptomyces axinellae Pol001T cultivated from the Mediterranean sponge Axinella polypoides. Structures were assigned using extensive 1D and 2D NMR spectroscopy as well as HRESIMS analysis. The compounds were tested for antiparasitic activities against Leishmania major and Trypanosoma brucei, and for protease inhibition against several cysteine proteases such as falcipain, rhodesain, cathepsin L, cathepsin B, and viral proteases SARS-CoV Mpro, and PLpro. The compounds showed antiparasitic activities against T. brucei and time-dependent inhibition of cathepsin L-like proteases with Ki values in the low micromolar range.
During the last few years an increasing number of physiological processes in plants have been shown to be regulated by NO. NO plays important roles in growth and development, plant disease resistance, abiotic stress, and in above and underground plant organs. In recent years several enzymatic pathways and few non-enzymatic pathways were proposed for nitric oxide production in plants. The major goal of this work was to quantify NO production by plants and especially by roots, and to identify the enzymes responsible for NO production. As a major method, NO production by roots was followed through on-line measurement of NO emission into the gas phase by chemiluminescence (= direct chemiluminescence), and also by indirect chemiluminescence where trace amounts of oxidized products like NO2- and NO3- can be easily measured. Plants used were tobacco wild-type (N. tabacum cv Xanthi or cv Gatersleben), NR-free mutants grown on ammonium in order to prevent NR induction, plants grown on tungstate to inhibit synthesis of functional MoCo-enzymes, and a NO-overproducing nitrite reductase (NiR)-deficient transformant as well as barley, rice and pea. Induction of a hypersensitive response (HR) in tobacco leaves was achieved by using avirulent Pseudomonas syringae pv phaseolicola. At oxygen concentrations of <1%, even completely nitrate reductase (NR)-free root tissues reduced added nitrite to NO, indicating that in roots, NR was not the only source for nitrite-dependent NO formation. By contrast, NR-free leaf slices were not able to reduce nitrite to NO. Root NO formation was blocked by inhibitors of mitochondrial electron transport (Myxothiazol and SHAM), whereas NO formation by NR containing leaf slices was insensitive to the inhibitors. Consistent with that, mitochondria purified from roots, but not those from leaves, reduced nitrite to NO at the expense of NADH. The inhibitor studies suggest that, in root mitochondria, both terminal oxidases participate in NO formation, and they also suggest that even in NR-containing roots, a large part of the reduction of nitrite to NO was catalysed by mitochondria, and less by NR. The differential capacity of root and leaf mitochondria to reduce nitrite to NO appears to be common among higher plants, since it was observed with Arabidopsis, barley, pea, and tobacco. Nitrite and NADH consumption by mitochondria were also measured. Anaerobic, nitrite-dependent NO emission was exclusively associated with the membrane fraction, without participation of matrix components. It was also examined whether root mitochondria and mitochondrial membranes produce nitric oxide (NO) exclusively by reduction of nitrite or also via a nitric oxide synthase (NOS),- and to what extent direct NO measurements could be falsified by NO oxidation. In addition to chemiluminescence, Diaminofluoresceins (DAF) were used as an NO indicators for comparison. In air, mitochondria apparently produced no nitrite-dependent NO, and no NOS activity was detected by direct or indirect chemiluminescence. In contrast, with DAF-2 and DAR-4M an L-arginine-dependent fluorescence increase took place. However, the response of this apparent NOS activity to inhibitors, substrates and cofactors was untypical when compared with commercial iNOS and is considered an artefact. With iNOS, about 2/3 of the NO were oxidized to (nitrite + nitrate). Mitochondria also appear to consume NO without increasing oxidation to (nitrite+ nitrate). We therefore assume formation of NO to a volatile intermediate (eventually N2O3). It was recently shown that the hypersensitive response (HR) of tobacco triggered by the fungal elicitor cryptogein occurred independent of the presence or absence of nitrate reductase (NR). One conclusion was that NR-dependent NO formation played no role in the HR. Here we present evidence that the described scenario may be specific for cryptogein. Pseudomonas syringae pv. phaseolicola was infiltrated into tobacco leaves from WT plant and from the NiR-deficient NO-overproducing clone 271, grown either on nitrate or ammonium. Lesion development as well as bacterial growth and sugar concentrations in leaves and in the leaf apoplast was monitored. Lesion development was positively and bacterial growth was negatively correlated with nitrate nutrition and eventually with NO formation. Bacterial growth was positively correlated with ammonium nutrition and apoplastic sugar concentrations. Total (free and conjugated) SA content were always drastically increased by bacterial infection, but there was no clear correlation with NO production. In the presence of cryptogein, Pseudomonas growth was drastically reduced. This shows that the assumed interdependence of bacterial growth, NO production and the HR is complex and not unifactorial.
Nitric oxide production by tobacco plants and cell cultures under normal conditions and under stress
(2004)
Nitric oxide (NO) is a gaseous free radical involved in the regulation of diverse biochemical and physiological processes in animals. During the last decade, evidence has accumulated that NO might also play an important role as a second messenger in plants. Of special interest were observations that NO was involved in a signal chain leading to the hypersensitive response (HR) in incompatible plant-pathogen interactions. In contrast to animals, plants have probably several enzymes that may produce NO. Potential candidates are: Cytosolic nitrate reductase (NR; EC 1.6.6.1), plasma-membrane (PM)-nitrite: NO reductase (Ni:NOR), nitric oxide synthase (NOS; EC 1.14.13.39) and Xanthine dehydrogenase (XDH; EC 1.1.1.204). The major goal of this work was to quantify NO production by plants, and to identify the enzymes responsible for NO production. As a major method, NO production by tobacco leaves or cell suspensions was followed under normal, non-stress conditions, and under biotic stress, through on-line measurement of NO emission into the gas phase (chemiluminescence). Plants used were tobacco wild-type (N. tabacum cv Xanthi or cv Gatersleben), NR-free mutants grown on ammonium in order to prevent NR induction, plants grown on tungstate to inhibit synthesis of functional MoCoenzymes, and a NO-overproducing nitrite reductase (NiR)-deficient transformant. Induction of HR in tobacco leaves and in cell suspensions was achieved using the fungal peptide elicitor cryptogein. Non-elicited leaves from nitrate-grown plants showed a typical NO-emission pattern where NO-emission was low in dark, higher in the light and very high under dark-anaerobic conditions. Even at maximum rates, NO production in vivo was only a few percent of total NR activity (NRA). Consistent with that, with a solution of purified NR as a simple, “low quenching” system, NO-emission was also about 1 % of NRA. Thus, NO scavenging by leaves and stirred cell suspensions appeared small and NO-emission into purified air should give a reliable estimate of NO production. NO-emission was always high in a NiR-deficient transformant which accumulated nitrite, and NO-emission was completely absent in plants or cell suspensions which did not contain NR. Thus, in healthy plants or cell suspensions, NO-emission was exclusively due to the reduction of nitrite to NO, mainly by cytosolic NR. In addition to nitrite, cytosolic NADH appears as an important factor limiting NO production. Unexpectedly, plants (in absence of NR) were able to reduce nitrite to NO under anaerobic conditions through an unknown enzyme system that was not a MoCo-enzyme and was cyanide-sensitive. When infiltrated into leaves at nanomolar concentrations, the fungal elicitor cryptogein provoked cell death in tobacco leaves and cell suspensions. The HR could be prevented by the NO-scavengers PTIO or c-PTIO, suggesting that NO production was indeed required for the HR. However, the product of the reaction of c-PTIO with NO, c-PTI, also prevented cell death without quenching NO emission. Thus, prevention of cell death by c- PTIO is no proof for an involvement of NO. No differences were found in the HR induction between NR-free plants and/or cell suspensions and WT plants. Thus, NR appears not necessary for the HR. Further, and in contrast to literature suggestions, a continuously high NO-overproduction by a NiR-free mutant did not interfere with the development of the HR. Most surprisingly, no additional NO-emission from tobacco leaves was induced by cryptogein at any phase of the HR. In contrast, some NO-emission, paralleled by nitrite accumulation, was detected 3-6 h after cryptogein addition with nitrate grown cell suspensions, but not with NR free, ammonium- grown cells. Thus, induction of NO-emission by cryptogein appeared somehow correlated with NR and nitrite, at least in cell suspensions. But since cryptogein induced the HR even in NR-free cell suspensions, this nitrite-related NO- emission was not required for cell death. NOS inhibitors neither prevented cell death nor did they affect nitrite-dependent NO-emission. Thus, in total these data question the often proposed role of NO as a signal in the HR, and of NOS as source for NO.
Plant–pathogen interactions have been widely studied, but mostly from the site of the plant secondary defense. Less is known about the effects of pathogen infection on plant primary metabolism. The possibility to transform a fluorescing protein into prokaryotes is a promising phenotyping tool to follow a bacterial infection in plants in a noninvasive manner. In the present study, virulent and avirulent Pseudomonas syringae strains were transformed with green fluorescent protein (GFP) to follow the spread of bacteria in vivo by imaging Pulse-Amplitude-Modulation (PAM) fluorescence and conventional binocular microscopy. The combination of various wavelengths and filters allowed simultaneous detection of GFP-transformed bacteria, PAM chlorophyll fluorescence, and phenolic fluorescence from pathogen-infected plant leaves. The results show that fluorescence imaging allows spatiotemporal monitoring of pathogen spread as well as phenolic and chlorophyll fluorescence in situ, thus providing a novel means to study complex plant–pathogen interactions and relate the responses of primary and secondary metabolism to pathogen spread and multiplication. The study establishes a deeper understanding of imaging data and their implementation into disease screening.
Normoxic and anoxic metabolism of Nicotiana tabacum transformants lacking root nitrate reductase
(2002)
The aim of this work was to find out whether and how nitrate reduction in roots would facilitate survival of hypoxic and anoxic (flooding)-phases. For that purpose, we compared the response of roots of hydroponically grown tobacco wildtype (Nicotiana tabacum cv. Gatersleben) and of a transformant (LNR-H) with no nitrate reductase (NR) in the roots but almost normal NR in leaves (based on a nia2-double mutant). As an additional control we used occasionally a 35S-transformant of the same nia2-double mutant, which on the same genetic background constitutively expressed NR in all organs. In some cases, we also compared the response of roots from WT plants, which had been grown on tungstate for some time in order to completely suppress NR activity. The following root parameters were examined: 1) Growth and morphology 2) Root respiration rates and leaf transpiration 3) Metabolite contents in roots (ATP, hexosemonophosphates, free sugars, starch, amino acids, total protein) 4) Inorganic cation and anion contents 5) Lactate and ethanol production 6) Extractable LDH-and ADH-activities 7) Cytosolic pH values (by 31P-NMR) 8) NO Cation and anion contents of roots from WT and LNR-H were only slightly different, confirming that these plants would be better suited for our purposes than the widely used comparison of nitrate-versus ammonium-grown plants, which usually show up with dramatic differences in their ion contents. Normoxia: LNR-H-plants had shorter and thicker roots than WT with a lower roots surface area per leaf FW. This was probably the major cause for the significantly lower specific leaf transpiration of LNR-H. WT-roots had lower respiration rates, lower ATP-and HMP-contents, slightly lower sugar- and starch contents and somewhat lower amino acid contents than LNR-H roots. However, total protein/FW was almost identical. Obviously the LNR-H transformants did not suffer from N-defciency, and their energy status appeared even better than that of WT-roots. Data from the 35S-transformant were similar to those of WT. This indicates that the observed differences between WT and LNR-H were not due to unknown factors of the genetic nia2-background, but that they could be really traced back to the presence resp. absence of nitrate reduction. Anoxia: Under short-term anoxia (2h) LNR-H plants, but not WT-plants exhibited clear symptoms of wilting, although leaf transpiration was lower with LNR-H. Reasons are not known yet. LNR-H roots produced much more ethanol (which was excreted) and lactate compared to WT, but extractable ADH and LDH activities, were not induced by anoxia. However, the LDH activity background was twice as high as that of the WT troughout the time period studied. Tungstate-treated WT-roots also gave higher fermentation rates than normal WT roots. Sugar- and HMP-contents remained higher in LNR-H roots than in WT. NR in WT roots was activated under anoxia and roots accumulated nitrite, which was also released to the medium. 31P-NMR spectroscopy showed that LNR-H- roots, in spite of their better energy status, acidified their cytosol more than WT roots. Conclusions: Obviously nitrate reduction affects - by as yet unknown mechanisms - root growth and morphology. The much lower anoxic fermentation rates of WT-roots compared to LNR-H roots could not be traced back to an alternative NADH consumption by nitrate reduction, since NR activity was too low for that. An overall estimation of H+-production by glycolysis, fermentation and nitrate reduction (without nitrite reduction, which was absent under anoxia) indicated that the stronger cytosolic acidification of anoxic LNR-H roots was based on their higher fermentation rates. Thus, nitrate reduction under anoxia appears advantageous because of lower fermentation rates and concomitantly lower cytosolic acidification. However, it remained unclear why fermentation rates were so different. Perspective: Preliminary experiments had indicated that WT-roots produced more nitric oxide (NO) under anoxia than LNR-H-roots. Accordingly, we suggest that nitrate reduction, beyond a merely increased NADH-consumption, would lead to advantageous changes in metabolism, eventually via NO-production, which is increasingly recognized as an important signaling compound regulating many plant functions.
Marine sponges (Porifera) harbor diverse microbial communities within their mesohyl, among them representatives of the phylum Actinobacteria, commonly known as actinomycetes. Actinomycetes are prolific producers of pharmacologically important compounds and are responsible for producing the majority of antibiotics. The main aim of this Ph.D. study was to investigate the metabolic potential of the sponge-associated actinomycetes to produce novel anti-infective agents. The first aim was to cultivate actinomycetes derived from different marine sponges. 16S rDNA sequencing revealed that the strains belonged to diverse actinomycete genera such as Gordonia, Isoptericola, Micromonospora, Nocardiopsis, Saccharopolyspora and Streptomyces. Phylogenetic analyses and polyphasic characterization further revealed that two of these strains represent new species, namely Saccharopolyspora cebuensis strain SPE 10-1T (Pimentel-Elardo et al. 2008a) and Streptomyces axinellae strain Pol001T (Pimentel-Elardo et al. 2008b). Furthermore, secondary metabolite production of the actinomycete strains was investigated. The metabolites were isolated using a bioassay-guided purification scheme followed by structure elucidation using spectroscopic methods and subjected to an elaborate anti-infective screening panel. Several interesting compounds were isolated namely, the novel polyketides cebulactam A1 and A2 (Pimentel-Elardo et al. 2008c), a family of tetromycin compounds including novel derivatives, cyclodepsipeptide valinomycin, indolocarbazole staurosporine, diketopiperazine cycloisoleucylprolyl and butenolide. These compounds exhibited significant anti-parasitic as well as protease inhibitory activities. The third aim of this Ph.D. study was to identify biosynthetic gene clusters encoding for nonribosomal peptide synthetases (NRPS) and polyketide synthases (PKS) present in the actinomycete strains. Genomic library construction and sequencing revealed insights into the metabolic potential and biosynthetic pathways of selected strains. An interesting NRPS system detected in Streptomyces sp. strain Aer003 was found to be widely distributed in several sponge species, in an ascidian and in seawater and is postulated to encode for a large peptide molecule. Sequencing of the PKS gene cluster of Saccharopolyspora cebuensis strain SPE 10-1T allowed the prediction of the cebulactam biosynthetic pathway which utilizes 3-amino-5-hydroxybenzoic acid as the starter unit followed by successive condensation steps involving methylmalonyl extender units and auxiliary domains responsible for the polyketide assembly. In conclusion, this Ph.D. study has shown that diverse actinomycete genera are associated with marine sponges. The strains, two of them novel species, produced diverse chemical structures with interesting anti-infective properties. Lastly, the presence of biosynthetic gene clusters identified in this study substantiates the biosynthetic potential of actinomycetes to produce exploitable natural products and hopefully provides a sustainable supply of anti-infective compounds.
This study explores novelty choice, a behavioral paradigm for the investigation of visual pattern recognition and learning of the fly Drosophila melanogaster in the flight simulator. Pattern recognition in novelty choice differs significantly from pattern recognition studied by heat conditioning, although both paradigms use the same test. Out of the four pattern parameters that the flies can learn in heat conditioning, novelty choice can be shown for height (horizontal bars differing in height), size and vertical compactness but not for oblique bars oriented at +/- 45°. Upright and inverted Ts [differing in their centers of gravity (CsOG) by 13°] that have been extensively used for heat conditioning experiments, do not elicit novelty choice. In contrast, horizontal bars differing in their CsOG by 13° do elicit novelty choice; so do the Ts after increasing their CsOG difference from 13° to 23°. This indicates that in the Ts the heights of the CsOG are not the only pattern parameters that matter for the novelty choice behavior. The novelty choice and heat conditioning paradigms are further differentiated using the gene rutabaga (rut) coding for a type 1 adenylyl cyclase. This protein had been shown to be involved in memory formation in the heat conditioning paradigm. Novelty choice is not affected by mutations in the rut gene. This is in line with the finding that dopamine, which in olfactory learning is known to regulate Rutabaga via the dopamine receptor Dumb in the mushroom bodies, is dispensable for novelty choice. It is concluded that in novelty choice the Rut cAMP pathway is not involved. Novelty choice requires short term working memory, as has been described in spatial orientation during locomotion. The protein S6KII that has been shown to be involved in visual orientation memory in walking flies is found here to be also required for novelty choice. As in heat conditioning the central complex plays a major role in novelty choice. The S6KII mutant phenotype for height can be rescued in some subsets of the ring neurons of the ellipsoid body. In addition the finding that the ellipsoid body mutants ebo678 and eboKS263 also show a mutant phenotype for height confirm the importance of ellipsoid body for height novelty choice. Interestingly some neurons in the F1 layer of the fan-shaped body are necessary for height novelty choice. Furthermore, different novelty choice phenotypes for different pattern parameters are found with and without mushroom bodies. Mushroom bodies are required in novelty choice for size but they are dispensable for height and vertical compactness. This special circuit requirement for the size parameter in novelty choice is found using various means of interference with mushroom body function during development or adulthood.
This study explores novelty choice, a behavioral paradigm for the investigation of visual pattern recognition and learning of the fly Drosophila melanogaster in the flight simulator. Pattern recognition in novelty choice differs significantly from pattern recognition studied by heat conditioning, although both paradigms use the same test. Out of the four pattern parameters that the flies can learn in heat conditioning, novelty choice can be shown for height (horizontal bars differing in height), size and vertical compactness but not for oblique bars oriented at +/- 45°. Upright and inverted Ts [differing in their centers of gravity (CsOG) by 13°] that have been extensively used for heat conditioning experiments, do not elicit novelty choice. In contrast, horizontal bars differing in their CsOG by 13° do elicit novelty choice; so do the Ts after increasing their CsOG difference from 13° to 23°. This indicates that in the Ts the heights of the CsOG are not the only pattern parameters that matter for the novelty choice behavior. The novelty choice and heat conditioning paradigms are further differentiated using the gene rutabaga (rut) coding for a type 1 adenylyl cyclase. This protein had been shown to be involved in memory formation in the heat conditioning paradigm. Novelty choice is not affected by mutations in the rut gene. This is in line with the finding that dopamine, which in olfactory learning is known to regulate Rutabaga via the dopamine receptor Dumb in the mushroom bodies, is dispensable for novelty choice. It is concluded that in novelty choice the Rut cAMP pathway is not involved. Novelty choice requires short term working memory, as has been described in spatial orientation during locomotion. The protein S6KII that has been shown to be involved in visual orientation memory in walking flies is found here to be also required for novelty choice. As in heat conditioning the central complex plays a major role in novelty choice. The S6KII mutant phenotype for height can be rescued in some subsets of the ring neurons of the ellipsoid body. In addition the finding that the ellipsoid body mutants ebo678 and eboKS263 also show a mutant phenotype for height confirm the importance of ellipsoid body for height novelty choice. Interestingly some neurons in the F1 layer of the fan-shaped body are necessary for height novelty choice. Furthermore, different novelty choice phenotypes for different pattern parameters are found with and without mushroom bodies. Mushroom bodies are required in novelty choice for size but they are dispensable for height and vertical compactness. This special circuit requirement for the size parameter in novelty choice is found using various means of interference with mushroom body function during development or adulthood.
Maintaining the balance between CO2 uptake and transpiration is important for plants and depends on tightly controlled turgor changes caused by the activity of various anion and cation channels. These channels are part of signaling cascades triggered, for example, by phytohormones such as ABA (abscisic acid) and JA (jasmonate), both of which act during drought stress in guard cells. In addition, JA is known to be involved in the plant's response to pathogen attack or wounding.
GORK (guard cell outward rectifying K+ channel) is the only known outward rectifying K+ channel in guard cells and therefore responsible for K+ efflux during stomatal closure.
In the course of this work it could be demonstrated by stomatal aperture assays, that GORK is an essential part of JA-induced stomatal closure. This is true for both triggers, leaf wounding as well as direct MeJA (methyl jasmonate) application. Patch clamp experiments on guard cell protoplasts backed this finding by revealing GORK K+ outward currents as a target of JA signaling in guard cells. As cytosolic Ca2+ signals are known to be involved in both ABA as well as JA signaling, the interaction of GORK with Ca2+-dependent kinases was examined consequently. An antagonistic regulation of GORK by
CIPK5-CBL1/9 complexes and ABI2 was identified by DEVC (double electrode voltage clamp) and protein-protein interaction experiments and backed up by in vitro kinase assays. Patch-clamp recordings on guard cell protoplasts of cipk5-2 kinase loss-of-function mutant revealed the importance of CIPK5 for JA-triggered stomatal closure via activation of GORK. The interaction of different CDPKs (Ca2+-dependent protein kinases) with GORK was also investigated.
Besides Ca2+ signaling also ROS (reactive oxygen species) production is essential in ABA and MeJA signaling. In DEVC experiments a reversible effect of ROS on GORK channel activity could be demonstrated, which could be one piece in the explanation of those ROS effects in ABA and MeJA signaling.
Blood glucose control is the primary strategy to prevent complications in diabetes. At the onset of kidney disease, therapies that inhibit components of the renin angiotensin system (RAS) are also indicated, but these approaches are not wholly effective. Here, we show that once daily administration of the novel glucose lowering agent, empagliflozin, an SGLT2 inhibitor which targets the kidney to block glucose reabsorption, has the potential to improve kidney disease in type 2 diabetes. In male db/db mice, a 10-week treatment with empagliflozin attenuated the diabetes-induced upregulation of profibrotic gene markers, fibronectin and transforming-growth-factor-beta. Other molecular (collagen IV and connective tissue growth factor) and histological (tubulointerstitial total collagen and glomerular collagen IV accumulation) benefits were seen upon dual therapy with metformin. Albuminuria, urinary markers of tubule damage (kidney injury molecule-1, KIM-1 and neutrophil gelatinase-associated lipocalin, NGAL), kidney growth, and glomerulosclerosis, however, were not improved with empagliflozin or metformin, and plasma and intra-renal renin activity was enhanced with empagliflozin. In this model, blood glucose lowering with empagliflozin attenuated some molecular and histological markers of fibrosis but, as per treatment with metformin, did not provide complete renoprotection. Further research to refine the treatment regimen in type 2 diabetes and nephropathy is warranted.
Plants attacked by herbivorous insects emit a blend of volatile compounds that serve as important host location cues for parasitoid wasps. Variability in the released blend may exist on the whole-plant and within-plant level and can affect the foraging efficiency of parasitoids. We comprehensively assessed the kinetics of herbivore-induced volatiles in soybean in the context of growth stage, plant organ, leaf age, and direction of signal transport. The observed patterns were used to test the predictions of the optimal defence hypothesis (OD). We found that plants in the vegetative stage emitted 10-fold more volatiles per biomass than reproductive plants and young leaves emitted >2.6 times more volatiles than old leaves. Systemic induction in single leaves was stronger and faster by one day in acropetal than in basipetal direction while no systemic induction was found in pods. Herbivore-damaged leaves had a 200-fold higher release rate than pods. To some extent these findings support the OD: i) indirect defence levels were increased in response to herbivory and ii) young leaves, which are more valuable, emitted more volatiles. However, the fact that reproductive structures emitted no constitutive or very few inducible volatiles is in seeming contrast to the OD predictions. We argue that in case of volatile emission the OD can only partially explain the patterns of defence allocation due to the peculiarity that volatiles act as signals not as toxins or repellents.
Young grapevines (Vitis vinifera) suffer and eventually can die from the crown gall disease caused by the plant pathogen Allorhizobium vitis (Rhizobiaceae). Virulent members of A. vitis harbor a tumor-inducing plasmid and induce formation of crown galls due to the oncogenes encoded on the transfer DNA. The expression of oncogenes in transformed host cells induces unregulated cell proliferation and metabolic and physiological changes. The crown gall produces opines uncommon to plants, which provide an important nutrient source for A. vitis harboring opine catabolism enzymes. Crown galls host a distinct bacterial community, and the mechanisms establishing a crown gall–specific bacterial community are currently unknown. Thus, we were interested in whether genes homologous to those of the tumor-inducing plasmid coexist in the genomes of the microbial species coexisting in crown galls. We isolated 8 bacterial strains from grapevine crown galls, sequenced their genomes, and tested their virulence and opine utilization ability in bioassays. In addition, the 8 genome sequences were compared with 34 published bacterial genomes, including closely related plant-associated bacteria not from crown galls. Homologous genes for virulence and opine anabolism were only present in the virulent Rhizobiaceae. In contrast, homologs of the opine catabolism genes were present in all strains including the nonvirulent members of the Rhizobiaceae and non-Rhizobiaceae. Gene neighborhood and sequence identity of the opine degradation cluster of virulent and nonvirulent strains together with the results of the opine utilization assay support the important role of opine utilization for cocolonization in crown galls, thereby shaping the crown gall community.
Guard cells control the aperture of plant stomata, which are crucial for global fluxes of CO\(_2\) and water. In turn, guard cell anion channels are seen as key players for stomatal closure, but is activation of these channels sufficient to limit plant water loss? To answer this open question, we used an optogenetic approach based on the light-gated anion channelrhodopsin 1 (GtACR1). In tobacco guard cells that express GtACR1, blue- and green-light pulses elicit Cl\(^-\) and NO\(_3\)\(^-\) currents of -1 to -2 nA. The anion currents depolarize the plasma membrane by 60 to 80 mV, which causes opening of voltage-gated K+ channels and the extrusion of K+. As a result, continuous stimulation with green light leads to loss of guard cell turgor and closure of stomata at conditions that provoke stomatal opening in wild type. GtACR1 optogenetics thus provides unequivocal evidence that opening of anion channels is sufficient to close stomata.
Channelrhodopsin-2 (ChR2) is widely used for rapid photodepolarization of neurons, yet, as it requires high-intensity blue light for activation, it is not suited for long-term in vivo applications, e. g. for manipulations of behavior, or photoactivation of neurons during development. We used "slow" ChR2 variants with mutations in the C128 residue, that exhibit delayed off-kinetics and increased light sensitivity in Caenorhabditis elegans. Following a 1 s light pulse, we could photodepolarize neurons and muscles for minutes (and with repeated brief stimulation, up to days) with low-intensity light. Photoactivation of ChR2(C128S) in command interneurons elicited long-lasting alterations in locomotion. Finally, we could optically induce profound changes in animal development: Long-term photoactivation of ASJ neurons, which regulate larval growth, bypassed the constitutive entry into the "dauer" larval state in daf-11 mutants. These lack a guanylyl cyclase, which possibly renders ASJ neurons hyperpolarized. Furthermore, photostimulated ASJ neurons could acutely trigger dauer-exit. Thus, slow ChR2s can be employed to long-term photoactivate behavior and to trigger alternative animal development.
Water transport through the water channels, aquaporins (AQPs), is involved in epithelial fluid secretion and absorption, cell migration, brain edema, adipocyte metabolism, and other physiological or pathological functions. Modulation of AQP function has therapeutic potential in edema, cancer, obesity, brain injury, glaucoma, etc. The function of AQPs is in response to the osmotic gradient that is formed by the concentration differences of ions or small molecules. In terms of brain edema, it is a pathophysiological condition, resulting from dysfunction of the plasma membrane that causes a disorder of intracellular ion homeostasis and thus increases intracellular fluid content. Optogenetics can be used to regulate ion transport easily by light with temporal and spatial precision. Therefore, if we control the cell ion influx, boosting the water transport through AQPs, this will help to investigate the pathological mechanisms in e.g. brain edema. To this end, I investigated the possibility for optogenetic manipulating water transport in Xenopus oocytes. The main ions in Xenopus oocyte cytoplasm are ~10 mM Na+, ~50 mM Cl- and ~100 mM K+, similar to the mammalian cell physiological condition. Three light-gated channels, ChR2-XXM 2.0 (light-gated cation channel), GtACR1 (light-gated anion channel) and SthK-bPAC (light-gated potassium channel), were used in my study to regulate ion transport by light and thus manipulate the osmotic gradient and water transport. To increase water flow, I also used coexpression of AQP1. When expressing ChR2-XXM 2.0 and GtACR1 together, mainly Na+ influx was triggered by ChR2-XXM2.0 under blue light illumination, which then made the membrane potential more positive and facilitated Cl- influx by GtACR1. Due to this inward movement of Na+ and Cl-, the osmotic gradient was formed to trigger water influx through AQP1. Large amounts of water uptake can speedily increase the oocyte volume until membrane rupture. Next, when co-expressing GtACR1 and SthK-bPAC, water efflux will be triggered with blue light because of the light-gated KCl efflux and then oocyte shrinking could be observed.
I also developed an optogenetic protein purification method based on a light-induced protein interactive system. Currently, the most common protein purification method is based on affinity chromatography, which requires different chromatography columns and harsh conditions, such as acidic pH 4.5 - 6 and/or adding imidazole or high salt concentration, to elute and collect the purified proteins. The change in conditions could influence the activity of target proteins. So, an easy and flexible protein purification method based on the photo-induced protein interactive system iLID was designed, which regulates protein binding with light in mild conditions and does not require a change of solution composition. For expression in E. coli, the blue light-sensitive part of iLID, the LOV2 domain, was fused with a membrane anchor and expressed in the plasma membrane, and the other binding partner, SspB, was fused with the protein of interest (POI), expressed in the cytosol. The plasma membrane fraction and the soluble cytosolic fraction of E. coli can be easily separated by centrifugation. The SspB-POI can be then captured to the membrane fraction by light stimulation and released to clean buffer in the dark after washing. This method does not require any specific column and functions in mild conditions, which are very flexible at scale and will facilitate extensive protein engineering and purification of proteins, sensitive to changed buffer conditions.
Optogenetics is a powerful technique that utilizes light to precisely regulate physiological activities of neurons and other cell types. Specifically, light-sensitive ion channels, pumps or enzymes are expressed in cells to enable their regulation by illumination, thus allowing for precise control of biochemical signaling pathways. The first part of my study involved the construction, optimization, and characterization of two optogenetic tools, KCR1 and NCR1. Elena Govorunova et al. discovered a lightgated potassium channel, KCR1, in the protozoan Hyphochytrium catenoides. Traditional potassium ion channels are classified as either ligand-gated or voltage-gated and possess conserved pore-forming domains and K+ -selective filters. However, KCR1 is unique in that it does not contain the signature sequence of previously known K+ channels and is a channelrhodopsin. We synthesized the KCR1 plasmid according to the published sequence and expressed it in Xenopus oocytes. Due to the original KCR1 current being too small, I optimized it into KCR1 2.0 to improve its performance by fusing LR (signal peptide LucyRho, enhances expression) at the N-terminal and T (trafficking signal peptide) and E (ER export signal peptide) at the C-terminal. Additionally, I investigated the light sensitivity, action spectrum, and kinetics of KCR1 2.0 in Xenopus oocytes. The potassium permeability of KCR1 2.0, PK/Pna 24, makes KCR1 2.0 a powerful hyperpolarizing tool that can be used to inhibit neuronal firing in animals. Inspired by KCR1, we used the KCR1 sequence as a template for gene sequence alignment with the sequences in H. catenoides. We found that NCR1 and KCR1 have similar gene sequences. NCR1 was characterized by us as a light-gated sodium channel. This NCR1 was also characterized and published by Govorunova et al. very recently, with the name HcCCR. Due to the original NCR1 current being too small, I optimized it into NCR1 2.0 to improve its performance by fusing LR at the N-terminal and T and E at the C-terminal, which significantly improved the expression level and greatly increased the current amplitude of NCR1. Full-length NCR1 2.0 contains 432 amino acids. To test whether the number of amino acids changes the characteristics of NCR1 2.0, we designed NCR1 2.0 (330), NCR1 2.0 (283), and NCR1 2.0 (273) by retaining the number of amino acids at 330, 280, and 273 in NCR1 2.0, respectively. As the number of amino acids decreased, the current in NCR1 2.0 increased. I also investigated the light sensitivity, action spectrum, and kinetics of NCR1 2.0 (273) in the Xenopus Abstract 2 oocytes. We performed four point mutations at amino acid positions 133 and 116 of NCR1 2.0 and analyzed the reversal potentials of the mutants. The mutations were as follows: NCR1 2.0 (273 D116H), NCR1 2.0 (273 D116E), NCR1 2.0 (283 V133H), and NCR1 2.0 (283 D116Q). The second part of this study focuses on light-induced water transport using optogenetic tools. We explored the use of optogenetic tools to regulate water flow by changing the osmolarity in oocytes. Water flux through AQP1 is driven by the osmotic gradient that results from concentration differences of small molecules or ions. Therefore, we seek to regulate ion concentrations, using optogenetic tools to regulate the flux of water noninvasively. To achieve this, I applied the light-gated cation channels XXM 2.0 and NCR1 2.0 to regulate the concentration of Na+ , while K + channel KCR1 2.0 was used to regulate K + concentration. As Na+ flows into the Xenopus oocytes, the membrane potential of the oocytes becomes positive, and Clcan influx through the light-gated anion channel GtACR1. By combining these optogenetic tools to regulate NaCl or KCl concentrations, I can change the osmolarity inside the oocytes, thus regulating the flux of water. I co-expressed AQP1 with optogenetic tools in the oocytes to accelerate water flux. Overall, I designed three combinations (1: AQP1, XXM 2.0 and GtACR1. 2: AQP1, NCR1 2.0 and GtACR1. 3: AQP1, KCR1 2.0 and GtACR1) to regulate the flow of water in oocytes. The shrinking or swelling of the oocytes can only be achieved when AQP1, light-gated cation channels (XXM 2.0/NCR1 2.0/KCR1 2.0), and light-gated anion channels (GtACR1) are expressed together. The illumination after expression of either or both alone does not result in changes in oocyte morphology. In sum, I demonstrated a novel strategy to manipulate water movement into and out of Xenopus oocytes, non-invasively through illumination. These findings provide a new avenue to interfere with water homeostasis as a means to study related biological phenomena across cell types and organisms.
Funktionelle Expression von ChR2 in Pflanzen In der vorliegenden Arbeit konnte erstmalig die funktionelle Expression des licht-aktivierten Channelrhodopsin-2 aus Chlamydomonas reinhardtii in höheren Pflanzen gezeigt werden. Obwohl die erfolgreiche Transformation auf der Basis der Integration einer Expressionskassette für WT-ChR2 in Pflanzen genetisch nachgewiesen werden konnte, war ein funktioneller Nachweis nicht möglich. Demgegenüber war die funktio-nelle Expression aller getesteten ChR2-Mutanten im transienten Expressionsansatz er-folgreich und konnte schließlich auf der Basis der im Rahmen dieser Arbeit generierten Konstrukte auch für stabil transformierte Arabidopsis-Pflanzen bestätigt werden. ChR2 wurde in Arabidopsis-Protoplasten sowie Tabak-Epidermis- und Mesophyllzellen an der Plasmamembran lokalisiert, zeigte jedoch aufgrund der Überexpression eine starke Überladung des Endomembransystems. Elektrophysiologische Messungen mit Hilfe der Einstichtechnik belegten, dass ChR2 sowohl in Arabidopsis-Keimlingen als auch im Tabakmesophyll funktionell ist, wobei sich die erzeugten Blaulicht-vermittelten Depolarisationen weitaus erfolgreicher im Ta-baksystem darstellten. Alle eingesetzten ChR2-Mutanten waren funktionell und zeigten in Einstichmessungen mit Oozytendaten korrelierende Kinetiken. Die Mutante C128A wurde hinsichtlich der erzielten lichtinduzierten Membranpotentialdepolarisationen als effektivste ChR2-Variante identifiziert. Calcium-Messungen mit dem Reporterprotein Aequorin lieferten keinen Beweis für einen direkt durch ChR2-C128A vermittelten Calcium-Einstrom in Arabidopsis-Protoplasten. Jedoch konnte ein cytosolischer Calcium-Anstieg ca. 3min nach Blau-lichtapplikation beobachtet werden. Dies deutet darauf hin, dass die durch ChR2 vermittelten Membranpotentialänderungen zu einer Aktivierung endogener, Calcium-permeabler Ionenkanäle führen könnte. Für die ChR2-L132C Mutante konnte allerdings in ersten Messungen ein direkter Calcium-Anstieg nach Lichtgabe beobachtet werden. Transkriptionelle Änderungen aufgrund ChR2-basierter, elektrischer Signalmuster In RNA-Seq-Analysen mit transient transformierten Tabakblättern konnte die Bedeu-tung der Signalsignatur elektrischer bzw. Calcium-basierter Signale verifiziert werden: Die Applikation zweier in ihrer Form gänzlich unterschiedlicher elektrischer Signal-muster lieferte ein signifikant unterschiedlich reguliertes Set an Genen, wobei einige wenige durch beide Behandlungen induziert werden konnten. Langanhaltende Depolari-sationen regulierten deutlich mehr Gene und waren daher in ihrer Wirkung weitaus ef-fektiver als kurze, repetitive Depolarisationen. Die bioinformatische Analyse dieser Daten zeigte, dass die Nachahmung eines im Zuge der Pathogenantwort bekannten, langen Depolarisationspulses Gene der Flagellin-induzierten Signaltransduktion adressierte, während kurze, wiederkehrende Pulse mit gleichem Informationsgehalt diese nicht regulierten.
Oxylipine sind Signalmoleküle, welche durch die enzymatische oder nicht-enzymatische Oxidation von Fettsäuren gebildet werden. Eine bedeutende Gruppe von Oxylipinen in Pflanzen sind die Jasmonate. Dazu zählen Jasmonsäure (JA), deren Vorstufe 12-Oxophytodiensäure (OPDA) sowie deren Metabolite. Ein bedeutender Metabolit von JA ist das Aminosäure-Konjugat JA-Isoleucin (JA-Ile), welches hohe biologische Aktivität besitzt. Besonders für die oberirdischen Organe von Pflanzen wurden bisher vielfältige Funktionen von Jasmonaten beschrieben. Sie sind beteiligt an verschiedenen Entwicklungsprozessen wie der Fertilität von Blüten, aber auch an der Abwehr von Pathogenen und Herbivoren und bei der Reaktion von Pflanzen auf abiotische Stressoren wie hohe Salzkonzentrationen oder Trockenheit. Über die Bildung und Funktion von Oxylipinen in Wurzeln ist bisher jedoch nur wenig bekannt. Aus diesem Grund wurden in der vorliegenden Arbeit die Gehalte von Galaktolipiden und Jasmonaten in Spross und Wurzel von Arabidopsis thaliana Pflanzen verglichen. Mit Hilfe verschiedener JA Biosynthese-Mutanten konnte zudem die Bildung von Jasmonaten in der Wurzel und deren biologische Funktion in diesem Pflanzenorgan untersucht werden. Um die Wurzeln der Arabidopsis Pflanzen einfach behandeln zu können und um schnell und stressfrei größere Mengen von Wurzelmaterial ernten zu können, wurde ein hydroponisches Anzuchtsystem etabliert. Die Analyse von Galaktolipiden zeigte, dass in der Wurzel deutlich geringere Galaktolipid Gehalte als im Spross vorhanden sind. Da Galaktolipide den Hauptbestandteil plastidärer Membranen ausmachen, in den Wurzeln insgesamt jedoch weniger Plastiden vorkommen als in Blättern, wäre dies ein möglicher Grund für den beobachteten Unterschied. Das Vorkommen von mit OPDA oder dnOPDA veresterten Galaktolipiden (Arabidopsiden) wird in der Literatur für die Thylakoidmembranen der Chloroplasten beschrieben. Die Analyse der Arabidopsid Gehalte von Wurzeln konnte diese Aussage stützen, da in Wurzeln, welche normalerweise keine Chloroplasten besitzen, nahezu keine Arabidopside detektiert werden konnten. Die Analyse der Jasmonate zeigte anhand von Pfropfungsexperimenten mit der Jasmonat-freien dde2 Mutante, dass die Wurzeln unabhängig vom Spross in der Lage sind Jasmonate zu bilden, obwohl die Expression vieler JA-Biosynthese-Gene in den Wurzeln sehr gering ist. Zudem zeigten diese Experimente, dass es keinen direkten Transport von Jasmonaten zwischen Spross und Wurzel gibt. Die Bildung von Jasmonaten in der Wurzel konnte durch verschiedene Stresse wie Verwundung, osmotischen Stress oder Trockenheit induziert werden. Kälte und Salzstress hatten hingegen keinen Jasmonat-Anstieg in den Wurzeln zur Folge. Anders als bei osmotischem Stress und Trockenheit, wo sowohl die Gehalte von OPDA als auch von JA und JA-Ile anstiegen, konnte bei Verwundung keine Zunahme der OPDA-Spiegel detektiert werden. Hier kam es zu einer deutlichen Abnahme, wohingegen die JA und JA-Ile Spiegel sehr stark anstiegen. Dies deutet darauf hin, dass es sehr komplexe und vielfältige Regulationsmechanismen hinsichtlich der Bildung von Jasmonaten gibt. Der erste Schritt der JA-Biosynthese, die Bildung von 13-Hydroperoxyfettsäuren (HPOTE), wird durch 13-Lipoxygenase (LOX) Enzyme katalysiert. In Arabidopsis sind vier unterschiedliche 13-LOX Isoformen bekannt. Die Untersuchung verschiedener 13-LOX-Mutanten ergab, dass nur die LOX6 an der Biosynthese von Jasmonaten in der Wurzel beteiligt ist. So konnten in Wurzeln der lox6 Mutante weder basal noch nach verschiedenen Stressen bedeutende Mengen von Jasmonaten gemessen werden. Im Spross dieser Mutante war basal kein OPDA vorhanden, nach Stresseinwirkung wurden jedoch ähnliche Jasmonat Gehalte wie im Wildtyp detektiert. Um Hinweise auf die biologische Funktion von Jasmonaten in Wurzeln zu erhalten, wurden Untersuchungen mit einer lox6 KO Mutante durchgeführt. Dabei zeigte sich, dass abgeschnittene lox6 Wurzeln, welche keine Jasmonate bilden, im Vergleich zum Wildtyp von saprobiont lebenden Kellerasseln (Porcellio scaber) bevorzugt als Futter genutzt werden. Blätter dieser Mutante, welche nach Stress annähernd gleiche Jasmonat Gehalte wie der Wildtyp aufweisen, wurden nicht bevorzugt gefressen. Von der Jasmonat-freien dde2 Mutante wurden hingegen sowohl die Wurzeln als auch die Blätter bevorzugt gefressen. Neben den Experimenten mit Kellerasseln wurden auch Welke-Versuche mit lox6 und dde2 Pflanzen durchgeführt. Hierbei wiesen die lox6 Pflanzen, nicht aber die dde2 Pflanzen, eine erhöhte Suszeptibilität gegenüber Trockenheit auf. dde2 Pflanzen haben im Gegensatz zu LOX Mutanten unveränderte 13-HPOTE Gehalte, aus denen auch andere Oxylipine als Jasmonate gebildet werden können. Dies zeigt, dass durch LOX6 gebildete Oxylipine, im Falle von Trockenheit aber nicht Jasmonate, an der Reaktion von Arabidopsis Pflanzen auf biotische und abiotische Stresse beteiligt sind.
RS1 is the intron less singel copy gene involved in regulation of plasme membrane transporters. Ornithine decarboxylase is identified as the receptor of RS1 specific for the release of vesicles containing SGLT1 specifically at the trans-golgi network. RS1 decreases the activity of ODC there by inhibiting the release of vesicles containing specifically SGLT1.
Phytoprostane (PP) können nichtenzymatisch in vitro und in vivo durch freie Radikal-katalysierte Peroxidation von alpha-Linolensäure entstehen. In der vorliegenden Arbeit konnte gezeigt werden, dass über den D1-Phytoprostan-Weg zwei weitere Klassen von Phytoprostanen gebildet werden können, die D1-Phytoprostane (PPD1) und die Deoxy-J1-Phytoprostane (dPPJ1). PPD1 und dPPJ1 wurden erstmals durch Partialsynthese hergestellt. Zudem konnten diese Verbindungen durch Autoxidation von alpha-Linolensäure gewonnen werden. PPD1 und dPPJ1 wurden chromatographisch aufgetrennt und UV-spektroskopisch und massenspektrometrisch charakterisiert. Zum Nachweis von PPD1 und dPPJ1 in planta wurde eine neuartige Analysenmethode mittels Fluoreszenz-HPLC entwickelt. Mit dieser Methode konnten PPD1 und dPPJ1 in drei unterschiedlichen Pflanzenspezies nachgewiesen werden. Zudem wurde eine verstärkte Biosynthese von dPPJ1 in planta durch oxidativen Stress beobachtet, z.B. durch eine Belastung mit Schwermetallen oder einen kurzfristigen Kälteschock. Darüber hinaus konnte gezeigt werden, dass dPPJ1 sowohl in Pflanzen als auch in Tieren biologisch aktiv sind.
By comparison with plant microbe interaction, little is known about the interaction of parasitic plants with their hosts. Plants of the genus Cuscuta belong to the family of Cuscutaceae and comprise about 200 species, all of which live as stem holoparasites on other plants. Cuscuta spp. possess no roots nor fully expanded leaves and the vegetative portion appears to be a stem only. The parasite winds around plants and penetrates the host stems via haustoria, forming direct connections to the vascular bundles of their hosts to withdraw water, carbohydrates, and other solutes. Besides susceptible hosts, a few plants exist that exhibit an active resistance against infestation by Cuscuta spp. For example, cultivated tomato (Solanum lycopersicum) fends off Cuscuta reflexa by means of a hypersensitive-type response occurring in the early penetration phase. This report on the plant plant dialog between Cuscuta spp. and its host plants focuses on the incompatible interaction of C. reflexa with tomato.
Simple Summary
Abiotic and biotic stress conditions result in profound changes in plant lipid metabolism. Vegetable oil consists of triacylglycerols, which are important energy and carbon storage compounds in seeds of various plant species. These compounds are also present in vegetative tissue, and levels have been reported to increase with different abiotic stresses in leaves. This work shows that triacylglycerols accumulate in roots and in distal, non-treated leaves upon treatment with a fungal pathogen or lipopolysaccharide (a common bacterial-derived elicitor in animals and plants). Treatment of leaves with a bacterial pathogen or a bacterial effector molecule results in triacylglycerol accumulation in leaves, but not systemically in roots. These results suggest that elicitor molecules are sufficient to induce an increase in triacylglycerol levels, and that unidirectional long-distance signaling from roots to leaves is involved in pathogen and elicitor-induced triacylglycerol accumulation.
Abstract
Interaction of plants with the environment affects lipid metabolism. Changes in the pattern of phospholipids have been reported in response to abiotic stress, particularly accumulation of triacylglycerols, but less is known about the alteration of lipid metabolism in response to biotic stress and leaves have been more intensively studied than roots. This work investigates the levels of lipids in roots as well as leaves of Arabidopsis thaliana in response to pathogens and elicitor molecules by UPLC-TOF-MS. Triacylglycerol levels increased in roots and systemically in leaves upon treatment of roots with the fungus Verticillium longisporum. Upon spray infection of leaves with the bacterial pathogen Pseudomonas syringae, triacylglycerols accumulated locally in leaves but not in roots. Treatment of roots with a bacterial lipopolysaccharide elicitor induced a strong triacylglycerol accumulation in roots and leaves. Induction of the expression of the bacterial effector AVRRPM1 resulted in a dramatic increase of triacylglycerol levels in leaves, indicating that elicitor molecules are sufficient to induce accumulation of triacylglycerols. These results give insight into local and systemic changes to lipid metabolism in roots and leaves in response to biotic stresses.
Photosynthetic plants have a remarkable ability to modify their metabolism and development according to ever changing environmental conditions. The root system displays continuous growth of the primary root and formation of lateral roots enabling efficient water and nutrient uptake and anchorage of the plant in soil. With regard to lateral roots, development is post-embryonic, originating from the pericycle of the primary root. Coordinated activity of several molecular signalling pathways controlled by the hormone auxin is important throughout all stages of lateral root development.At first, two adjacent Xylem Pole Pericycle (XPP) cells are activated and the nuclei of these cells migrate towards a common cell wall.This is followed by XPP cells acquiring volume thus swelling up.The XPP cells then undergo anticlinal cell division, followed by a series of periclinal and anticlinal divisions,leading to lateral root primordia.These break through the radial cell layers and emerge out the primary root.
Although root system plasticity is well-described in response to environmental cues such as ion nutrition in the soil, little is known on how root development is shaped according to the endogenous energy status of the plant.In this study, we were able to connect limited perturbations in photosynthetic energy supply to lateral root development.We established two experimental systems – treatment with low light and unexpected darkness which led to short-term energy imbalance in the plant.These short perturbations administered, showed an increase in the emerged lateral root density and decrease in root hexose availability and activation of the low energy marker gene ASN1 (ASPARAGINE SYNTHETASE 1).Although not demonstrated, presumably, these disturbances in the plant energy homeo-stasis activates SnRK1 (SNF1 RELATED KINASE 1),an evolutionary conserved kinase mediat-ing metabolic and transcriptional responses towards low energy conditions. In A. thaliana, two catalytic α-subunits of this kinase (SnRK1.α1 and SnRK1.α2) are functionally active and form ternary complexes with the regulatory β- and γ- subunits. Whereas unexpected darkness results in an increase in emerged lateral root density, the snrk1.α1 loss-of-function mutant displayed decrease in emerged lateral root density. As this effect is not that pronounced in the snrk1.α2 loss-of-function mutant, the α1 catalytic subunit is important for the observed lateral root phenotype under short-term energy perturbations. Moreover, root expression patterns of SnRK1.α1:GFP supports a role of this catalytic subunit in lateral root development. Furthermore, the lateral root response during short-term perturbations requires the SnRK1 downstream transcriptional regulator bZIP63 (BASIC LEU-CINE ZIPPER 63), as demonstrated here by a loss-of-function approach. Phenotypic studies showed that in comparison to wild-type, bzip63 mutants displayed decreased lateral root density upon low-light and unexpected darkness conditions. Previous work has demonstrat-ed that SnRK1 directly phosphorylates bZIP63 at three serine residues. Alanine-exchange mutants of the SnRK1 dependent bZIP63 phosphorylation sites behave similarly to bzip63 loss-of-function mutants and do not display increased lateral root density upon short-term unexpected darkness. This data strongly supports an impact of SnRK1-bZIP63 signalling in mediating the observed lateral root density phenotype. Plants expressing a bZIP63:YFP fu-sion protein showed specific localization patterns in primary root and in all developmental stages of the lateral root. bzip63 loss-of-function mutant lines displayed reduced early stage lateral root initiation events under unexpected darkness as demonstrated by Differen-tial Interference Contrast microscopy (DIC) and the use of a GATA23 reporter line. This data supports a role of bZIP63 in early lateral root initiation.
Next, by employing Chromatin Immunoprecitation (ChIP) sequencing, we were able to iden-tify global binding targets of bZIP63, including the auxin-regulated transcription factor (TF) ARF19 (AUXIN RESPONSE FACTOR 19), a well-described central regulator of lateral root development. Additional ChIP experiments confirmed direct binding of bZIP63 to an ARF19 promoter region harboring a G-Box cis-element, a well-established bZIP63 binding site. We also observed that short-term energy perturbation upon unexpected darkness induced tran-scription of ARF19, which was impaired in the bzip63 loss-of-function mutant. These results propose that bZIP63 mediates lateral root development under short-term energy perturba-tion via ARF19.
In conclusion, this study provides a novel mechanistic link between energy homeostasis and plant development. By employing reverse genetics, confocal imaging and high-throughput sequencing strategies, we were able to propose a SnRK1-bZIP63-ARF19 signalling module in integrating energy signalling into lateral root developmental programs.
Zusammenfassung: Untersucht wurden die Pflanzenbemalungen in drei unterfränkischen Kirchen, die in ihrer Naturnähe und damit botanischen Korrektheit sowie in ihrer Intention differieren. Die Aufgabe der Arbeit war, soweit möglich eine botanische Bestimmung durchzuführen, nach Gründen für das Auftauchen von floralen Dekorationen in Sakralräumen allgemein und speziell für das Auftauchen einer bestimmten Species im speziellen zu suchen. Die drei betrachteten Kirchen unterscheiden sich zum einen in ihrer ursprünglichen Nutzung: "normale" Pfarrkirche, Hofkapelle eines Domherrenhofs und Betort einer Rosenkranzbruderschaft, die im Zuge der Gegenreformation unter Julius Echter gegründet wurde. Letztere diente wohl auch als repräsentative Schloßkapelle zum Schloß Büchold. Weitere Unterschiede sind in der Qualität der Ausmalung zu erkennen: Die Gotteshäuser in Rothenfels und im Seebacher Hof verfügen über Pflanzendarstellungen, die stark schematisiert sind, wobei die der Allendorfkapelle noch Ansätze von Naturbeobachtung erkennen lassen. Demgegenüber erscheinen die Fresken im Chor der Bücholder Pfarrkirche zwar auch leicht schematisiert, aber doch so nah an der Natur, daß wenigstens zum Teil eine Bestimmung bis auf die Art gelungen ist; bei einigen Exemplaren war dies jedoch nicht möglich. In letzterem Gotteshaus ist die Bemalung ein existentieller Teil des ikonographischen Konzeptes; Rothenfels läßt ein solches nicht erkennen; die Kapelle im Hof Luden entzieht sich einer Beurteilung diesbezüglich, da ihre Innenausstattung kriegsbedingt verbrannt ist. Das dortige Vorkommen von Ruta graveolens L., Rosa spec. und Tulipa spec. als bekannten Marienpflanzen macht ein früher erkennbares Konzept jedoch wahrscheinlich. Zur Kirche St. Nikolaus und Mariae Heimsuchung in Arnstein-Büchold: Der Chor ist in seiner Gesamtheit Teil des Ausstattungsprogramms der Kirche: er symbolisiert den hortus conclusus, den Garten, der Sinnbild nicht nur für die Gottesmutter ist. Innerhalb dieses Chorgartens lassen sich an den liturgisch wichtigen Stellen - Chorbogen, Chorhaupt und Schlußstein - durchweg bekannte Symbolpflanzen finden. Das Chorgewölbe ist in sich gegliedert in 50 Teile und korrespondiert direkt mit der Anzahl der Rosenkränze im Rosenkranzgebet; diese 50 Deckenteile bilden zusammen zwei vierzählige Blüten, die das Garten- oder Blumenmotiv verstärken. An Stellen, die ohne besondere Wichtigkeit sind, hat der Maler Wolfgang Ritterlein eine bunte Mischung aus einheimischen, fremdländischen und phantastischen Pflänzlein gestaltet, so daß in der Gesamtheit nicht nur ein umschlossener Garten, sondern auch eine Wunderkammer, ein Kuriositätenkabinett entsteht. - Damit erweist sich die Bemalung dieses Chors als eine schöne Symbiose aus symbolhafter Ausstattung und Repräsentation wie sie zu Beginn des Barocks nicht selten begegnet.
The present study was aimed at revealing the early signalling events during the interaction of the diazotrophic soil bacterium Azospirillum brasilense with its host plant Arabidopsis thaliana. Furthermore, taking advantage of the micro array technique, a comprehensive overview of Arabidopsis genes has been undertaken which are affected upon association with A. brasilense The characterization of the early responses of Arabidopsis plants upon inoculation with Azospirillum brasilense strain Sp7 clearly indicated parallels with the initial events in plant pathogen interaction. For instance, not only bacterial preprations (lysates) form Azospirillum elicited an apoplastic alkalinization of the culture medium, but also the live bacteria, which were even more effective. Besides, in a luminol based assay, the bacterial lysates triggered production of the reactive oxygen species (ROS) in the Arabidopsis leaf discs. Interestingly, the elongation factor receptor mutants (efr) were completely insensitive to Azospirillum, suggesting elongation factor Tu (EF-TU) recognition as elicitor by Arabidopsis. This hypothesis was further validated with a bioinformatic approach. The N terminus initial 26 amino acids from Azospirillum EF-TU gene (elf26) showed more similarity to the elf26 sequences of bacteria like Agrobacterium tumefaciens which elicit responses in the plants through EF-TU rather than Pseudomonas syringae where the potent elicitor is flagellin 22. Universal transcriptome profiling of Arabidopsis thaliana seedlings upon inoculation with Azospirillum brasilense over a time course of six, twenty four and ninty six hours revealed very little genetic responses in the early time points. However, a bulk of genes was differentially regulated in 96 hours post inoculation (96hpi). The nature of these genes indicated that the bacterial treatment, among others, greatly affect the processes like cell wall modification, hormone metabolism, stress and secondary metabolism. Additionally expression levels of a numer of transcription factors (TFs) related to basic helix loop helix (BHLH) and MYB domain containing TF families were altered with Azospirillum inoculation. Particularly the BHLH TFs were among the most highly regulated genes. The array results from Azospirillum treated plants were further compared with the already available data emnating from treatment with flagellin 22 (flg22), oligogalacturonides (OGs) and Agrobacterium tumefaciens. Noteworthy, very different set of genes were affected upon inoculation with Azospirillum in relation to other treatments. Secondly a cluster of proteins involved in the biosynthesis of aliphatic glucosinolates (GSL) were uniquely induced upon Sp7 exposure. Genes operating in flavonoid biosynthesis also showed a distinct regulation trend in the comparative analysis. Taken together, the study in question provides insights into the early signalling events in the context of Azospirillum-Arabidopsis association and the bacterial signals recognized by the plants. The array data, at the same time, elucidates the genetic factors of Arabidopsis triggered upon association with Azospirillum brasilense.
Physiological Role of Fatty Acid Desaturation in Agrobacterium-induced Arabidopsis Crown Galls
(2011)
Crown gall development is accompanied by hypoxia, drought and oxidative stress. These abiotic stress factors are known to have an impact on fatty acid (FA) desaturation. Thus, an alteration in the lipid profile of plant tumors was expected. A comprehensive lipid analysis of Arabidopsis thaliana crown galls induced by Agrobacterium tumefaciens showed an increase in the degree of FA desaturation. The poly unsaturated fatty acid (PUFA) linolenic acid (18:3) of endoplasmic reticulum (ER) derived phospholipids was especially affected. The increased levels of desaturated FAs were reflected by a strong induction of two genes encoding desaturases, FAD3 and SAD6. In contrast to FAD3, which encodes the ER membrane bound fatty acid desaturase enzyme that synthesizes 18:3 PUFAs in the ER, the function of SAD6 is unknown. The ability of SAD6 to complement the extreme dwarf growth phenotype of the ssi2-2 mutant allele suggests that SAD6 is a functional stearoyl-acyl-carrier-protein delta-9 desaturase (SAD) which catalyzes the first step in FA desaturation and forms stearic acid (18:1). Overexpression of the SAD6 gene in Arabidopsis (SAD6-OE) to a similar degree as in tumors resulted in a light-dependent chlorosis phenotype and caused a similar shift in the lipid profile towards unsaturated phospholipids. Posttranscriptional down-regulation of SAD6 overexpression by RNA reverted the chlorosis phenotype and the changes in the lipid profile, showing that SAD6 overexpression forms the unsaturated FA profile and the phenotype in SAD6-OE. The subcellular localization of the SAD6 protein in chloroplasts, which is obligatory for SAD function was demonstrated. SSI2, which encodes the major contributor to the 18:1 FA levels in Arabidopsis is down-regulated in crown galls pointing to a replacement of SSI2 function by SAD6 in the tumor. SAD6 transcripts were almost undetectable in Arabidopsis under normal growth condition, whereas under hypoxia the gene was strongly activated. In the tumor hypoxia most likely caused the very high transcription of SAD6. Hypoxia is known to limit FA desaturation and it is associated with an elevated reactive oxygen species (ROS) production which is detrimental for unsaturated FAs. Thus, up-regulation of SAD6 in the crown gall, most likely serves as an adaptive mechanism to activate desaturation under low oxygen concentrations and to maintain the levels of unsaturated FA under oxidative stress. The ER localized FAD3 most likely is responsible for the rise in 18:3 of the phospholipid class to cope with drought stress in crown galls. This hypothesis was supported by the loss of function mutant, fad3-2, which developed significantly smaller tumors as the wild type under low relative humidity.Taken together, this study suggests that the induction of SAD6 and FAD3 shapes the tumor lipid profile by increasing the levels of unsaturated FAs. Unsaturated fatty acids prepare the crown gall to cope with ongoing hypoxia, drought and oxidative stress during growth and development.
In vorausgegangenen Experimenten unseres Labors war bereits gezeigt worden, dass die Applikation von Glutamat zur transienten Erhöhung der cytosolischen Calciumkonzentration sowie zu einer Depolarisation der Plasmamembran von Mesophyllzellen führt. Pharmakologische Studien weisen auf mögliche Orthologe tierischer ionotroper Glutamatrezeptoren (iGLuRs) hin. Ziel dieser Arbeit war eine vertiefte molekulare und funktionelle Analyse der Glutamatrezeptoren (GLRs) aus Arabidopsis thaliana. Dabei konnten folgende Erkenntnisse gewonnen werden: i. Zugabe von extrazellulärem Glutamat in Kombination mit Glycin führt in Abhängigkeit der extrazellulären ATP-Konzentration (eATP) zu einer transienten Erhöhung der Calciumkonzentration in Mesophyllzellen. ii. Die Reaktion von Mesophyllprotoplasten auf die Applikation von Glutamat und Glycin ist im Vergleich zum intakten Blatt stark reduziert, kann jedoch in Gegenwart von eATP oder Glucose signifikant gesteigert werden. iii. Diese Responsibilität von Mesophyllprotoplasten ist zum Zeitpunkt des Einsetzens der Zellwandsynthese (48h) am höchsten. iv. In Patch-Clamp Experimenten führt die photolytische Freisetzung von extrazellulärem caged-Glutamat bei 34 % der gemessenen A. thaliana Mesophyllprotoplasten zu einem verstärkten Kationentransport über die Plasmamembran. Dieser Kationenstrom kann durch gleichzeitige Anwesenheit von extrazellulärem ATP noch verstärkt werden und ist durch einen Desensitivierungsprozess gekennzeichnet. Die Empfindlichkeit dieser Ströme gegenüber Antagonisten tierischer iGluRs stellt eine Verbindung zu der Genfamilie der AtGLRs dar. v. Coexpressionexperimente ausgewählter AtGLRs geben erste Hinweise auf eine Homo- bzw. eine Heteromerbildung von AtGLR1.1 und AtGLR1.4. Aufgrund fehlender Kanalaktivität konnten einzelne, in Oozyten exprimierte AtGLRs bislang nicht funktionell charakterisiert werden. vi. Studien zur transienten und stabilen Überexpression im homologen Expressionssystem zeigen einen cytotoxischen Effekt bei funktioneller Überexpression ausgewählter AtGLRs. vii. Die Analyse der Stellung des Glutamatrezeptors 3.4 in kälteregulierten Signalnetzwerken via Microarrays weist auf ein überlappendes Aufgabenspektrum der Familie der AtGLRs hin. viii. Im Rahmen von Microarray Transkriptionsanalysen an der glr3.4-1 Mutante konnte ein bisher nicht charakterisiertes, co-reguliertes Protein identifiziert werden. Dieses Protein ist durch den Besitz einer transmembranen Region sowie einer ATP-Bindedomäne charakterisiert und könnte einen möglichen Regulator des AtGLR3.4-Kanals darstellen. ix. Die Überprüfung einer möglichen Beteiligung der pflanzlichen Glutamatrezeptoren an der Generierung der glutamatabhängigen Ca2+-Signale sowie die Suche nach Regulatoren bzw. fehlenden Untereinheiten erfolgte mithilfe Mutanten-„Sreenings“. Die Analyse der bis dato identifizierten, Glutamat-insensitiven Mutanten konnte im Rahmen dieser Arbeit nicht abgeschlossen werden.
Bis heute wurden acht Handschriften der Wundarznei des Heinrich von Pfalzpaint entdeckt. Nach einer Revision der „Breslauer Handschrift“ wurde am Medizinhistorischen Institut der Universität Würzburg bereits mit einer textkritischen Gesamtedition aller bisher bekannten Pfalzpaint-Texte begonnen. Was nun die Konzeption und die Makrostruktur der vorliegenden Studie angeht, hat sich die Grobgliederung in einen allgemeinen Teil, einen Kommentar zur ‚Wündärznei‘ und einen pflanzenmonographischen Abschnitt bewährt. Somit kann sowohl über den Pfalzpaintschen Text ein schneller Zugriff auf den alphabetisch geordneten Pflanzenteil erfolgen. Aber auch der umgekehrte Weg ist möglich, da in den einzelnen Monographien stets sämtliche Synonymnamen sowie die Indikationsbereiche mit genauer Kapitelnummer angegeben wurden. Durch Erstellen eines Kommentars konnten zunächst zahlreiche wundärztliche Begriffe geklärt und der Textinhalt in eine heute verständliche Sprache gebracht werden. Dabei muß festgehalten werden, daß die am Ende der ‚Wündärznei‘ positionierten Pestrezepte mit großer Wahrscheinlichkeit nicht von Pfalzpaint stammen, sondern zu einem späteren Zeitpunkt angehängt wurden. Textaufbau, Schreibstil, verwendete Fachtermini und das Fehlen in Pfalzpaints Register sprechen für diese Annahme. In der vorliegenden Studie wurden alle arzneilich verwendeten Pflanzen registriert, auch wenn es nicht möglich war, jede mit absoluter Sicherheit zu identifizieren. Hier hat sich das bereits in der Einleitung erwähnte Differenzierungsschema bewährt. Es ermöglicht, daß man schon bei Betrachtung der Pflanzenkapitel anhand der Identifikationsklassen I-V sofort erkennen kann, ob es sich um eine eindeutig identifizierte Pflanze handelt. Bei unsicherer Zuordnung erfolgt in der Monographie jeweils eine argumentative Abwägung der konkurrierenden Identifikationsmöglichkeiten. Nun möchte ich, um hinsichtlich der Identifizierung der Statistik zu genügen, noch einige Prozentangaben bereitstellen: Bei der Auswertung der fünf erwähnten Identifikationsklassen konnte festgestellt werden, daß fast zwei Drittel der verwendeten Pflanzen (65%) bereits über den Namen zu identifizieren waren. Durch Pfalzpaints Nennung von Synonymen, botanischen Beschreibungen und Indikationen wurde es weiterhin möglich, weitere 18% sicher zuzuordnen. In 25 Fällen (15%) konkurrierten mehrere Lösungsansätze, und es mußte eine eindeutige Identifizierung unterbleiben. Von den 171 bearbeiteten Pflanzen sind heute noch 20% (34 Drogen) offizinell im Europäischen Arzneibuch, Nachtrag 2001, verzeichnet; hier seien beispielhaft die Enzianwurzel, der Tormentillwurzelstock, die Gewürznelken und die Salbeiblätter genannt. Beim Vergleich mit dem „Leitfaden Phytotherapie“ von Schilcher/Kammerer fällt auf, daß etwa 40% des Pfalzpaint-Repertoires heute noch verwendet werden und daß weitere 17% zwar erwähnt, aber mit einer Negativmonographie belegt sind. Bei etwa 15% der Arzneipflanzen handelt es sich um importierte Drogen (z.B. Mastix, Zitwer, Ingwer), die stets eindeutig identifiziert werden konnten. In diesem Zusammenhang vermute ich - gestützt auf das ‚Circa instans‘ -, daß durch den Import und die damit verbundenen Handelsgeschäfte die Identifizierung bereits beim Kauf erfolgte (auch wenn es sich möglicherweise um Fälschungen wie z.B. beim Safran handeln konnte). Was machte die Bearbeitung der ‚Wündarznei‘ des Heinrich von Pfalzpaint so interessant und einmalig? Zum einen enthält der Text einen überraschenden Reichtum an wundchirurgischen Arbeitsweisen - angefangen mit der Versorgung einer einfachen Schnittwunde bis hin zu progressiven operativen Verfahren: ich erinnere an die Nasenersatzplastik, an die Hasenschartenoperation oder an das Vorgehen bei Darmoperationen. Bei der Nasenersatzplastik handelt es sich um eine Erstbeschreibung eines hochkomplexen Verfahrens, was erkennen läßt, daß Pfalzpaint ein Meister im Umgang mit der Sprache ist und erstmals solch schwierige Techniken zu erklären vermag. Auch auf dem Gebiet der Arzneistoffkenntnis und der galenischen Herstellungstechnik von Salben, Pflastern und anderen Arzneiformen kennt sich Pfalzpaint sehr gut aus. Auch durch die politische Situation bedingt, nämlich durch die Belagerung der Marienburg, erhält man Einblick in die medizinische und arzneiliche Versorgung von Kranken in Notzeiten. Alle diese Aspekt machen die ‚Wündärznei‘ Heinrich von Pfalzpaints zu einem wichtigen Dokument des medizinischen Systems des Spätmittelalters.
Phytoprostane F1
(2001)
Isoprostane F2 sind Autoxidationsprodukte der Arachidonsäure, die über radikal-katalysierte Oxidation entstehen. Bei einigen Erkrankungen im Tier konnte gezeigt werden, daß die Konzentration von Isoprostanen F2 mit dem verstärkten Vorkommen von freien Radikalen korreliert, weshalb Isoprostane heute als Marker des oxidativen Streß genutzt werden. Darüber hinaus weisen einige Isoprostane eine biologische Aktivität auf, weshalb sie heute als Signalstoffe des oxidativen Streß im Tier diskutiert werden. Pflanzen hingegen können keine Isoprostane F2 synthetisieren, da ihnen der Precursor Arachidonsäure fehlt. In der vorliegenden Arbeit wird gezeigt, daß analog zu den Isoprostanen F2 Phytoprostane F1 in Pflanzen aus Linolensäure gebildet werden. Hierfür wurden HPLC- und Gaschromatographie-Massenspektroskopie-Methoden entwickelt, die eine Quantifizierung von Phytoprostanen F1 in Pflanzen ermöglichten. In frischen Pflanzenorganen wurden Phytoprostane F1 sowohl in freier als auch in veresterter Form detektiert. Darüber hinaus stieg die Konzentration sowohl freier als auch veresterter Phytoprostane F1 in Pfefferminzblättern nach Verwundung und in pflanzlichen Zellkulturen nach Zusatz von Agentien, von denen bekannt ist, daß sie pflanzliche Zellen oxidativ schädigen, an. In getrockneten Pflanzenmaterialien wurden extrem hohe Konzentrationen an Phytoprostanen F1 quantifiziert. Daher steht die Vermutung nahe, daß Phytoprostane F1 ähnlich wie die Isoprostane F2 im Tier als sensitiver Marker der oxidativen Zellverletzung in der Pflanze eingesetzt werden können. Darüber hinaus konnte gezeigt werden, daß der Zusatz von Phytoprostanen F1 zu Eschscholzia californica-, Crotalaria cobalticola- and Thalictrum tuberosum-Zellsuspensionskulturen zu einer Phytoalexinakkumulation führte.
Piriformospora indica is a basidiomycete fungus colonizing roots of a wide range of higher plants, including crop plants and the model plant Arabidopsis thaliana. Previous studies have shown that P. indica improves growth, and enhances systemic pathogen resistance in leaves of host plants. To investigate systemic effects within the root system, we established a hydroponic split-root cultivation system for Arabidopsis. Using quantitative real-time PCR, we show that initial P. indica colonization triggers a local, transient response of several defense-related transcripts, of which some were also induced in shoots and in distal, non-colonized roots of the same plant. Systemic effects on distal roots included the inhibition of secondary P. indica colonization. Faster and stronger induction of defense-related transcripts during secondary inoculation revealed that a P. indica pretreatment triggers root-wide priming of defense responses, which could cause the observed reduction of secondary colonization levels. Secondary P. indica colonization also induced defense responses in distant, already colonized parts of the root. Endophytic fungi therefore trigger a spatially specific response in directly colonized and in systemic root tissues of host plants.
The carbohydrate D-glucose is the main source of energy in living organisms. In contrast to animals, as well as most fungi, bacteria, and archaea, plants are capable to synthesize a surplus of sugars characterizing them as autothrophic organisms. Thus, plants are de facto the source of all food on earth, either directly or indirectly via feed to livestock. Glucose is stored as polymeric glucan, in animals as glycogen and in plants as starch. Despite serving a general source for metabolic energy and energy storage, glucose is the main building block for cellulose synthesis and represents the metabolic starting point of carboxylate- and amino acid synthesis. Finally yet importantly, glucose functions as signalling molecule conveying the plant metabolic status for adjustment of growth, development, and survival. Therefore, cell-to-cell and long-distance transport of photoassimilates/sugars throughout the plant body require the fine-tuned activity of sugar transporters facilitating the transport across membranes. The functional plant counterparts of the animal sodium/glucose transporters (SGLTs) are represented by the proton-coupled sugar transport proteins (STPs) of the plant monosaccharide transporter(-like) family (MST). In the framework of this special issue on “Glucose Transporters in Health and Disease,” this review gives an overview of the function and structure of plant STPs in comparison to the respective knowledge obtained with the animal Na+-coupled glucose transporters (SGLTs).
Agrobacterium tumefaciens causes crown gall disease on various plant species by introducing its T-DNA into the genome. Therefore, Agrobacterium has been extensively studied both as a pathogen and an important biotechnological tool. The infection process involves the transfer of T-DNA and virulence proteins into the plant cell. At that time the gene expression patterns of host plants differ depending on the Agrobacterium strain, plant species and cell-type used. Later on, integration of the T-DNA into the plant host genome, expression of the encoded oncogenes, and increase in phytohormone levels induce a fundamental reprogramming of the transformed cells. This results in their proliferation and finally formation of plant tumors. The process of reprogramming is accompanied by altered gene expression, morphology and metabolism. In addition to changes in the transcriptome and metabolome, further genome-wide ("omic") approaches have recently deepened our understanding of the genetic and epigenetic basis of crown gall tumor formation. This review summarizes the current knowledge about plant responses in the course of tumor development. Special emphasis is placed on the connection between epigenetic, transcriptomic, metabolomic, and morphological changes in the developing tumor. These changes not only result in abnormally proliferating host cells with a heterotrophic and transport-dependent metabolism, but also cause differentiation and serve as mechanisms to balance pathogen defense and adapt to abiotic stress conditions, thereby allowing the coexistence of the crown gall and host plant.
A central objective of many ecophysiological investigations is the establishment of mechanistic explanations for plant distributions in time and space. The important, albeit mostly ignored, question arises as to the nature of the organisms that should be used as representative in pertinent experiments. I suggest that it is essential to use a “demographic approach” in physiological ecology, because physiological parameters such as photosynthetic capacity (PC, determined under non-limiting conditions with the oxygen electrode) may change considerably with plant size. Moreover, as shown for nine epiphyte species covering the most important taxonomic groups, the intraspecific variability in PC was almost always higher than the interspecific variability when comparing only large individuals. In situ studies with the epiphytic bromeliad V. sanguinolenta revealed that besides physiological parameters (such as PC) almost all morphological, anatomical and other physiological leaf parameters studied changed with plant size as well. Likewise, important processes proved to be size-dependent on whole-plant level. For example, long-term water availability was clearly improved in large specimens compared to smaller conspecifics due to the increased efficiency of the tanks to bridge rainless periods. As model calculations on whole-plant level for V. sanguinolenta under natural conditions have shown photosynthetic leaf carbon gain as well as respiratory losses of heterotrophic plant parts scaled with plant size. The resulting area related annual carbon balances were similar for plants of varying size, which corresponded to observations of size-independent (and low) relative growth rates in situ. Under favorable conditions in the greenhouse, however, small V. sanguinolenta exhibited surprisingly high relative growth rates, similar to annuals, which clearly contradicts the prevalent, but barely tested notion of epiphytes as inherently slow growing plants and simultaneously illustrates the profound resource limitations that epiphytes are subjected to in the canopy of a seasonal rain forest. From habitat conditions it seems that size-related differences in water availability are the driving force behind the observed size-dependent ecophysiological changes: the larger an epiphyte grows the more independent it is with regard to precipitation patterns. In conclusion, the results strongly emphasize the need to treat plant size as an important source of intraspecific variability and thus urge researchers to consider plant size in the design of ecophysiological experiments with vascular epiphytes.
The plant surface is the substrate upon which herbivorous insects and natural enemies meet and thus represents the stage for interactions between the three trophic levels. Plant surfaces are covered by an epicuticular wax layer which is highly variable depending on species, cultivar or plant part. Differences in wax chemistry may modulate ecological interactions. We explored whether caterpillars of Spodoptera frugiperda, when walking over a plant surface, leave a chemical trail (kairomones) that can be detected by the parasitoid Cotesia marginiventris. Chemistry and micromorphology of cuticular waxes of two barley eceriferum wax mutants (cer-za.126, cer-yp.949) and wild type cv. Bonus (wt) were assessed. The plants were then used to investigate potential surface effects on the detectability of caterpillar kairomones. Here we provide evidence that C. marginiventris responds to chemical footprints of its host. Parasitoids were able to detect the kairomone on wild type plants and on both cer mutants but the response to cer-yp.949 (reduced wax, high aldehyde fraction) was less pronounced. Experiments with caterpillar-treated wt and mutant leaves offered simultaneously, confirmed this observation: no difference in wasp response was found when wt was tested against cer-za.126 (reduced wax, wt-like chemical composition) but wt was significantly more attractive than cer-yp.949. This demonstrates for the first time that the wax layer can modulate the detectability of host kairomones.
Plants are exposed to high temperature, especially during hot summer days. Temperatures are typically lowest in the morning and reach a maximum in the afternoon. Plants can tolerate and survive short-term heat stress even on hot summer days. A. thaliana seedlings have been reported to tolerate higher temperatures for different time periods, a phenomenon that has been termed basal thermotolerance. In addition, plants have the inherent capacity to acclimate to otherwise lethal temperatures. Arabidopsis thaliana seedlings acclimate at moderately elevated temperatures between 32–38° C. During heat acclimation, a genetically programmed heat shock response (HSR) is triggered that is characterized by a rapid activation of heat shock transcription factors (HSFs), which trigger a massive accumulation of heat shock proteins that are chiefly involved in protein folding and protection.
Although the HSF-triggered heat-shock response is well characterized, little is known about the metabolic adjustments during heat stress. The aim of this work was to get more insight into heat-responsive metabolism and its importance for thermotolerance.
In order to identify the response of metabolites to elevated temperatures, global metabolite profiles of heat-acclimated and control seedlings were compared. Untargeted metabolite analyses revealed that levels of polyunsaturated triacylglycerols (TG) rapidly increase during heat acclimation. TG accumulation was found to be temperature-dependent in a temperature range from 32–50° C (optimum at 42° C). Heat-induced TG accumulation was localized in extra-chloroplastic compartments by chloroplast isolation as well as by fluorescence microscopy of A. thaliana cell cultures.
Analysis of mutants deficient in all four HSFA1 master regulator genes or the HSFA2 gene revealed that TG accumulation occurred independently to HSF. Moreover, the TG response was not limited to heat stress since drought and salt stress (but not short-term osmotic, cold and high light stress) also triggered an accumulation of TGs.
In order to reveal the origin of TG synthesis, lipid analysis was carried out. Heat-induced accumulation of TGs does not derive from massive de novo fatty acid (FA) synthesis. On the other hand, lipidomic analyses of A. thaliana seedlings indicated that polyunsaturated FA from thylakoid galactolipids are incorporated into cytosolic TGs during heat stress. This was verified by lipidomic analyses of A. thaliana fad7/8 transgenic seedlings, which displayed altered FA compositions of plastidic lipids. In addition, wild type A. thaliana seedlings displayed a rapid conversion of plastidic monogalactosyldiacylglycerols (MGDGs) into oligogalactolipids, acylated MGDGs and diacylglycerols (DGs). For TG synthesis, DG requires a FA from the acyl CoA pool or phosphatidylcholine (PC). Seedlings deficient in phospholipid:diacylglycerol acyltransferase1 (PDAT1) were unable to accumulate TGs following heat stress; thus PC appears to be the major FA donor for TGs during heat treatment. These results suggest that TG and oligogalactolipid accumulation during heat stress is driven by post-translationally regulated plastid lipid metabolism.
TG accumulation following heat stress was found to increase basal thermotolerance. Pdat1 mutant seedlings were more sensitive to severe heat stress without prior acclimatization, as revealed by a more dramatic decline of the maximum efficiency of PSII and lower survival rate compared to wild type seedlings. In contrast, tgd1 mutants over-accumulating TGs and oligogalactolipids displayed a higher basal thermotolerance compared to wild type seedlings. These results therefore suggest that accumulation of TGs increases thermotolerance in addition to the genetically encoded heat shock response.
In this study poplar trees have been examined under different stress conditions. Apart from the detailed descriptions above two main conclusions might be drawn: i) A small plant like Arabidopsis thaliana is highly susceptible to stress situations that might become life-threatening compared to a tree that has extremely more biomass at its disposal. Such an organism might be able to compensate severe stress much longer than a smaller one. It seems therefore reasonable that a crop like Arabidopsis reacts earlier and faster to a massive threat. ii) In poplar both tested stress responses seemed to be regulated by hormones. The reactions to abiotic salt stress are mainly controlled by ABA, which also has a strong impact upon cold and drought stress situations. The term commonly used for ABA is “stress hormone” and is at least applicable to all abiotic stresses. In case of herbivory (biotic stress), jasmonic acid appears to be the key-player that coordinates the defence mechanism underlying extrafloral nectary and nectar production. Thus the presented work has gained a few more insights into the complex network of general stress induced processes of poplar trees. Future studies will help to understand the particular role of the intriguing indirect defence system of the extrafloral nectaries in more detail.
The genus Borrelia belongs to the spirochete phylum, an ancient evolutionary branch of the domain bacteria that is only afar related to Gram-negative bacteria. Borreliae can be subdivided into the agents of the two borrelian-caused human diseases, Lyme disease and relapsing fever. Both disease patterns are closely related to the peculiar biology of Borrelia species and exhibit a wide spectrum of diverse clinical manifestations. Due to the small 0.91 Mb chromosome, borreliae have a lack of biosynthetic capacity. Thus, all Borrelia species are highly dependent on nutrients provided by their hosts. The transport of nutrients and other molecules across the outer membrane is enabled by pore-forming proteins, so-called porins. Porins are water-filled channels and can be subdivided into two different classes, general diffusion pores and substrate-specific porins. In terms of the Lyme disease agent Borrelia burgdorferi, three putative porins were characterized in previous studies: P13, Oms28 and P66. In contrast to Lyme disease species, the porin knowledge of relapsing fever Borrelia is low, which means that not any porin has actually been described for representatives of these agents. Thus, the general aim of this thesis was to provide insight into the porin content of both, Lyme disease and relapsing fever spirochetes. This aim could be achieved by isolating and identifying porins from Borrelia outer membranes and by biophysically characterizing them in artificial lipid membranes. In one chapter of this study, the first identification and characterization of a relapsing fever porin is presented. The pore-forming protein was isolated from outer membranes of Borrelia duttonii, Borrelia hermsii and Borrelia recurrentis and designated Oms38, for “outer membrane-spanning protein of 38 kDa”. Biophysical characterization of Oms38 was achieved by using the black lipid bilayer method and demonstrated that Oms38 forms small, water-filled channels with a single-channel conductance of 80 pS in 1 M KCl. The Oms38 channel did not exhibit voltage-dependent closure and is slightly selective for anions with a permeability ratio of cations over anions of 0.41 in KCl. Subsequently, a protein homologous to Oms38 was identified in the Lyme disease agents Borrelia burgdorferi, Borrelia garinii and Borrelia afzelii. The pore-forming protein of these species exhibits high sequence homology to Oms38 and similar biophysical properties, i.e. it forms pores of 50 pS in 1 M KCl. Interestingly, titration experiments revealed that this pore could be partly blocked by dicarboxylic anions, which means that this protein does not form a general diffusion pore but a channel with a binding-site specific for those compounds. Consequently, this porin was termed DipA, for “dicarboxylate-specific porin A”. In another set of experiments, it was shown that the porin P66 is present in both Lyme disease and relapsing fever species. Therefor, the outer membranes of the Lyme disease species Borrelia burgdorferi, Borrelia afzelii, Borrelia garinii and the relapsing fever species Borrelia duttonii, Borrelia recurrentis and Borrelia hermsii were closer investigated. Except of the P66 homologue of Borrelia hermsii P66 of all species was highly active in artificial lipid membranes, forming pores with huge single-channel conductances between 9 and 11 nS in 1 M KCl. Moreover, the channel diameter and the constitution of Borrelia burgdorferi P66 were investigated in detail. Therefor, the P66 single-channel conductance in the presence of different nonelectrolytes with known hydrodynamic radii was analyzed in black lipid bilayers. The effective diameter of the P66 channel lumen was determined to be ~1.9 nm. Furthermore, as derived from multi-channel experiments the P66-induced membrane conductance could be blocked by certain nonelectrolytes, such as PEG 400, PEG 600 and maltohexaose. Additional blocking experiments on the single-channel level revealed seven subconducting states and indicated a heptameric constitution of the P66 channel. This indication could be confirmed by Blue native PAGE analysis which demonstrated that P66 units form a complex with a corresponding mass of approximately 440 kDa. Taking together, this thesis describes detailed biochemical and biophysical investigations of both Lyme disease and relapsing fever Borrelia porins and represents an important step forward in understanding the outer membrane pathways for nutrient uptake of these strictly host-dependent, pathogenic spirochetes. Furthermore, it provides some knowledge of the outer-membrane protein composition of Borrelia spirochetes. A profound knowledge of surface-exposed proteins, such as porins, is one precondition for the production of a successful vaccine and the drug design against the two borrelian-caused diseases.
Virotherapy on the basis of oncolytic vaccinia virus (VACV) strains is a novel approach for canine cancer therapy. Here we describe, for the first time, the characterization and the use of VACV strain GLV-5b451 expressing the anti-vascular endothelial growth factor (VEGF) single-chain antibody (scAb) GLAF-2 as therapeutic agent against different canine cancers. Cell culture data demonstrated that GLV-5b451 efficiently infected and destroyed all four tested canine cancer cell lines including: mammary carcinoma (MTH52c), mammary adenoma (ZMTH3), prostate carcinoma (CT1258), and soft tissue sarcoma (STSA-1). The GLV-5b451 virus-mediated production of GLAF-2 antibody was observed in all four cancer cell lines. In addition, this antibody specifically recognized canine VEGF. Finally, in canine soft tissue sarcoma (CSTS) xenografted mice, a single systemic administration of GLV-5b451 was found to be safe and led to anti-tumor effects resulting in the significant reduction and substantial long-term inhibition of tumor growth. A CD31-based immuno-staining showed significantly decreased neo-angiogenesis in GLV-5b451-treated tumors compared to the controls. In summary, these findings indicate that GLV-5b451 has potential for use as a therapeutic agent in the treatment of CSTS.
Plant transpiration is a key element in the hydrological cycle. Widely used methods for its assessment comprise sap flux techniques for whole-plant transpiration and porometry for leaf stomatal conductance. Recently emerging approaches based on surface temperatures and a wide range of machine learning techniques offer new possibilities to quantify transpiration. The focus of this study was to predict sap flux and leaf stomatal conductance based on drone-recorded and meteorological data and compare these predictions with in-situ measured transpiration. To build the prediction models, we applied classical statistical approaches and machine learning algorithms. The field work was conducted in an oil palm agroforest in lowland Sumatra. Random forest predictions yielded the highest congruence with measured sap flux (r\(^2\) = 0.87 for trees and r\(^2\) = 0.58 for palms) and confidence intervals for intercept and slope of a Passing-Bablok regression suggest interchangeability of the methods. Differences in model performance are indicated when predicting different tree species. Predictions for stomatal conductance were less congruent for all prediction methods, likely due to spatial and temporal offsets of the measurements. Overall, the applied drone and modelling scheme predicts whole-plant transpiration with high accuracy. We conclude that there is large potential in machine learning approaches for ecological applications such as predicting transpiration.
Two sponge-derived actinomycetes, Actinokineospora sp. EG49 and Nocardiopsis sp. RV163, were grown in co-culture and the presence of induced metabolites monitored by H-1 NMR. Ten known compounds, including angucycline, diketopiperazine and beta-carboline derivatives 1-10, were isolated from the EtOAc extracts of Actinokineospora sp. EG49 and Nocardiopsis sp. RV163. Co-cultivation of Actinokineospora sp. EG49 and Nocardiopsis sp. RV163 induced the biosynthesis of three natural products that were not detected in the single culture of either microorganism, namely N-(2-hydroxyphenyl)-acetamide (11), 1,6-dihydroxyphenazine (12) and 5a, 6,11a, 12-tetrahydro-5a, 11a-dimethyl[1,4]benzoxazino[3,2-b][1,4]benzoxazine (13a). When tested for biological activity against a range of bacteria and parasites, only the phenazine 12 was active against Bacillus sp. P25, Trypanosoma brucei and interestingly, against Actinokineospora sp. EG49. These findings highlight the co-cultivation approach as an effective strategy to access the bioactive secondary metabolites hidden in the genomes of marine actinomycetes.
Climate change is increasing the frequency and intensity of warming and drought periods around the globe, currently representing a threat to many plant species. Understanding the resistance and resilience of plants to climate change is, therefore, urgently needed. As date palm (Phoenix dactylifera) evolved adaptation mechanisms to a xeric environment and can tolerate large diurnal and seasonal temperature fluctuations, we studied the protein expression changes in leaves, volatile organic compound emissions, and photosynthesis in response to variable growth temperatures and soil water deprivation. Plants were grown under controlled environmental conditions of simulated Saudi Arabian summer and winter climates challenged with drought stress. We show that date palm is able to counteract the harsh conditions of the Arabian Peninsula by adjusting the abundances of proteins related to the photosynthetic machinery, abiotic stress and secondary metabolism. Under summer climate and water deprivation, these adjustments included efficient protein expression response mediated by heat shock proteins and the antioxidant system to counteract reactive oxygen species formation. Proteins related to secondary metabolism were downregulated, except for the P. dactylifera isoprene synthase (PdIspS), which was strongly upregulated in response to summer climate and drought. This study reports, for the first time, the identification and functional characterization of the gene encoding for PdIspS, allowing future analysis of isoprene functions in date palm under extreme environments. Overall, the current study shows that reprogramming of the leaf protein profiles confers the date palm heat- and drought tolerance. We conclude that the protein plasticity of date palm is an important mechanism of molecular adaptation to environmental fluctuations.
Accumulating evidences have assigned a central role to parasite-derived proteins in immunomodulation. Here, we report on the proteomic identification and characterization of immunomodulatory excretory-secretory (ES) products from the metacestode larva (tetrathyridium) of the tapeworm Mesocestoides corti (syn. M. vogae). We demonstrate that ES products but not larval homogenates inhibit the stimuli-driven release of the pro-inflammatory, Th1-inducing cytokine IL-12p70 by murine bone marrow-derived dendritic cells (BMDCs). Within the ES fraction, we biochemically narrowed down the immunosuppressive activity to glycoproteins since active components were lipid-free, but sensitive to heat- and carbohydrate-treatment. Finally, using bioassay-guided chromatographic analyses assisted by comparative proteomics of active and inactive fractions of the ES products, we defined a comprehensive list of candidate proteins released by M. corti tetrathyridia as potential suppressors of DC functions. Our study provides a comprehensive library of somatic and ES products and highlight some candidate parasite factors that might drive the subversion of DC functions to facilitate the persistence of M. corti tetrathyridia in their hosts.
Since years, research on SnRK1, the major cellular energy sensor in plants, has tried to define its role in energy signalling. However, these attempts were notoriously hampered by the lethality of a complete knockout of SnRK1. Therefore, we generated an inducible amiRNA::SnRK1α2 in a snrk1α1 knock out background (snrk1α1/α2) to abolish SnRK1 activity to understand major systemic functions of SnRK1 signalling under energy deprivation triggered by extended night treatment. We analysed the in vivo phosphoproteome, proteome and metabolome and found that activation of SnRK1 is essential for repression of high energy demanding cell processes such as protein synthesis. The most abundant effect was the constitutively high phosphorylation of ribosomal protein S6 (RPS6) in the snrk1α1/α2 mutant. RPS6 is a major target of TOR signalling and its phosphorylation correlates with translation. Further evidence for an antagonistic SnRK1 and TOR crosstalk comparable to the animal system was demonstrated by the in vivo interaction of SnRK1α1 and RAPTOR1B in the cytosol and by phosphorylation of RAPTOR1B by SnRK1α1 in kinase assays. Moreover, changed levels of phosphorylation states of several chloroplastic proteins in the snrk1α1/α2 mutant indicated an unexpected link to regulation of photosynthesis, the main energy source in plants.
In contrast to the well described molecular basis for S-type anion currents, the genes underlying R-type anion currents were unknown until 2010. Meyer S. and colleagues (2010) showed that, localized in the guard cell plasma membrane, AtALMT12 is an R-type anion channel involved in stomatal closure. However, knocking out AtALMT12 did not fully shut down R-type currents; the almt12 loss-of-function mutant has residual R-type-like currents indicating that ALMT12 is not the only gene encoding Arabidopsis thaliana R-type channels (Meyer S. et al., 2010). This PhD thesis is focussed on understanding the properties, regulation and molecular nature of the R-type channels in Arabidopsis thaliana plants. To fulfil these aims, the patch clamp technique was used to characterize electrical features of R-type currents in various conditions such as the presence/absence of ATP, variation in cytosolic calcium concentration or the presence of cytosolic chloride. Electrophysiological study revealed many similarities between the features of Arabidopsis thaliana R-type currents (Col0) and residual R-type currents (the almt12 loss-of-function mutant). Strong voltage dependency, channel activity in the same voltage range, position of maximal recorded current and blockage by cytosolic ATP all pointed to a shared phylogenetic origin of the channels underlying these R-type currents. Expression patterns of the ALMT family members for Col0 and the almt12 mutant revealed ALMT13 and AMT14 as potential candidates of the R-type channels. Electrical characterization of Col0, almt12 and the two double loss-of-function mutants (almt12/almt13 and almt12/almt14) strongly suggest that ALMT13 mediates the calcium-dependent R-type current component that is directly regulated by cytosolic calcium. Additionally, similarly to ALMT12, ALMT14 could participate as a calcium-independent R-type anion channel. Differences in response to the cytosolic calcium concentration between ALMT12, ALMT13 and ALMT14 suggest their possible involvement in different signalling pathways leading to stomatal closure. Moreover, a study performed for the two Arabidopsis thaliana ecotypes Col0 and WS showed drastically increased ALMT13 expression for WS, which is related to R-type current properties. The WS ecotype has calcium-dependent R-type current behaviour, while it is calcium-independent in Col0. Furthermore, this plant line showed lower peak current densities compared to Col0 and almt mutants. These facts strongly suggest interaction between ALMT12 and ALMT13, with ALMT13 as a repressor of the ALMT12. Acquired patch clamp data revealed sulphate-dependent increases in ALMT13 current. This could be caused by changes in absolute open probability and/or permeability for sulphate and possibly chloride and links ALMT13 with sulphate-mediated stomatal closure under drought stress. It was then confirmed that ATP affects R-type currents. In contrast to Vicia faba, ATP was identified as a negative regulator of the Arabidopsis thaliana R-type anion channels. The effect of ATP is ambiguous but there is a high probability that it is a result of direct block and phosphorylation. However, the phosphorylation site and place of ATP binding needs further investigation.
The story of the ALMT family, as examined in this thesis, sheds light on the complexity of the stomatal closure process.
Plant stress signalling involves bursts of reactive oxygen species (ROS), which can be mimicked by the application of acute pulses of ozone. Such ozone-pulses inhibit photosynthesis and trigger stomatal closure in a few minutes, but the signalling that underlies these responses remains largely unknown.
We measured changes in Arabidopsis thaliana gas exchange after treatment with acute pulses of ozone and set up a system for simultaneous measurement of membrane potential and cytosolic calcium with the fluorescent reporter R-GECO1.
We show that within 1 min, prior to stomatal closure, O\(_{3}\) triggered a drop in whole-plant CO\(_{2}\) uptake. Within this early phase, O\(_{3}\) pulses (200–1000 ppb) elicited simultaneous membrane depolarization and cytosolic calcium increase, whereas these pulses had no long-term effect on either stomatal conductance or photosynthesis. In contrast, pulses of 5000 ppb O\(_{3}\) induced cell death, systemic Ca\(^{2+}\) signals and an irreversible drop in stomatal conductance and photosynthetic capacity.
We conclude that mesophyll cells respond to ozone in a few seconds by distinct pattern of plasma membrane depolarizations accompanied by an increase in the cytosolic calcium ion (Ca\(^{2+}\)) level. These responses became systemic only at very high ozone concentrations. Thus, plants have rapid mechanism to sense and discriminate the strength of ozone signals.
Electrophilic oxylipins trigger a heat-shock-like response in the absence of heat through the canonical heat-shock transcription factor A1, thereby helping to cope with stresses associated with protein damage.Abiotic and biotic stresses are often characterized by an induction of reactive electrophile species (RES) such as the jasmonate 12-oxo-phytodienoic acid (OPDA) or the structurally related phytoprostanes. Previously, RES oxylipins have been shown massively to induce heat-shock-response (HSR) genes including HSP101 chaperones. Moreover, jasmonates have been reported to play a role in basal thermotolerance. We show that representative HSR marker genes are strongly induced by RES oxylipins through the four master regulator transcription factors HSFA1a, b, d, and e essential for short-term adaptation to heat stress in Arabidopsis. When compared with Arabidopsis seedlings treated at the optimal acclimation temperature of 37 A degrees C, the exogenous application of RES oxylipins at 20 A degrees C induced a much weaker induction of HSP101 at both the gene and protein expression levels which, however, was not sufficient to confer short-term acquired thermotolerance. Moreover, jasmonate-deficient mutant lines displayed a wild-type-like HSR and were not compromised in acquiring thermotolerance. Hence, the OPDA- and RES oxylipin-induced HSR is not sufficient to protect seedlings from severe heat stress but may help plants to cope better with stresses associated with protein unfolding by inducing a battery of chaperones in the absence of heat.
Because of growth and development, plant tissues are characterised by a permanent change in source-sink relations. Tissues with a net carbohydrate export (source) or import (sink) have to adopt their actual demand for assimilates according to the developmental status. Furthermore, plants, as sessile life forms, have developed regulatory mechanisms that enable a flexible response of assimilate partitioning to specific requirements of the habitat, like biotic and abiotic stress factors and changing light conditions. The distribution of assimilates involves specific enzyme functions including sugar transporters and sucrose cleaving enzymes and is regulated by a variety of stimuli. Extracellular invertases cover an essential function in apoplastic phloem unloading and play an important role in regulating source-sink relations. This property is reflected by the occurrence of different invertase isoenzymes with specific expression and regulation patterns that enable a co-ordination of the carbohydrate metabolism in diverse tissues, at different developmental stages, and under varying environmental conditions. Improved knowledge of extracellular invertase function might allow altering growth, development or pathogen resistance of crop plants in a specific way. The present study is aimed at elucidating the regulation patterns and functions of three members of the extracellular invertase gene family of tomato, Lin5, Lin6, and Lin7. Detailed promoter analysis revealed a tissue- and developmental-specific expression of isoenzymes and corresponding regulation patterns. Lin5 shows a developmental regulated expression in fruits. Lin6 is expressed in early developmental stages starting in germinating seeds; in grown up plants Lin6 is solely expressed in pollen and upon wound-stimulation. Lin7 is exclusively expressed in tapetum and pollen tissue. The hormonal regulation of all three isogenes was analysed in detail, whereby known GA- and JA-mediated flower phenotypes could be correlated with invertase functions. In addition, an important role of Lin7 invertase in pollen germination was demonstrated in a functional approach. This is the most profound analysis of extracellular invertases in the delicate process of floral organ development that includes three tomato isoenzymes. In particular, dissection of the individual roles of Lin5, Lin6, and Lin7 reveals novel insights in carbohydrate supply during flower and fruit development. The analysed tissue-specific promoters are profitable tools in plant biotechnology, which in particular applies to the pollen-specific Lin7 promoter. It has been demonstrated that the Lin6 promoter serves as target for hormonal-, sugar-, and wound-mediated signalling pathways. Moreover, a functional interaction of circadian oscillator elements of A. thaliana with the Lin6 promoter and a diurnal rhythm of Lin6 expression have been substantiated. This complex regulation pattern is reflected by the identification of many well-defined cis-acting elements within the Lin6 promoter. This feature supports an integration of various stimuli mediated via extracellular invertase expression resulting in a co-ordinated cellular response to changing internal and external conditions. As sugars on their part induce Lin6 expression, this could result in signal amplification via a positive feedback loop. Furthermore, the extensive appearance and constellation of cisacting elements within the Lin6 promoter provides the basis to answer questions in signal cross-talk and signal integration in plant gene expression. In addition, the Lin6 promoter was successfully used as an inducible expression system. In transgenic tobacco lines an invertase inhibitor was expressed under control of the cytokinin-inducible Lin6 promoter. Thereby, a causal relationship between cytokinin and extracellular invertase for the delay of senescence was demonstrated. This study emphasises the importance of inducible expression systems to address specific questions on a molecular basis. The above-mentioned promoter sequences were obtained via sequential genome walks. Hereby two interesting structural features appeared. First, Lin5 and Lin7 genes are arranged in a direct tandem repeat on the genome. Second, a CACTA-like transposon insertion in intron I of the Lin5 gene was revealed. A primer pair deduced from the transposase region of this transposon allowed the amplification of similar sequences of various Solanaceae species.
Lipasen regulieren die Biosynthese von Jasmonaten, die eine elementare Signalfunktion bei der Entwicklung von Pflanzen und der Abwehr von Pathogenen haben. Entsprechend dem klassischen „Vick-Zimmerman-Pathway“ dienen die aus Galaktolipiden freigesetzten Fettsäuren α-18:3 und 16:3 als Substrate der Jasmonsäure (JA)-Synthese. In den letzen zehn Jahren wurden jedoch die Intermediate der JA-Biosynthese 12-Oxo-Phytodiensäure (OPDA, ausgehend von α-18:3) und Dinor-12-Oxo-Phytodiensäure (dnOPDA, ausgehend von 16:3) verestert in Galaktolipiden der Art Arabidopsis thaliana nachgewiesen. Die Biosynthese und die mögiche Speicherfunktion dieser komplexen, als Arabidopside bezeichneten, Lipide war jedoch noch unklar. In der Literatur wird ein alternativer Syntheseweg postuliert, in dem analog zum klassischen „Vick-Zimmerman-Pathway“ die Biosynthese von veresterter OPDA/dnOPDA ausgehend von veresterter α-18:3/16:3 vollständig in Galaktolipiden der Pastidenmembran stattfindet. Nach Freisetzung von OPDA/dnOPDA durch eine Lipase könnten OPDA/dnOPDA dann als Intermediate in die JA-Biosynthese einfliessen. Sowohl im klassischen „Vick-Zimmerman-Pathway“ als auch im postulierten alternativen Syntheseweg ist die Aktivität von Lipasen von essentieller Bedeutung für die JA-Biosynthese. Für zwei plastidäre sn1-spezifische Acyl-Hydrolasen, DEFECTIVE IN ANTHER DEHISCENCE1 (DAD1) und DONGLE (DGL), wurde eine zentrale Funktion innerhalb der Jasmonat-Biosynthese in Blättern von A. thaliana beschrieben. Dem zufolge ist DGL für die basalen und die frühen wundinduzierten JA-Gehalte und DAD1 für die Aufrechterhaltung der erhöhten JA-Konzentrationen in der späteren Verwundungsantwort verantwortlich. In der vorliegenden Arbeit wiesen drei unabhängige DGL-RNAi-Linien sowie DAD1-Knock-out-Mutanten sowohl unter basalen Bedingungen als auch zu frühen Zeitpunkten nach Verwundung sowie nach Infektion mit dem Bakterienstamm P. syringae DC3000 (avrRPM1) mit dem Wildtyp vergleichbare Konzentrationen an OPDA/JA auf. Dies steht im klaren Widerspruch zu den publizierten Daten. Die Beteiligung von DAD1 an der OPDA/JA-Biosynthese zu späten Zeitpunkten nach Verwundung konnte jedoch bestätigt werden. Ferner konnte eine dramatische Über-Akkumulation von Arabidopsiden in DAD1-defizienten Mutanten nach Verwundung nachgewiesen werden, was auf eine Beteiligung von DAD1 bei der Freisetzung von membrangebundener OPDA/dnOPDA hinweist. Die Analyse der Einzelmutanten 16 weiterer plastidärer Lipasen unter basalen Bedingungen, nach Verwundung und nach Infektion mit P. syringae DC3000 (avrRPM1) zeigte, dass keine der analysierten Mutanten eine essentielle Rolle in der JA-Biosynthese spielt. Jedoch wiesen Mutanten der sn1-spezifischen Lipasen AtPLA1-Iγ1 (At1g06800) signifikant niedrigere Konzentrationen an dnOPDA, OPDA und JA nach Verwundung auf, was eine indirekte Beteiligung an der JA-Biosynthese vermuten lässt. Blattgewebe einer Quadrupel-Mutanten, welche defizient in vier DAD1-ähnlichen Lipasen (AtPLA1-Iβ2, AtPLA1-Iγ1, AtPLA1-Iγ2, AtPLA1-Iγ3) ist, wies nach Verwundung mit der AtPLA1-Iγ1-Mutante vergleichbar niedrige Gehalte an dnOPDA, OPDA sowie JA auf. Da stets in sn2-Position vorliegende 16:3/dnOPDA ebenfalls Substrat der JA-Biosynthese sein kann, müssen zusätzlich zu DAD1 und AtPLA1-Iγ1 noch weitere nicht identifizierte sn1- und sn2-spezifische Acyl-Hydrolasen an der JA-Biosynthese nach Verwundung und Pathogeninfektion beteiligt sein. Dies bedeutet, dass entgegen der in der Literatur vertretenen Meinung, nicht eine sondern mehrere Lipasen in redundanter Weise die Biosynthese von Jasmonaten regulieren. Zur Aufklärung der Biosynthese und möglichen Speicherfunktion der ausschließlich in Arabidopsis vorkommenden Arabidopside wurden A. thaliana Keimlinge mit D5-Linolensäure-Ethylester inkubiert, um eine D5-Markierung der komplexen Lipide zu erzielen. Durch einen anschließenden Stressstimulus mittels Zugabe von Silbernitrat wurde die Jasmonat-Synthese induziert. Die vergleichende Analyse der Markierungsgrade der komplexen Membranlipide MGDG, DGDG, PC sowie der freien OPDA und JA vor und nach Zugabe des Silbernitrats zeigte, eine hohe Übereinstimmung der Markierungsgrade der komplexen Membranlipide 18:3-18:3-MGDG, 18:3-OPDA-MGDG, Arabidopsid B (MGDG-OPDA-OPDA) und Arabidopsid G (OPDA-MGDG-OPDA-OPDA) vor der Silbernitratbehandlung mit denjenigen der durch Silbernitratbehandlung neu gebildeten OPDA/JA. Dagegen wird die hochmarkierte freie Linolensäure nicht direkt zu freier OPDA umgesetzt. Die erhaltenen Ergebnisse zeigen, dass 18:3-OPDA-MGDG, Arabidopsid B und Arabidopsid G direkte Vorstufen von freier OPDA sein können. Damit übereinstimmend konnte gezeigt werden, dass nach Silbernitratstress die Spiege der Vorstufe 18:3-18:3-MGDG abnehmen und zeitgleich die entsprechenden unmittelbaren Metabolite 18:3-OPDA-MGDG, Arabidopsid B und Arabidopsid G akkumulieren.
Stomata sind mikroskopisch kleine Poren in der Blattoberfläche der Landpflanzen, über die das Blattgewebe mit CO2 versorgt wird. Als Schutz vor Austrocknung oder einer Infektion durch Pathogene entwickelte sich ein Mechanismus, um die Porenweite durch Bewegung der sie umgebenden Schließzellen an die Bedürfnisse der Pflanze anzupassen. Ein eng geknüpftes Signalnetzwerk kontrolliert diese Bewegungen und ist in der Lage, externe wie interne Stimuli zu verarbeiten. Der Schließvorgang wird osmotisch durch den Turgorverlust in den Schließzellen angetrieben, der durch den Efflux von Ionen wie K+ ausgelöst wird. In dieser Arbeit wurde die Regulation durch Phosphorylierung des wichtigsten K+-Effluxkanals für den Stomaschluss, GORK, untersucht. Folgende Erkenntnisse wurden durch elektrophysiologische Untersuchungen mit der DEVC-Methode gewonnen: GORK wird durch OST1 auf Ca2+- unabhängige und durch CBL1/9-CIPK5 und CBL1-CIPK23 auf Ca2+-abhängige Weise phosphoryliert und damit aktiviert. CBL1 muss CIPK5 an der Plasmamembran verankern und Ca2+ binden. CIPK5 benötigt ATP und eine Konformationsänderung, um GORK zu phosphorylieren. Im Rahmen dieser Arbeit wurde auch zum ersten Mal gezeigt, dass die PP2CPhosphatase ABI2 direkt mit einem Kanal interagiert und dessen Aktivität hemmt. ABI2 interagiert auch mit den Kinasen OST1, CIPK5 und CIPK23, sodass die Kontrolle der Kanalaktivität auf multiple Weise stattfinden kann. OST1 und ABI2 verbinden die GORKRegulation mit dem ABA-Signalweg. Schließzellen von gork1-2, cbl1/cbl9 und cipk5-2 sind insensitiv auf MeJA, nicht aber auf ABA. Dies stellt eine direkte Verbindung zwischen dem Jasmonatsignalweg und der Ca2+-Signalgebung dar. Im Rahmen dieser Arbeit konnten weitere Hinweise für das komplexe Zusammenspiel der Phytohormone ABA, JA und des Pseudomonas- Effektors Coronatin gefunden werden. Hier konnte zum ersten Mal gezeigt werden, dass Schließzellen je nach Inkubationszeit unterschiedlich auf MeJA und das Phytotoxin Coronatin reagieren. ABA und Coronatin verhalten sich dabei antagonistisch zueinander, wobei der Effekt der Stimuli auf die Stomaweite von der zeitlichen Abfolge der Perzeption abhängt. Der Jasmonat-Signalweg in Schließzellen löst eine geringe ABA-Synthese sowie den Proteinabbau durch das Ubiquitin/26S-Proteasom-System aus und benötigt ABA-Rezeptoren (PYR/PYLs), um einen Stomaschluss einzuleiten. Durch diese Arbeit konnte somit die JA-gesteuerte Regulation des Kaliumefflux-Kanals GORK entschlüsselt sowie einige Unterschiede zwischen den ABA, JA und Coronatin-vermittelten Schließzellbewegungen aufgedeckt werden.